The phase of cell nucleus division following PROMETAPHASE, in which the CHROMOSOMES line up across the equatorial plane of the SPINDLE APPARATUS prior to separation.
In a prokaryotic cell or in the nucleus of a eukaryotic cell, a structure consisting of or containing DNA which carries the genetic information essential to the cell. (From Singleton & Sainsbury, Dictionary of Microbiology and Molecular Biology, 2d ed)
A type of CELL NUCLEUS division by means of which the two daughter nuclei normally receive identical complements of the number of CHROMOSOMES of the somatic cells of the species.
Female germ cells derived from OOGONIA and termed OOCYTES when they enter MEIOSIS. The primary oocytes begin meiosis but are arrested at the diplotene state until OVULATION at PUBERTY to give rise to haploid secondary oocytes or ova (OVUM).
A microtubule structure that forms during CELL DIVISION. It consists of two SPINDLE POLES, and sets of MICROTUBULES that may include the astral microtubules, the polar microtubules, and the kinetochore microtubules.
A type of CELL NUCLEUS division, occurring during maturation of the GERM CELLS. Two successive cell nucleus divisions following a single chromosome duplication (S PHASE) result in daughter cells with half the number of CHROMOSOMES as the parent cells.
The phase of cell nucleus division following METAPHASE, in which the CHROMATIDS separate and migrate to opposite poles of the spindle.
Large multiprotein complexes that bind the centromeres of the chromosomes to the microtubules of the mitotic spindle during metaphase in the cell cycle.
Very long DNA molecules and associated proteins, HISTONES, and non-histone chromosomal proteins (CHROMOSOMAL PROTEINS, NON-HISTONE). Normally 46 chromosomes, including two sex chromosomes are found in the nucleus of human cells. They carry the hereditary information of the individual.
Slender, cylindrical filaments found in the cytoskeleton of plant and animal cells. They are composed of the protein TUBULIN and are influenced by TUBULIN MODULATORS.
Mapping of the KARYOTYPE of a cell.
The interval between two successive CELL DIVISIONS during which the CHROMOSOMES are not individually distinguishable. It is composed of the G phases (G1 PHASE; G0 PHASE; G2 PHASE) and S PHASE (when DNA replication occurs).
The first phase of cell nucleus division, in which the CHROMOSOMES become visible, the CELL NUCLEUS starts to lose its identity, the SPINDLE APPARATUS appears, and the CENTRIOLES migrate toward opposite poles.
The orderly segregation of CHROMOSOMES during MEIOSIS or MITOSIS.
Either of the two longitudinally adjacent threads formed when a eukaryotic chromosome replicates prior to mitosis. The chromatids are held together at the centromere. Sister chromatids are derived from the same chromosome. (Singleton & Sainsbury, Dictionary of Microbiology and Molecular Biology, 2d ed)
The final phase of cell nucleus division following ANAPHASE, in which two daughter nuclei are formed, the CYTOPLASM completes division, and the CHROMOSOMES lose their distinctness and are transformed into CHROMATIN threads.
Cellular proteins encoded by the c-mos genes (GENES, MOS). They function in the cell cycle to maintain MATURATION PROMOTING FACTOR in the active state and have protein-serine/threonine kinase activity. Oncogenic transformation can take place when c-mos proteins are expressed at the wrong time.
The clear constricted portion of the chromosome at which the chromatids are joined and by which the chromosome is attached to the spindle during cell division.
Abnormal number or structure of chromosomes. Chromosome aberrations may result in CHROMOSOME DISORDERS.
A type of IN SITU HYBRIDIZATION in which target sequences are stained with fluorescent dye so their location and size can be determined using fluorescence microscopy. This staining is sufficiently distinct that the hybridization signal can be seen both in metaphase spreads and in interphase nuclei.
Nocodazole is an antineoplastic agent which exerts its effect by depolymerizing microtubules.
A unisexual reproduction without the fusion of a male and a female gamete (FERTILIZATION). In parthenogenesis, an individual is formed from an unfertilized OVUM that did not complete MEIOSIS. Parthenogenesis occurs in nature and can be artificially induced.
Proteins that control the CELL DIVISION CYCLE. This family of proteins includes a wide variety of classes, including CYCLIN-DEPENDENT KINASES, mitogen-activated kinases, CYCLINS, and PHOSPHOPROTEIN PHOSPHATASES as well as their putative substrates such as chromatin-associated proteins, CYTOSKELETAL PROTEINS, and TRANSCRIPTION FACTORS.
Staining of bands, or chromosome segments, allowing the precise identification of individual chromosomes or parts of chromosomes. Applications include the determination of chromosome rearrangements in malformation syndromes and cancer, the chemistry of chromosome segments, chromosome changes during evolution, and, in conjunction with cell hybridization studies, chromosome mapping.
Male germ cells derived from SPERMATOGONIA. The euploid primary spermatocytes undergo MEIOSIS and give rise to the haploid secondary spermatocytes which in turn give rise to SPERMATIDS.
Nucleoproteins, which in contrast to HISTONES, are acid insoluble. They are involved in chromosomal functions; e.g. they bind selectively to DNA, stimulate transcription resulting in tissue-specific RNA synthesis and undergo specific changes in response to various hormones or phytomitogens.
The fusion of a spermatozoon (SPERMATOZOA) with an OVUM thus resulting in the formation of a ZYGOTE.
Protein kinase that drives both the mitotic and meiotic cycles in all eukaryotic organisms. In meiosis it induces immature oocytes to undergo meiotic maturation. In mitosis it has a role in the G2/M phase transition. Once activated by CYCLINS; MPF directly phosphorylates some of the proteins involved in nuclear envelope breakdown, chromosome condensation, spindle assembly, and the degradation of cyclins. The catalytic subunit of MPF is PROTEIN P34CDC2.
Mad2 is a component of the spindle-assembly checkpoint apparatus. It binds to and inhibits the Cdc20 activator subunit of the anaphase-promoting complex, preventing the onset of anaphase until all chromosomes are properly aligned at the metaphase plate. Mad2 is required for proper microtubule capture at KINETOCHORES.
The process of germ cell development in the female from the primordial germ cells through OOGONIA to the mature haploid ova (OVUM).
An alkaloid isolated from Colchicum autumnale L. and used as an antineoplastic.
An assisted reproductive technique that includes the direct handling and manipulation of oocytes and sperm to achieve fertilization in vitro.
The complex series of phenomena, occurring between the end of one CELL DIVISION and the end of the next, by which cellular material is duplicated and then divided between two daughter cells. The cell cycle includes INTERPHASE, which includes G0 PHASE; G1 PHASE; S PHASE; and G2 PHASE, and CELL DIVISION PHASE.
A mature haploid female germ cell extruded from the OVARY at OVULATION.
The phase of cell nucleus division following PROPHASE, when the breakdown of the NUCLEAR ENVELOPE occurs and the MITOTIC SPINDLE APPARATUS enters the nuclear region and attaches to the KINETOCHORES.
A cyclin subtype that is transported into the CELL NUCLEUS at the end of the G2 PHASE. It stimulates the G2/M phase transition by activating CDC2 PROTEIN KINASE.
Within a eukaryotic cell, a membrane-limited body which contains chromosomes and one or more nucleoli (CELL NUCLEOLUS). The nuclear membrane consists of a double unit-type membrane which is perforated by a number of pores; the outermost membrane is continuous with the ENDOPLASMIC RETICULUM. A cell may contain more than one nucleus. (From Singleton & Sainsbury, Dictionary of Microbiology and Molecular Biology, 2d ed)
The chromosomal constitution of cells which deviate from the normal by the addition or subtraction of CHROMOSOMES, chromosome pairs, or chromosome fragments. In a normally diploid cell (DIPLOIDY) the loss of a chromosome pair is termed nullisomy (symbol: 2N-2), the loss of a single chromosome is MONOSOMY (symbol: 2N-1), the addition of a chromosome pair is tetrasomy (symbol: 2N+2), the addition of a single chromosome is TRISOMY (symbol: 2N+1).
Phosphoprotein with protein kinase activity that functions in the G2/M phase transition of the CELL CYCLE. It is the catalytic subunit of the MATURATION-PROMOTING FACTOR and complexes with both CYCLIN A and CYCLIN B in mammalian cells. The maximal activity of cyclin-dependent kinase 1 is achieved when it is fully dephosphorylated.
The fertilized OVUM resulting from the fusion of a male and a female gamete.
A genus of the family Heteromyidae which contains 22 species. Their physiology is adapted for the conservation of water, and they seldom drink water. They are found in arid or desert habitats and travel by hopping on their hind limbs.
A subdiscipline of genetics which deals with the cytological and molecular analysis of the CHROMOSOMES, and location of the GENES on chromosomes, and the movements of chromosomes during the CELL CYCLE.
A microtubule subunit protein found in large quantities in mammalian brain. It has also been isolated from SPERM FLAGELLUM; CILIA; and other sources. Structurally, the protein is a dimer with a molecular weight of approximately 120,000 and a sedimentation coefficient of 5.8S. It binds to COLCHICINE; VINCRISTINE; and VINBLASTINE.
The material of CHROMOSOMES. It is a complex of DNA; HISTONES; and nonhistone proteins (CHROMOSOMAL PROTEINS, NON-HISTONE) found within the nucleus of a cell.
Examination of CHROMOSOMES to diagnose, classify, screen for, or manage genetic diseases and abnormalities. Following preparation of the sample, KARYOTYPING is performed and/or the specific chromosomes are analyzed.
The first continuously cultured human malignant CELL LINE, derived from the cervical carcinoma of Henrietta Lacks. These cells are used for VIRUS CULTIVATION and antitumor drug screening assays.
A family of highly conserved serine-threonine kinases that are involved in the regulation of MITOSIS. They are involved in many aspects of cell division, including centrosome duplication, SPINDLE APPARATUS formation, chromosome alignment, attachment to the spindle, checkpoint activation, and CYTOKINESIS.
The injection of very small amounts of fluid, often with the aid of a microscope and microsyringes.
PHENOTHIAZINES with an amino group at the 3-position that are green crystals or powder. They are used as biological stains.
Complexes of enzymes that catalyze the covalent attachment of UBIQUITIN to other proteins by forming a peptide bond between the C-terminal GLYCINE of UBIQUITIN and the alpha-amino groups of LYSINE residues in the protein. The complexes play an important role in mediating the selective-degradation of short-lived and abnormal proteins. The complex of enzymes can be broken down into three components that involve activation of ubiquitin (UBIQUITIN-ACTIVATING ENZYMES), conjugation of ubiquitin to the ligase complex (UBIQUITIN-CONJUGATING ENZYMES), and ligation of ubiquitin to the substrate protein (UBIQUITIN-PROTEIN LIGASES).
An E3 ubiquitin ligase primarily involved in regulation of the metaphase-to-anaphase transition during MITOSIS through ubiquitination of specific CELL CYCLE PROTEINS. Enzyme activity is tightly regulated through subunits and cofactors, which modulate activation, inhibition, and substrate specificity. The anaphase-promoting complex, or APC-C, is also involved in tissue differentiation in the PLACENTA, CRYSTALLINE LENS, and SKELETAL MUSCLE, and in regulation of postmitotic NEURONAL PLASTICITY and excitability.
A microtubule-associated mechanical adenosine triphosphatase, that uses the energy of ATP hydrolysis to move organelles along microtubules toward the plus end of the microtubule. The protein is found in squid axoplasm, optic lobes, and in bovine brain. Bovine kinesin is a heterotetramer composed of two heavy (120 kDa) and two light (62 kDa) chains. EC 3.6.1.-.
Microscopy of specimens stained with fluorescent dye (usually fluorescein isothiocyanate) or of naturally fluorescent materials, which emit light when exposed to ultraviolet or blue light. Immunofluorescence microscopy utilizes antibodies that are labeled with fluorescent dye.
Interactive processes between the oocyte (OVUM) and the sperm (SPERMATOZOA) including sperm adhesion, ACROSOME REACTION, sperm penetration of the ZONA PELLUCIDA, and events leading to FERTILIZATION.
An aspect of protein kinase (EC 2.7.1.37) in which serine residues in protamines and histones are phosphorylated in the presence of ATP.
The cell center, consisting of a pair of CENTRIOLES surrounded by a cloud of amorphous material called the pericentriolar region. During interphase, the centrosome nucleates microtubule outgrowth. The centrosome duplicates and, during mitosis, separates to form the two poles of the mitotic spindle (MITOTIC SPINDLE APPARATUS).
Securin is involved in the control of the metaphase-anaphase transition during MITOSIS. It promotes the onset of anaphase by blocking SEPARASE function and preventing proteolysis of cohesin and separation of sister CHROMATIDS. Overexpression of securin is associated with NEOPLASTIC CELL TRANSFORMATION and tumor formation.
A technique for visualizing CHROMOSOME ABERRATIONS using fluorescently labeled DNA probes which are hybridized to chromosomal DNA. Multiple fluorochromes may be attached to the probes. Upon hybridization, this produces a multicolored, or painted, effect with a unique color at each site of hybridization. This technique may also be used to identify cross-species homology by labeling probes from one species for hybridization with chromosomes from another species.
Mature male germ cells derived from SPERMATIDS. As spermatids move toward the lumen of the SEMINIFEROUS TUBULES, they undergo extensive structural changes including the loss of cytoplasm, condensation of CHROMATIN into the SPERM HEAD, formation of the ACROSOME cap, the SPERM MIDPIECE and the SPERM TAIL that provides motility.
High molecular weight proteins found in the MICROTUBULES of the cytoskeletal system. Under certain conditions they are required for TUBULIN assembly into the microtubules and stabilize the assembled microtubules.
A family of rat kangaroos found in and around Australia. Genera include Potorous and Bettongia.
The earliest developmental stage of a fertilized ovum (ZYGOTE) during which there are several mitotic divisions within the ZONA PELLUCIDA. Each cleavage or segmentation yields two BLASTOMERES of about half size of the parent cell. This cleavage stage generally covers the period up to 16-cell MORULA.
Methods of implanting a CELL NUCLEUS from a donor cell into an enucleated acceptor cell.
A technique that labels specific sequences in whole chromosomes by in situ DNA chain elongation or PCR (polymerase chain reaction).
A cyclin B subtype that colocalizes with MICROTUBULES during INTERPHASE and is transported into the CELL NUCLEUS at the end of the G2 PHASE.
A major alkaloid from Colchicum autumnale L. and found also in other Colchicum species. Its primary therapeutic use is in the treatment of gout, but it has been used also in the therapy of familial Mediterranean fever (PERIODIC DISEASE).
The prophase of the first division of MEIOSIS (in which homologous CHROMOSOME SEGREGATION occurs). It is divided into five stages: leptonema, zygonema, PACHYNEMA, diplonema, and diakinesis.
A post-MORULA preimplantation mammalian embryo that develops from a 32-cell stage into a fluid-filled hollow ball of over a hundred cells. A blastocyst has two distinctive tissues. The outer layer of trophoblasts gives rise to extra-embryonic tissues. The inner cell mass gives rise to the embryonic disc and eventual embryo proper.
Proteins found in the nucleus of a cell. Do not confuse with NUCLEOPROTEINS which are proteins conjugated with nucleic acids, that are not necessarily present in the nucleus.
The chromosome region which is active in nucleolus formation and which functions in the synthesis of ribosomal RNA.
Echinoderms having bodies of usually five radially disposed arms coalescing at the center.
An aurora kinase that is a component of the chromosomal passenger protein complex and is involved in the regulation of MITOSIS. It mediates proper CHROMOSOME SEGREGATION and contractile ring function during CYTOKINESIS.
Clinical conditions caused by an abnormal chromosome constitution in which there is extra or missing chromosome material (either a whole chromosome or a chromosome segment). (from Thompson et al., Genetics in Medicine, 5th ed, p429)
An exchange of segments between the sister chromatids of a chromosome, either between the sister chromatids of a meiotic tetrad or between the sister chromatids of a duplicated somatic chromosome. Its frequency is increased by ultraviolet and ionizing radiation and other mutagenic agents and is particularly high in BLOOM SYNDROME.
Undifferentiated cells resulting from cleavage of a fertilized egg (ZYGOTE). Inside the intact ZONA PELLUCIDA, each cleavage yields two blastomeres of about half size of the parent cell. Up to the 8-cell stage, all of the blastomeres are totipotent. The 16-cell MORULA contains outer cells and inner cells.
Highly conserved proteins that specifically bind to and activate the anaphase-promoting complex-cyclosome, promoting ubiquitination and proteolysis of cell-cycle-regulatory proteins. Cdc20 is essential for anaphase-promoting complex activity, initiation of anaphase, and cyclin proteolysis during mitosis.
A type of chromosome aberration characterized by CHROMOSOME BREAKAGE and transfer of the broken-off portion to another location, often to a different chromosome.
The cellular signaling system that halts the progression of cells through MITOSIS or MEIOSIS if a defect that will affect CHROMOSOME SEGREGATION is detected.
A group of enzymes that catalyzes the phosphorylation of serine or threonine residues in proteins, with ATP or other nucleotides as phosphate donors.
The part of a cell that contains the CYTOSOL and small structures excluding the CELL NUCLEUS; MITOCHONDRIA; and large VACUOLES. (Glick, Glossary of Biochemistry and Molecular Biology, 1990)
An aquatic genus of the family, Pipidae, occurring in Africa and distinguished by having black horny claws on three inner hind toes.
An assisted fertilization technique consisting of the microinjection of a single viable sperm into an extracted ovum. It is used principally to overcome low sperm count, low sperm motility, inability of sperm to penetrate the egg, or other conditions related to male infertility (INFERTILITY, MALE).
The alignment of CHROMOSOMES at homologous sequences.
Minute cells produced during development of an OOCYTE as it undergoes MEIOSIS. A polar body contains one of the nuclei derived from the first or second meiotic CELL DIVISION. Polar bodies have practically no CYTOPLASM. They are eventually discarded by the oocyte. (from King & Stansfield, A Dictionary of Genetics, 4th ed)
Proteins obtained from various species of Xenopus. Included here are proteins from the African clawed frog (XENOPUS LAEVIS). Many of these proteins have been the subject of scientific investigations in the area of MORPHOGENESIS and development.
The fission of a CELL. It includes CYTOKINESIS, when the CYTOPLASM of a cell is divided, and CELL NUCLEUS DIVISION.
Morphological and physiological development of EMBRYOS.
Cells propagated in vitro in special media conducive to their growth. Cultured cells are used to study developmental, morphologic, metabolic, physiologic, and genetic processes, among others.
The performance of dissections, injections, surgery, etc., by the use of micromanipulators (attachments to a microscope) that manipulate tiny instruments.
Any method used for determining the location of and relative distances between genes on a chromosome.
A broad category of nuclear proteins that are components of or participate in the formation of the NUCLEAR MATRIX.
Complex nucleoprotein structures which contain the genomic DNA and are part of the CELL NUCLEUS of MAMMALS.
The homologous chromosomes that are dissimilar in the heterogametic sex. There are the X CHROMOSOME, the Y CHROMOSOME, and the W, Z chromosomes (in animals in which the female is the heterogametic sex (the silkworm moth Bombyx mori, for example)). In such cases the W chromosome is the female-determining and the male is ZZ. (From King & Stansfield, A Dictionary of Genetics, 4th ed)
Test for tissue antigen using either a direct method, by conjugation of antibody with fluorescent dye (FLUORESCENT ANTIBODY TECHNIQUE, DIRECT) or an indirect method, by formation of antigen-antibody complex which is then labeled with fluorescein-conjugated anti-immunoglobulin antibody (FLUORESCENT ANTIBODY TECHNIQUE, INDIRECT). The tissue is then examined by fluorescence microscopy.
The large, metacentric human chromosomes, called group A in the human chromosome classification. This group consists of chromosome pairs 1, 2, and 3.
Transforming proteins coded by mos oncogenes. The v-mos proteins were originally isolated from the Moloney murine sarcoma virus (Mo-MSV).
Established cell cultures that have the potential to propagate indefinitely.
The full set of CHROMOSOMES presented as a systematized array of METAPHASE chromosomes from a photomicrograph of a single CELL NUCLEUS arranged in pairs in descending order of size and according to the position of the CENTROMERE. (From Stedman, 25th ed)
The medium-sized, acrocentric human chromosomes, called group D in the human chromosome classification. This group consists of chromosome pairs 13, 14, and 15.
The chromosomal constitution of a cell containing multiples of the normal number of CHROMOSOMES; includes triploidy (symbol: 3N), tetraploidy (symbol: 4N), etc.
The process by which the CYTOPLASM of a cell is divided.
A deoxyribonucleotide polymer that is the primary genetic material of all cells. Eukaryotic and prokaryotic organisms normally contain DNA in a double-stranded state, yet several important biological processes transiently involve single-stranded regions. DNA, which consists of a polysugar-phosphate backbone possessing projections of purines (adenine and guanine) and pyrimidines (thymine and cytosine), forms a double helix that is held together by hydrogen bonds between these purines and pyrimidines (adenine to thymine and guanine to cytosine).
Descriptions of specific amino acid, carbohydrate, or nucleotide sequences which have appeared in the published literature and/or are deposited in and maintained by databanks such as GENBANK, European Molecular Biology Laboratory (EMBL), National Biomedical Research Foundation (NBRF), or other sequence repositories.
Susceptibility of chromosomes to breakage leading to translocation; CHROMOSOME INVERSION; SEQUENCE DELETION; or other CHROMOSOME BREAKAGE related aberrations.
The granulosa cells of the cumulus oophorus which surround the OVUM in the GRAAFIAN FOLLICLE. At OVULATION they are extruded with OVUM.
Microscopy using an electron beam, instead of light, to visualize the sample, thereby allowing much greater magnification. The interactions of ELECTRONS with specimens are used to provide information about the fine structure of that specimen. In TRANSMISSION ELECTRON MICROSCOPY the reactions of the electrons that are transmitted through the specimen are imaged. In SCANNING ELECTRON MICROSCOPY an electron beam falls at a non-normal angle on the specimen and the image is derived from the reactions occurring above the plane of the specimen.
The portion of chromosome material that remains condensed and is transcriptionally inactive during INTERPHASE.
The use of silver, usually silver nitrate, as a reagent for producing contrast or coloration in tissue specimens.
Retrovirus-associated DNA sequences (mos) originally isolated from the Moloney murine sarcoma virus (Mo-MSV). The proto-oncogene mos (c-mos) codes for a protein which is a member of the serine kinase family. There is no evidence as yet that human c-mos can become transformed or has a role in human cancer. However, in mice, activation can occur when the retrovirus-like intracisternal A-particle inserts itself near the c-mos sequence. The human c-mos gene is located at 8q22 on the long arm of chromosome 8.
The failure of homologous CHROMOSOMES or CHROMATIDS to segregate during MITOSIS or MEIOSIS with the result that one daughter cell has both of a pair of parental chromosomes or chromatids and the other has none.
The introduction of a phosphoryl group into a compound through the formation of an ester bond between the compound and a phosphorus moiety.
Preservation of cells, tissues, organs, or embryos by freezing. In histological preparations, cryopreservation or cryofixation is used to maintain the existing form, structure, and chemical composition of all the constituent elements of the specimens.
The transfer of mammalian embryos from an in vivo or in vitro environment to a suitable host to improve pregnancy or gestational outcome in human or animal. In human fertility treatment programs, preimplantation embryos ranging from the 4-cell stage to the blastocyst stage are transferred to the uterine cavity between 3-5 days after FERTILIZATION IN VITRO.
Methods used to induce premature oocytes, that are maintained in tissue culture, to progress through developmental stages including to a stage that is competent to undergo FERTILIZATION.
Elements of limited time intervals, contributing to particular results or situations.
A family of multisubunit cytoskeletal motor proteins that use the energy of ATP hydrolysis to power a variety of cellular functions. Dyneins fall into two major classes based upon structural and functional criteria.
Widely used technique which exploits the ability of complementary sequences in single-stranded DNAs or RNAs to pair with each other to form a double helix. Hybridization can take place between two complimentary DNA sequences, between a single-stranded DNA and a complementary RNA, or between two RNA sequences. The technique is used to detect and isolate specific sequences, measure homology, or define other characteristics of one or both strands. (Kendrew, Encyclopedia of Molecular Biology, 1994, p503)
A plant genus of the family POACEAE originating from the savanna of eastern Africa. It is widely grown for livestock forage.
The property of nonisotropic media, such as crystals, whereby a single incident beam of light traverses the medium as two beams, each plane-polarized, the planes being at right angles to each other. (Cline et al., Dictionary of Visual Science, 4th ed)
The developmental entity of a fertilized egg (ZYGOTE) in animal species other than MAMMALS. For chickens, use CHICK EMBRYO.
Small chromosomal proteins (approx 12-20 kD) possessing an open, unfolded structure and attached to the DNA in cell nuclei by ionic linkages. Classification into the various types (designated histone I, histone II, etc.) is based on the relative amounts of arginine and lysine in each.
A subfamily in the family MURIDAE, comprising the hamsters. Four of the more common genera are Cricetus, CRICETULUS; MESOCRICETUS; and PHODOPUS.
A class in the phylum MOLLUSCA comprised of mussels; clams; OYSTERS; COCKLES; and SCALLOPS. They are characterized by a bilaterally symmetrical hinged shell and a muscular foot used for burrowing and anchoring.
A family of Urodela consisting of 15 living genera and about 42 species and occurring in North America, Europe, Asia, and North Africa.
Preparations of cell constituents or subcellular materials, isolates, or substances.
The short, acrocentric human chromosomes, called group G in the human chromosome classification. This group consists of chromosome pairs 21 and 22 and the Y chromosome.
The process by which the CELL NUCLEUS is divided.
Aberrant chromosomes with no ends, i.e., circular.
Any cell, other than a ZYGOTE, that contains elements (such as NUCLEI and CYTOPLASM) from two or more different cells, usually produced by artificial CELL FUSION.
The three-part structure of ribbon-like proteinaceous material that serves to align and join the paired homologous CHROMOSOMES. It is formed during the ZYGOTENE STAGE of the first meiotic division. It is a prerequisite for CROSSING OVER.

Sequential PKC- and Cdc2-mediated phosphorylation events elicit zebrafish nuclear envelope disassembly. (1/1817)

Molecular markers of the zebrafish inner nuclear membrane (NEP55) and nuclear lamina (L68) were identified, partially characterized and used to demonstrate that disassembly of the zebrafish nuclear envelope requires sequential phosphorylation events by first PKC, then Cdc2 kinase. NEP55 and L68 are immunologically and functionally related to human LAP2beta and lamin B, respectively. Exposure of zebrafish nuclei to meiotic cytosol elicits rapid phosphorylation of NEP55 and L68, and disassembly of both proteins. L68 phosphorylation is completely inhibited by simultaneous inhibition of Cdc2 and PKC and only partially blocked by inhibition of either kinase. NEP55 phosphorylation is completely prevented by inhibition or immunodepletion of cytosolic Cdc2. Inhibition of cAMP-dependent kinase, MEK or CaM kinase II does not affect NEP55 or L68 phosphorylation. In vitro, nuclear envelope disassembly requires phosphorylation of NEP55 and L68 by both mammalian PKC and Cdc2. Inhibition of either kinase is sufficient to abolish NE disassembly. Furthermore, novel two-step phosphorylation assays in cytosol and in vitro indicate that PKC-mediated phosphorylation of L68 prior to Cdc2-mediated phosphorylation of L68 and NEP55 is essential to elicit nuclear envelope breakdown. Phosphorylation elicited by Cdc2 prior to PKC prevents nuclear envelope disassembly even though NEP55 is phosphorylated. The results indicate that sequential phosphorylation events elicited by PKC, followed by Cdc2, are required for zebrafish nuclear disassembly. They also argue that phosphorylation of inner nuclear membrane integral proteins is not sufficient to promote nuclear envelope breakdown, and suggest a multiple-level regulation of disassembly of nuclear envelope components during meiosis and at mitosis.  (+info)

Sexual dimorphism in white campion: deletion on the Y chromosome results in a floral asexual phenotype. (2/1817)

White campion is a dioecious plant with heteromorphic X and Y sex chromosomes. In male plants, a filamentous structure replaces the pistil, while in female plants the stamens degenerate early in flower development. Asexual (asx) mutants, cumulating the two developmental defects that characterize the sexual dimorphism in this species, were produced by gamma ray irradiation of pollen and screening in the M1 generation. The mutants harbor a novel type of mutation affecting an early function in sporogenous/parietal cell differentiation within the anther. The function is called stamen-promoting function (SPF). The mutants are shown to result from interstitial deletions on the Y chromosome. We present evidence that such deletions tentatively cover the central domain on the (p)-arm of the Y chromosome (Y2 region). By comparing stamen development in wild-type female and asx mutant flowers we show that they share the same block in anther development, which results in the production of vestigial anthers. The data suggest that the SPF, a key function(s) controlling the sporogenous/parietal specialization in premeiotic anthers, is genuinely missing in females (XX constitution). We argue that this is the earliest function in the male program that is Y-linked and is likely responsible for "male dimorphism" (sexual dimorphism in the third floral whorl) in white campion. More generally, the reported results improve our knowledge of the structural and functional organization of the Y chromosome and favor the view that sex determination in this species results primarily from a trigger signal on the Y chromosome (Y1 region) that suppresses female development. The default state is therefore the ancestral hermaphroditic state.  (+info)

Karyotyping of human oocytes by chromosomal analysis of the second polar bodies. (3/1817)

This paper describes a method for obtaining metaphase chromosomes from human second polar bodies. The second polar body nucleus was injected into the cytoplasm of an enucleated oocyte, which is activated shortly after injection. When the polar body nucleus is transformed into a haploid pronucleus, treatment with okadaic acid was used to induce premature chromosome condensation. A total of 25 analysable chromosome plates were obtained from 38 polar bodies karyotyped using this technique. Whole chromosome painting was used to detect second polar bodies (and respectively, oocytes) with unbalanced translocations. In combination with the first polar body analysis, this technique may be useful in preimplantation genetic diagnosis for patients carrying maternal translocations.  (+info)

Direct imaging of DNA in living cells reveals the dynamics of chromosome formation. (4/1817)

Individual chromosomes are not directly visible within the interphase nuclei of most somatic cells; they can only be seen during mitosis. We have developed a method that allows DNA strands to be observed directly in living cells, and we use it to analyze how mitotic chromosomes form. A fluorescent analogue (e.g., Cy5-dUTP) of the natural precursor, thymidine triphosphate, is introduced into cells, which are then grown on the heated stage of a confocal microscope. The analogue is incorporated by the endogenous enzymes into DNA. As the mechanisms for recognizing and removing the unusual residues do not prevent subsequent progress around the cell cycle, the now fluorescent DNA strands can be followed as they assemble into chromosomes, and segregate to daughters and granddaughters. Movies of such strands in living cells suggest that chromosome axes follow simple recognizable paths through their territories during G2 phase, and that late replicating regions maintain their relative positions as prophase chromosomes form. Quantitative analysis confirms that individual regions move little during this stage of chromosome condensation. As a result, the gross structure of an interphase chromosome territory is directly related to that of the prophase chromosome.  (+info)

Polymorphisms for the size of heterochromatic regions allow sex-independent quantification of post-BMT chimerism targeting metaphase and interphase cells. (5/1817)

BACKGROUND AND OBJECTIVE: Fully quantitative cytological techniques for the analysis of hemopoietic chimerism are very limited and largely restricted to sex-chromosome detection after sex-mismatched bone marrow transplants (BMTs). The aim of the present investigation was to assess the usefulness of autosomal polymorphisms for the size of heterochromatic regions in the identification of donor and recipient cells and therefore in the quantification of the hemopoietic chimerism after sex-matched BMT. DESIGN AND METHODS: Hemopoietic chimerism was followed up in 3 transplanted patients targeting a polymorphism for the size of the pericentromeric heterochromatin (PCH) of chromosome 9, uncovered by restriction endonuclease (RE) in situ digestion (REISD) with the RE Sau3A, to differentiate donor and recipient cells on conventional bone marrow chromosome preparations. RESULTS: The polymorphism for the size of the PCH of chromosome 9 allowed differentiation of donor and recipient cells targeting both metaphase and interphase nuclei. The misidentification error for the polymorphism for the size of HPC of chromosome 9 was estimated as 1% for metaphases and 6-11% for interphases. The 3 cases studied showed complete chimerism in the first post-BMT sample analyzed, which was maintained in 2 of them. One patient relapsed and showed transient mixed chimerism. One month later, this patient achieved a second complete remission, showing complete chimerism again. In this patient, who received a sex-mismatched BMT, chimerism was also quantified by sex-chromosome identification using established methods, such as conventional cytogenetics and FISH, and the results obtained were similar to those rendered by Sau3A-REISD. INTERPRETATION AND CONCLUSIONS: The polymorphism for the size of the PCH of chromosome 9 uncovered by Sau3A-REISD allows accurate quantification of the hemopoietic chimerism after sex-matched BMT.  (+info)

Oocyte quality and treatment outcome in intracytoplasmic sperm injection cycles of polycystic ovarian syndrome patients. (6/1817)

Patients with polycystic ovarian syndrome (PCOS) have higher miscarriage rates. It is postulated that this is caused by a lower rate of mature oocytes, and a lower quality of embryos. Retrospectively we analysed 51 intracytoplasmic sperm injection (ICSI) cycles of 31 PCOS patients. These data were compared to age-matched controls (105 cycles) during the same period. All patients of both groups received gonadotrophin-releasing hormone (GnRH) agonists prior to gonadotrophin treatment. The rate of metaphase II oocytes (MII) was not different. However, the mean absolute number of normally fertilized oocytes was significantly higher in PCOS patients (5.00 versus 3.56, P < 0.01), due to a higher number of oocytes retrieved. More embryos were transferred by cycle in the PCOS group (2.69 versus 2.17, P < 0.05), with a higher cumulative embryo score. The overall and multiple pregnancy rate showed no differences and the clinical abortion rate was lower (21 versus 41.67%, P < 0.05) in the controls. Our findings demonstrate that negative factors unconnected to oocyte morphology must be present in PCOS patients. It is possible that only cytoplasmic, not nuclear, maturity is influenced in these patients.  (+info)

Rapid visualization of metaphase chromosomes in single human blastomeres after fusion with in-vitro matured bovine eggs. (7/1817)

The present study was aimed to facilitate karyotyping of human blastomeres using the metaphase-inducing factors present in unfertilized eggs. A rapid technique for karyotyping would have wide application in the field of preimplantation genetic diagnosis. When cryopreserved in-vitro matured bovine oocytes were fused with human blastomeres, the transferred human nuclei were forced into metaphase within a few hours. Eighty-seven human blastomeres from abnormal or arrested embryos were fused with bovine oocytes in a preclinical study. Fusion efficiency was 100%. In 21 of the hybrid cells, no trace of human chromatin was found. Of the remaining 66, 64 (97%) yielded chromosomes suitable for analysis. The method was used to karyotype embryos from two patients with maternal translocations. One embryo which was judged to be karyotypically normal was replaced in the first patient, resulting in one pregnancy with a normal fetus. None of the second patient's embryos was diagnosed as normal, and hence none was transferred. The results of the present study demonstrated that the ooplasmic factors which induce and maintain metaphase in bovine oocytes can force transferred human blastomere nuclei into premature metaphase, providing the basis for a rapid method of karyotyping blastomeres from preimplantation embryos and, by implication, cells from other sources.  (+info)

Karyotypes on three species of Chinese mesogastropod snails, Semisulcospira libertina, S. dolichostoma and Viviparus rivularis. (8/1817)

Three species of the families Viviparidae and Pleuroceridae, the first intermediate host of paragonimiasis, metagonimiasis and echinostomiasis were studied cytologically. The observed diploid chromosome number was as follows: Semisulcospira libertina 36, S. dolichostoma 34, and Viviparus rivularis 64. The mitotic chromosome complement of S. libertina has nine metacentric pairs and nine submetacentric pairs, and S. dolichostoma has three metacentric pairs and 14 submetacentric pairs of chromosomes. Viviparus rivularis showed two metacentric pairs and 30 submetacentric pairs of chromosomes.  (+info)

Metaphase is a phase in the cell division process (mitosis or meiosis) where the chromosomes align in the middle of the cell, also known as the metaphase plate or equatorial plane. During this stage, each chromosome consists of two sister chromatids attached to each other by a protein complex called the centromere. The spindle fibers from opposite poles of the cell attach to the centromeres of each chromosome, and through a process called congression, they align the chromosomes in the middle of the cell. This alignment allows for accurate segregation of genetic material during the subsequent anaphase stage.

Chromosomes are thread-like structures that exist in the nucleus of cells, carrying genetic information in the form of genes. They are composed of DNA and proteins, and are typically present in pairs in the nucleus, with one set inherited from each parent. In humans, there are 23 pairs of chromosomes for a total of 46 chromosomes. Chromosomes come in different shapes and forms, including sex chromosomes (X and Y) that determine the biological sex of an individual. Changes or abnormalities in the number or structure of chromosomes can lead to genetic disorders and diseases.

Mitosis is a type of cell division in which the genetic material of a single cell, called the mother cell, is equally distributed into two identical daughter cells. It's a fundamental process that occurs in multicellular organisms for growth, maintenance, and repair, as well as in unicellular organisms for reproduction.

The process of mitosis can be broken down into several stages: prophase, prometaphase, metaphase, anaphase, and telophase. During prophase, the chromosomes condense and become visible, and the nuclear envelope breaks down. In prometaphase, the nuclear membrane is completely disassembled, and the mitotic spindle fibers attach to the chromosomes at their centromeres.

During metaphase, the chromosomes align at the metaphase plate, an imaginary line equidistant from the two spindle poles. In anaphase, sister chromatids are pulled apart by the spindle fibers and move toward opposite poles of the cell. Finally, in telophase, new nuclear envelopes form around each set of chromosomes, and the chromosomes decondense and become less visible.

Mitosis is followed by cytokinesis, a process that divides the cytoplasm of the mother cell into two separate daughter cells. The result of mitosis and cytokinesis is two genetically identical cells, each with the same number and kind of chromosomes as the original parent cell.

An oocyte, also known as an egg cell or female gamete, is a large specialized cell found in the ovary of female organisms. It contains half the number of chromosomes as a normal diploid cell, as it is the product of meiotic division. Oocytes are surrounded by follicle cells and are responsible for the production of female offspring upon fertilization with sperm. The term "oocyte" specifically refers to the immature egg cell before it reaches full maturity and is ready for fertilization, at which point it is referred to as an ovum or egg.

The spindle apparatus is a microtubule-based structure that plays a crucial role in the process of cell division, specifically during mitosis and meiosis. It consists of three main components:

1. The spindle poles: These are organized structures composed of microtubules and associated proteins that serve as the anchoring points for the spindle fibers. In animal cells, these poles are typically formed by centrosomes, while in plant cells, they form around nucleation sites called microtubule-organizing centers (MTOCs).
2. The spindle fibers: These are dynamic arrays of microtubules that extend between the two spindle poles. They can be categorized into three types: kinetochore fibers, which connect to the kinetochores on chromosomes; astral fibers, which radiate from the spindle poles and help position the spindle within the cell; and interpolar fibers, which lie between the two spindle poles and contribute to their separation during anaphase.
3. Regulatory proteins: Various motor proteins, such as dynein and kinesin, as well as non-motor proteins like tubulin and septins, are involved in the assembly, maintenance, and dynamics of the spindle apparatus. These proteins help to generate forces that move chromosomes, position the spindle, and ultimately segregate genetic material between two daughter cells during cell division.

The spindle apparatus is essential for ensuring accurate chromosome separation and maintaining genomic stability during cell division. Dysfunction of the spindle apparatus can lead to various abnormalities, including aneuploidy (abnormal number of chromosomes) and chromosomal instability, which have been implicated in several diseases, such as cancer and developmental disorders.

Meiosis is a type of cell division that results in the formation of four daughter cells, each with half the number of chromosomes as the parent cell. It is a key process in sexual reproduction, where it generates gametes or sex cells (sperm and eggs).

The process of meiosis involves one round of DNA replication followed by two successive nuclear divisions, meiosis I and meiosis II. In meiosis I, homologous chromosomes pair, form chiasma and exchange genetic material through crossing over, then separate from each other. In meiosis II, sister chromatids separate, leading to the formation of four haploid cells. This process ensures genetic diversity in offspring by shuffling and recombining genetic information during the formation of gametes.

Anaphase is a stage in the cell division process called mitosis, where sister chromatids (the two copies of each chromosome formed during DNA replication) separate at the centromeres and move toward opposite poles of the cell. This separation is facilitated by the attachment of microtubules from the spindle apparatus to the kinetochores, protein structures located on the centromeres of each sister chromatid. Anaphase is followed by telophase, during which the nuclear membrane reforms around each set of separated chromosomes, and cytokinesis, the division of the cytoplasm to form two separate daughter cells.

Kinetochores are specialized protein structures that form on the centromere region of a chromosome. They play a crucial role in the process of cell division, specifically during mitosis and meiosis. The primary function of kinetochores is to connect the chromosomes to the microtubules of the spindle apparatus, which is responsible for separating the sister chromatids during cell division. Through this connection, kinetochores facilitate the movement of chromosomes towards opposite poles of the cell during anaphase, ensuring equal distribution of genetic material to each resulting daughter cell.

Chromosomes are thread-like structures that contain genetic material, i.e., DNA and proteins, present in the nucleus of human cells. In humans, there are 23 pairs of chromosomes, for a total of 46 chromosomes, in each diploid cell. Twenty-two of these pairs are called autosomal chromosomes, which come in identical pairs and contain genes that determine various traits unrelated to sex.

The last pair is referred to as the sex chromosomes (X and Y), which determines a person's biological sex. Females have two X chromosomes (46, XX), while males possess one X and one Y chromosome (46, XY). Chromosomes vary in size, with the largest being chromosome 1 and the smallest being the Y chromosome.

Human chromosomes are typically visualized during mitosis or meiosis using staining techniques that highlight their banding patterns, allowing for identification of specific regions and genes. Chromosomal abnormalities can lead to various genetic disorders, including Down syndrome (trisomy 21), Turner syndrome (monosomy X), and Klinefelter syndrome (XXY).

Microtubules are hollow, cylindrical structures composed of tubulin proteins in the cytoskeleton of eukaryotic cells. They play crucial roles in various cellular processes such as maintaining cell shape, intracellular transport, and cell division (mitosis and meiosis). Microtubules are dynamic, undergoing continuous assembly and disassembly, which allows them to rapidly reorganize in response to cellular needs. They also form part of important cellular structures like centrioles, basal bodies, and cilia/flagella.

Karyotyping is a medical laboratory test used to study the chromosomes in a cell. It involves obtaining a sample of cells from a patient, usually from blood or bone marrow, and then staining the chromosomes so they can be easily seen under a microscope. The chromosomes are then arranged in pairs based on their size, shape, and other features to create a karyotype. This visual representation allows for the identification and analysis of any chromosomal abnormalities, such as extra or missing chromosomes, or structural changes like translocations or inversions. These abnormalities can provide important information about genetic disorders, diseases, and developmental problems.

Interphase is a phase in the cell cycle during which the cell primarily performs its functions of growth and DNA replication. It is the longest phase of the cell cycle, consisting of G1 phase (during which the cell grows and prepares for DNA replication), S phase (during which DNA replication occurs), and G2 phase (during which the cell grows further and prepares for mitosis). During interphase, the chromosomes are in their relaxed, extended form and are not visible under the microscope. Interphase is followed by mitosis, during which the chromosomes condense and separate to form two genetically identical daughter cells.

Prophase is the first phase of mitosis, the process by which eukaryotic cells divide and reproduce. During prophase, the chromosomes condense and become visible. The nuclear envelope breaks down, allowing the spindle fibers to attach to the centromeres of each chromatid in the chromosome. This is a critical step in preparing for the separation of genetic material during cell division. Prophase is also marked by the movement of the centrosomes to opposite poles of the cell, forming the mitotic spindle.

Chromosome segregation is the process that occurs during cell division (mitosis or meiosis) where replicated chromosomes are separated and distributed equally into two daughter cells. Each chromosome consists of two sister chromatids, which are identical copies of genetic material. During chromosome segregation, these sister chromatids are pulled apart by a structure called the mitotic spindle and moved to opposite poles of the cell. This ensures that each new cell receives one copy of each chromosome, preserving the correct number and composition of chromosomes in the organism.

Chromatids are defined as the individual strands that make up a duplicated chromosome. They are formed during the S phase of the cell cycle, when replication occurs and each chromosome is copied, resulting in two identical sister chromatids. These chromatids are connected at a region called the centromere and are held together by cohesin protein complexes until they are separated during mitosis or meiosis.

During mitosis, the sister chromatids are pulled apart by the mitotic spindle apparatus and distributed equally to each daughter cell. In meiosis, which is a type of cell division that occurs in the production of gametes (sex cells), homologous chromosomes pair up and exchange genetic material through a process called crossing over. After crossing over, each homologous chromosome consists of two recombinant chromatids that are separated during meiosis I, and then sister chromatids are separated during meiosis II.

Chromatids play an essential role in the faithful transmission of genetic information from one generation to the next, ensuring that each daughter cell or gamete receives a complete set of chromosomes with intact and functional genes.

Telophase is a phase in the cell division process (mitosis or meiosis) where the chromosomes reach their most condensed form and move to the poles of the cell. The nuclear membrane begins to reform around each set of chromosomes, and the spindle fibers that were used to separate the chromosomes break down. This phase is followed by cytokinesis, where the cytoplasm of the cell divides, resulting in two separate daughter cells. In telophase I of meiosis, crossing over between homologous chromosomes has already occurred during prophase I and sister chromatids remain together until anaphase II.

Proto-oncogene proteins c-mos are a type of serine/threonine protein kinase that play crucial roles in cell cycle regulation, particularly during the G2 phase and the transition to mitosis. The c-mos gene is a normal version of an oncogene, which can become cancer-causing when mutated or overexpressed. In its normal form, the c-mos protein is involved in controlling the progression of the cell cycle, meiosis, and also has been implicated in neuronal development and synaptic plasticity. Dysregulation of c-mos proto-oncogene proteins can contribute to tumorigenesis and cancer development.

A centromere is a specialized region found on chromosomes that plays a crucial role in the separation of replicated chromosomes during cell division. It is the point where the sister chromatids (the two copies of a chromosome formed during DNA replication) are joined together. The centromere contains highly repeated DNA sequences and proteins that form a complex structure known as the kinetochore, which serves as an attachment site for microtubules of the mitotic spindle during cell division.

During mitosis or meiosis, the kinetochore facilitates the movement of chromosomes by interacting with the microtubules, allowing for the accurate distribution of genetic material to the daughter cells. Centromeres can vary in their position and structure among different species, ranging from being located near the middle of the chromosome (metacentric) to being positioned closer to one end (acrocentric). The precise location and characteristics of centromeres are essential for proper chromosome segregation and maintenance of genomic stability.

Chromosome aberrations refer to structural and numerical changes in the chromosomes that can occur spontaneously or as a result of exposure to mutagenic agents. These changes can affect the genetic material encoded in the chromosomes, leading to various consequences such as developmental abnormalities, cancer, or infertility.

Structural aberrations include deletions, duplications, inversions, translocations, and rings, which result from breaks and rearrangements of chromosome segments. Numerical aberrations involve changes in the number of chromosomes, such as aneuploidy (extra or missing chromosomes) or polyploidy (multiples of a complete set of chromosomes).

Chromosome aberrations can be detected and analyzed using various cytogenetic techniques, including karyotyping, fluorescence in situ hybridization (FISH), and comparative genomic hybridization (CGH). These methods allow for the identification and characterization of chromosomal changes at the molecular level, providing valuable information for genetic counseling, diagnosis, and research.

In situ hybridization, fluorescence (FISH) is a type of molecular cytogenetic technique used to detect and localize the presence or absence of specific DNA sequences on chromosomes through the use of fluorescent probes. This technique allows for the direct visualization of genetic material at a cellular level, making it possible to identify chromosomal abnormalities such as deletions, duplications, translocations, and other rearrangements.

The process involves denaturing the DNA in the sample to separate the double-stranded molecules into single strands, then adding fluorescently labeled probes that are complementary to the target DNA sequence. The probe hybridizes to the complementary sequence in the sample, and the location of the probe is detected by fluorescence microscopy.

FISH has a wide range of applications in both clinical and research settings, including prenatal diagnosis, cancer diagnosis and monitoring, and the study of gene expression and regulation. It is a powerful tool for identifying genetic abnormalities and understanding their role in human disease.

Nocodazole is not a medical condition or disease, but rather a pharmacological agent used in medical research and clinical settings. It's a synthetic chemical compound that belongs to the class of drugs known as microtubule inhibitors. Nocodazole works by binding to and disrupting the dynamic assembly and disassembly of microtubules, which are important components of the cell's cytoskeleton and play a critical role in cell division.

Nocodazole is primarily used in research settings as a tool for studying cell biology and mitosis, the process by which cells divide. It can be used to synchronize cells in the cell cycle or to induce mitotic arrest, making it useful for investigating various aspects of cell division and chromosome behavior.

In clinical settings, nocodazole has been used off-label as a component of some cancer treatment regimens, particularly in combination with other chemotherapeutic agents. Its ability to disrupt microtubules can interfere with the proliferation of cancer cells and enhance the effectiveness of certain anti-cancer drugs. However, its use is not widespread due to potential side effects and the availability of alternative treatments.

Parthenogenesis is a form of asexual reproduction in which offspring develop from unfertilized eggs or ovums. It occurs naturally in some plant and insect species, as well as a few vertebrates such as reptiles and fish. Parthenogenesis does not involve the fusion of sperm and egg cells; instead, the development of offspring is initiated by some other trigger, such as a chemical or physical stimulus. This type of reproduction results in offspring that are genetically identical to the parent organism. In humans and other mammals, parthenogenesis is not a natural occurrence and would require scientific intervention to induce.

Cell cycle proteins are a group of regulatory proteins that control the progression of the cell cycle, which is the series of events that take place in a eukaryotic cell leading to its division and duplication. These proteins can be classified into several categories based on their functions during different stages of the cell cycle.

The major groups of cell cycle proteins include:

1. Cyclin-dependent kinases (CDKs): CDKs are serine/threonine protein kinases that regulate key transitions in the cell cycle. They require binding to a regulatory subunit called cyclin to become active. Different CDK-cyclin complexes are activated at different stages of the cell cycle.
2. Cyclins: Cyclins are a family of regulatory proteins that bind and activate CDKs. Their levels fluctuate throughout the cell cycle, with specific cyclins expressed during particular phases. For example, cyclin D is important for the G1 to S phase transition, while cyclin B is required for the G2 to M phase transition.
3. CDK inhibitors (CKIs): CKIs are regulatory proteins that bind to and inhibit CDKs, thereby preventing their activation. CKIs can be divided into two main families: the INK4 family and the Cip/Kip family. INK4 family members specifically inhibit CDK4 and CDK6, while Cip/Kip family members inhibit a broader range of CDKs.
4. Anaphase-promoting complex/cyclosome (APC/C): APC/C is an E3 ubiquitin ligase that targets specific proteins for degradation by the 26S proteasome. During the cell cycle, APC/C regulates the metaphase to anaphase transition and the exit from mitosis by targeting securin and cyclin B for degradation.
5. Other regulatory proteins: Several other proteins play crucial roles in regulating the cell cycle, such as p53, a transcription factor that responds to DNA damage and arrests the cell cycle, and the polo-like kinases (PLKs), which are involved in various aspects of mitosis.

Overall, cell cycle proteins work together to ensure the proper progression of the cell cycle, maintain genomic stability, and prevent uncontrolled cell growth, which can lead to cancer.

Chromosome banding is a technique used in cytogenetics to identify and describe the physical structure and organization of chromosomes. This method involves staining the chromosomes with specific dyes that bind differently to the DNA and proteins in various regions of the chromosome, resulting in a distinct pattern of light and dark bands when viewed under a microscope.

The most commonly used banding techniques are G-banding (Giemsa banding) and R-banding (reverse banding). In G-banding, the chromosomes are stained with Giemsa dye, which preferentially binds to the AT-rich regions, creating a characteristic banding pattern. The bands are numbered from the centromere (the constriction point where the chromatids join) outwards, with the darker bands (rich in A-T base pairs and histone proteins) labeled as "q" arms and the lighter bands (rich in G-C base pairs and arginine-rich proteins) labeled as "p" arms.

R-banding, on the other hand, uses a different staining procedure that results in a reversed banding pattern compared to G-banding. The darker R-bands correspond to the lighter G-bands, and vice versa. This technique is particularly useful for identifying and analyzing specific regions of chromosomes that may be difficult to visualize with G-banding alone.

Chromosome banding plays a crucial role in diagnosing genetic disorders, identifying chromosomal abnormalities, and studying the structure and function of chromosomes in both clinical and research settings.

Spermatocytes are a type of cell that is involved in the process of spermatogenesis, which is the formation of sperm in the testes. Specifically, spermatocytes are the cells that undergo meiosis, a special type of cell division that results in the production of four haploid daughter cells, each containing half the number of chromosomes as the parent cell.

There are two types of spermatocytes: primary and secondary. Primary spermatocytes are diploid cells that contain 46 chromosomes (23 pairs). During meiosis I, these cells undergo a process called crossing over, in which genetic material is exchanged between homologous chromosomes. After crossing over, the primary spermatocytes divide into two secondary spermatocytes, each containing 23 chromosomes (but still with 23 pairs).

Secondary spermatocytes then undergo meiosis II, which results in the formation of four haploid spermatids. Each spermatid contains 23 single chromosomes and will eventually develop into a mature sperm cell through a process called spermiogenesis.

It's worth noting that spermatocytes are only found in males, as they are specific to the male reproductive system.

Chromosomal proteins, non-histone, are a diverse group of proteins that are associated with chromatin, the complex of DNA and histone proteins, but do not have the characteristic structure of histones. These proteins play important roles in various nuclear processes such as DNA replication, transcription, repair, recombination, and chromosome condensation and segregation during cell division. They can be broadly classified into several categories based on their functions, including architectural proteins, enzymes, transcription factors, and structural proteins. Examples of non-histone chromosomal proteins include high mobility group (HMG) proteins, poly(ADP-ribose) polymerases (PARPs), and condensins.

Fertilization is the process by which a sperm cell (spermatozoon) penetrates and fuses with an egg cell (ovum), resulting in the formation of a zygote. This fusion of genetic material from both the male and female gametes initiates the development of a new organism. In human biology, fertilization typically occurs in the fallopian tube after sexual intercourse, when a single sperm out of millions is able to reach and penetrate the egg released from the ovary during ovulation. The successful fusion of these two gametes marks the beginning of pregnancy.

Maturation-Promoting Factor (MPF) is not a medical term per se, but it is commonly used in the field of cell biology and cancer research. MPF refers to a complex of two proteins that play a crucial role in regulating the cell cycle, specifically during the transition from the G2 phase to mitosis (M phase).

MPF is composed of a cyclin-dependent kinase (CDK1) and a regulatory subunit called cyclin B. During the late G2 phase, the levels of cyclin B increase, which leads to the activation of CDK1. Once activated, MPF triggers a series of events that promote mitosis, including chromosome condensation, nuclear envelope breakdown, and spindle formation.

In summary, Maturation-Promoting Factor (MPF) is a protein complex made up of CDK1 and cyclin B, which regulates the transition from the G2 phase to mitosis during the cell cycle.

The Mad2 (Mitotic Arrest Deficient 2) proteins are a part of the spindle assembly checkpoint (SAC), which is a crucial surveillance mechanism that ensures accurate chromosome segregation during cell division. The primary function of Mad2 proteins is to prevent the onset of anaphase until all chromosomes have achieved proper attachment and tension on the mitotic spindle.

Mad2 proteins exist in two major conformational states: open (O-Mad2) and closed (C-Mad2). The transition between these two forms plays a critical role in the regulation of the SAC. In response to unattached kinetochores, Mad2 proteins bind to and inhibit the anaphase-promoting complex/cyclosome (APC/C), thereby preventing premature chromosome separation.

There are two main isoforms of Mad2 in humans: Mad2L1 (Mad2A) and Mad2L2 (Mad2B). While both isoforms share similar functions, they exhibit distinct biochemical properties and interact with other SAC components differently. Dysregulation of the Mad2 proteins has been implicated in various diseases, including cancer and neurological disorders.

Oogenesis is the biological process of formation and maturation of female gametes, or ova or egg cells, in the ovary. It begins during fetal development and continues throughout a woman's reproductive years. The process involves the division and differentiation of a germ cell (oogonium) into an immature ovum (oocyte), which then undergoes meiotic division to form a mature ovum capable of being fertilized by sperm.

The main steps in oogenesis include:

1. Multiplication phase: The oogonia divide mitotically to increase their number.
2. Growth phase: One of the oogonia becomes primary oocyte and starts to grow, accumulating nutrients and organelles required for future development.
3. First meiotic division: The primary oocyte undergoes an incomplete first meiotic division, resulting in two haploid cells - a secondary oocyte and a smaller cell called the first polar body. This division is arrested in prophase I until puberty.
4. Second meiotic division: At ovulation or just before fertilization, the secondary oocyte completes the second meiotic division, producing another small cell, the second polar body, and a mature ovum (egg) with 23 chromosomes.
5. Fertilization: The mature ovum can be fertilized by a sperm, restoring the normal diploid number of chromosomes in the resulting zygote.

Oogenesis is a complex and highly regulated process that involves various hormonal signals and cellular interactions to ensure proper development and maturation of female gametes for successful reproduction.

Demecolcine is a medication that belongs to the class of drugs called anticholinergics. It is derived from the plant alkaloid colchicine and has been used in medical research for its ability to arrest cells in metaphase, a specific stage of cell division. This property makes demecolcine useful in various laboratory procedures such as chromosome analysis and the production of cultured cell lines.

In clinical settings, demecolcine is not commonly used due to its narrow therapeutic index and potential for toxicity. However, it has been used off-label in some cases to treat conditions associated with uncontrolled cell division, such as certain types of cancer. Its use in these situations is typically reserved for when other treatments have failed or are not well tolerated.

It's important to note that demecolcine should only be administered under the close supervision of a healthcare professional and its use is generally avoided in pregnant women due to the risk of fetal harm.

Fertilization in vitro, also known as in-vitro fertilization (IVF), is a medical procedure where an egg (oocyte) and sperm are combined in a laboratory dish to facilitate fertilization. The fertilized egg (embryo) is then transferred to a uterus with the hope of establishing a successful pregnancy. This procedure is often used when other assisted reproductive technologies have been unsuccessful or are not applicable, such as in cases of blocked fallopian tubes, severe male factor infertility, and unexplained infertility. The process involves ovarian stimulation, egg retrieval, fertilization, embryo culture, and embryo transfer. In some cases, additional techniques such as intracytoplasmic sperm injection (ICSI) or preimplantation genetic testing (PGT) may be used to increase the chances of success.

The cell cycle is a series of events that take place in a cell leading to its division and duplication. It consists of four main phases: G1 phase, S phase, G2 phase, and M phase.

During the G1 phase, the cell grows in size and synthesizes mRNA and proteins in preparation for DNA replication. In the S phase, the cell's DNA is copied, resulting in two complete sets of chromosomes. During the G2 phase, the cell continues to grow and produces more proteins and organelles necessary for cell division.

The M phase is the final stage of the cell cycle and consists of mitosis (nuclear division) and cytokinesis (cytoplasmic division). Mitosis results in two genetically identical daughter nuclei, while cytokinesis divides the cytoplasm and creates two separate daughter cells.

The cell cycle is regulated by various checkpoints that ensure the proper completion of each phase before progressing to the next. These checkpoints help prevent errors in DNA replication and division, which can lead to mutations and cancer.

An ovum is the female reproductive cell, or gamete, produced in the ovaries. It is also known as an egg cell and is released from the ovary during ovulation. When fertilized by a sperm, it becomes a zygote, which can develop into a fetus. The ovum contains half the genetic material necessary to create a new individual.

Prometaphase is a stage in the cell division process called mitosis, where the nuclear membrane has broken down and the chromosomes are now moved into the center of the cell, also known as the metaphase plate. This movement is facilitated by the mitotic spindle, which attaches to specialized structures on the chromosomes called kinetochores. The prometaphase stage follows prophase and precedes metaphase in the mitosis process. It's characterized by the beginning of chromosome separation and the reorganization of the cell for the upcoming division into two daughter cells.

Cyclin B is a type of cyclin protein that regulates the cell cycle, specifically the transition from G2 phase to mitosis (M phase) in eukaryotic cells. Cyclin B binds and activates cyclin-dependent kinase 1 (CDK1), forming the complex known as M-phase promoting factor (MPF). This complex triggers the events leading to cell division, such as chromosome condensation, nuclear envelope breakdown, and spindle formation. The levels of cyclin B increase during the G2 phase and are degraded by the anaphase-promoting complex/cyclosome (APC/C) at the onset of anaphase, allowing the cell cycle to progress into the next phase.

The cell nucleus is a membrane-bound organelle found in the eukaryotic cells (cells with a true nucleus). It contains most of the cell's genetic material, organized as DNA molecules in complex with proteins, RNA molecules, and histones to form chromosomes.

The primary function of the cell nucleus is to regulate and control the activities of the cell, including growth, metabolism, protein synthesis, and reproduction. It also plays a crucial role in the process of mitosis (cell division) by separating and protecting the genetic material during this process. The nuclear membrane, or nuclear envelope, surrounding the nucleus is composed of two lipid bilayers with numerous pores that allow for the selective transport of molecules between the nucleoplasm (nucleus interior) and the cytoplasm (cell exterior).

The cell nucleus is a vital structure in eukaryotic cells, and its dysfunction can lead to various diseases, including cancer and genetic disorders.

Aneuploidy is a medical term that refers to an abnormal number of chromosomes in a cell. Chromosomes are thread-like structures located inside the nucleus of cells that contain genetic information in the form of genes.

In humans, the normal number of chromosomes in a cell is 46, arranged in 23 pairs. Aneuploidy occurs when there is an extra or missing chromosome in one or more of these pairs. For example, Down syndrome is a condition that results from an extra copy of chromosome 21, also known as trisomy 21.

Aneuploidy can arise during the formation of gametes (sperm or egg cells) due to errors in the process of cell division called meiosis. These errors can result in eggs or sperm with an abnormal number of chromosomes, which can then lead to aneuploidy in the resulting embryo.

Aneuploidy is a significant cause of birth defects and miscarriages. The severity of the condition depends on which chromosomes are affected and the extent of the abnormality. In some cases, aneuploidy may have no noticeable effects, while in others it can lead to serious health problems or developmental delays.

CDC2 protein kinase, also known as cell division cycle 2 or CDK1, is a type of enzyme that plays a crucial role in the regulation of the cell cycle. The cell cycle is the series of events that cells undergo as they grow, replicate their DNA, and divide into two daughter cells.

CDC2 protein kinase is a member of the cyclin-dependent kinase (CDK) family, which are serine/threonine protein kinases that are activated by binding to regulatory subunits called cyclins. CDC2 protein kinase is primarily associated with the regulation of the G2 phase and the entry into mitosis, the stage of the cell cycle where nuclear and cytoplasmic division occur.

CDC2 protein kinase functions by phosphorylating various target proteins, which alters their activity and contributes to the coordination of the different events that occur during the cell cycle. The activity of CDC2 protein kinase is tightly regulated through a variety of mechanisms, including phosphorylation and dephosphorylation, as well as the binding and destruction of cyclin subunits.

Dysregulation of CDC2 protein kinase has been implicated in various human diseases, including cancer, where uncontrolled cell division can lead to the formation of tumors. Therefore, understanding the regulation and function of CDC2 protein kinase is an important area of research in molecular biology and medicine.

A zygote is the initial cell formed when a sperm fertilizes an egg, also known as an oocyte. This occurs in the process of human reproduction and marks the beginning of a new genetic identity, containing 46 chromosomes - 23 from the sperm and 23 from the egg. The zygote starts the journey of cell division and growth, eventually developing into a blastocyst, then an embryo, and finally a fetus over the course of pregnancy.

'Dipodomys' is the genus name for kangaroo rats, which are small rodents native to North America. They are called kangaroo rats due to their powerful hind legs and long tails, which they use to hop around like kangaroos. Kangaroo rats are known for their ability to survive in arid environments, as they are able to obtain moisture from the seeds they eat and can concentrate their urine to conserve water. They are also famous for their highly specialized kidneys, which allow them to produce extremely dry urine.

Cytogenetics is a branch of genetics that deals with the study of chromosomes and their structure, function, and abnormalities. It involves the examination of chromosome number and structure in the cells of an organism, usually through microscopic analysis of chromosomes prepared from cell cultures or tissue samples. Cytogenetic techniques can be used to identify chromosomal abnormalities associated with genetic disorders, cancer, and other diseases.

The process of cytogenetics typically involves staining the chromosomes to make them visible under a microscope, and then analyzing their number, size, shape, and banding pattern. Chromosomal abnormalities such as deletions, duplications, inversions, translocations, and aneuploidy (abnormal number of chromosomes) can be detected through cytogenetic analysis.

Cytogenetics is an important tool in medical genetics and has many clinical applications, including prenatal diagnosis, cancer diagnosis and monitoring, and identification of genetic disorders. Advances in molecular cytogenetic techniques, such as fluorescence in situ hybridization (FISH) and comparative genomic hybridization (CGH), have improved the resolution and accuracy of chromosome analysis and expanded its clinical applications.

Tubulin is a type of protein that forms microtubules, which are hollow cylindrical structures involved in the cell's cytoskeleton. These structures play important roles in various cellular processes, including maintaining cell shape, cell division, and intracellular transport. There are two main types of tubulin proteins: alpha-tubulin and beta-tubulin. They polymerize to form heterodimers, which then assemble into microtubules. The assembly and disassembly of microtubules are dynamic processes that are regulated by various factors, including GTP hydrolysis, motor proteins, and microtubule-associated proteins (MAPs). Tubulin is an essential component of the eukaryotic cell and has been a target for anti-cancer drugs such as taxanes and vinca alkaloids.

Chromatin is the complex of DNA, RNA, and proteins that make up the chromosomes in the nucleus of a cell. It is responsible for packaging the long DNA molecules into a more compact form that fits within the nucleus. Chromatin is made up of repeating units called nucleosomes, which consist of a histone protein octamer wrapped tightly by DNA. The structure of chromatin can be altered through chemical modifications to the histone proteins and DNA, which can influence gene expression and other cellular processes.

Cytogenetic analysis is a laboratory technique used to identify and study the structure and function of chromosomes, which are the structures in the cell that contain genetic material. This type of analysis involves examining the number, size, shape, and banding pattern of chromosomes in cells, typically during metaphase when they are at their most condensed state.

There are several methods used for cytogenetic analysis, including karyotyping, fluorescence in situ hybridization (FISH), and comparative genomic hybridization (CGH). Karyotyping involves staining the chromosomes with a dye to visualize their banding patterns and then arranging them in pairs based on their size and shape. FISH uses fluorescent probes to label specific DNA sequences, allowing for the detection of genetic abnormalities such as deletions, duplications, or translocations. CGH compares the DNA content of two samples to identify differences in copy number, which can be used to detect chromosomal imbalances.

Cytogenetic analysis is an important tool in medical genetics and is used for a variety of purposes, including prenatal diagnosis, cancer diagnosis and monitoring, and the identification of genetic disorders.

HeLa cells are a type of immortalized cell line used in scientific research. They are derived from a cancer that developed in the cervical tissue of Henrietta Lacks, an African-American woman, in 1951. After her death, cells taken from her tumor were found to be capable of continuous division and growth in a laboratory setting, making them an invaluable resource for medical research.

HeLa cells have been used in a wide range of scientific studies, including research on cancer, viruses, genetics, and drug development. They were the first human cell line to be successfully cloned and are able to grow rapidly in culture, doubling their population every 20-24 hours. This has made them an essential tool for many areas of biomedical research.

It is important to note that while HeLa cells have been instrumental in numerous scientific breakthroughs, the story of their origin raises ethical questions about informed consent and the use of human tissue in research.

Aurora kinases are a family of serine/threonine protein kinases that play crucial roles in the regulation of cell division. There are three members of the Aurora kinase family, designated as Aurora A, Aurora B, and Aurora C. These kinases are involved in the proper separation of chromosomes during mitosis and meiosis, and their dysregulation has been implicated in various types of cancer.

Aurora A is primarily located at the centrosomes and spindle poles during cell division, where it regulates centrosome maturation, bipolar spindle formation, and chromosome segregation. Aurora B, on the other hand, is a component of the chromosomal passenger complex (CPC) that localizes to the centromeres during prophase and moves to the spindle midzone during anaphase. It plays essential roles in kinetochore-microtubule attachment, chromosome alignment, and cytokinesis. Aurora C is most similar to Aurora B and appears to have overlapping functions with it, although its specific roles are less well understood.

Dysregulation of Aurora kinases has been associated with various types of cancer, including breast, ovarian, colon, and lung cancers. Overexpression or amplification of Aurora A is observed in many cancers, leading to chromosomal instability and aneuploidy. Inhibition of Aurora kinases has emerged as a potential therapeutic strategy for cancer treatment, with several small molecule inhibitors currently under investigation in clinical trials.

Microinjection is a medical technique that involves the use of a fine, precise needle to inject small amounts of liquid or chemicals into microscopic structures, cells, or tissues. This procedure is often used in research settings to introduce specific substances into individual cells for study purposes, such as introducing DNA or RNA into cell nuclei to manipulate gene expression.

In clinical settings, microinjections may be used in various medical and cosmetic procedures, including:

1. Intracytoplasmic Sperm Injection (ICSI): A type of assisted reproductive technology where a single sperm is injected directly into an egg to increase the chances of fertilization during in vitro fertilization (IVF) treatments.
2. Botulinum Toxin Injections: Microinjections of botulinum toxin (Botox, Dysport, or Xeomin) are used for cosmetic purposes to reduce wrinkles and fine lines by temporarily paralyzing the muscles responsible for their formation. They can also be used medically to treat various neuromuscular disorders, such as migraines, muscle spasticity, and excessive sweating (hyperhidrosis).
3. Drug Delivery: Microinjections may be used to deliver drugs directly into specific tissues or organs, bypassing the systemic circulation and potentially reducing side effects. This technique can be particularly useful in treating localized pain, delivering growth factors for tissue regeneration, or administering chemotherapy agents directly into tumors.
4. Gene Therapy: Microinjections of genetic material (DNA or RNA) can be used to introduce therapeutic genes into cells to treat various genetic disorders or diseases, such as cystic fibrosis, hemophilia, or cancer.

Overall, microinjection is a highly specialized and precise technique that allows for the targeted delivery of substances into small structures, cells, or tissues, with potential applications in research, medical diagnostics, and therapeutic interventions.

'Azure stains' is a term used in pathology to describe a histological staining technique that uses a type of dye called methyl blue, which turns the stained structures a blue-purple color. This technique is often used to stain acid mucins, which are found in various types of tissues and can be indicative of certain medical conditions.

In particular, azure stains are sometimes used to help diagnose certain types of cancer, such as mucoepidermoid carcinoma, a type of salivary gland tumor that produces acid mucins. The staining technique can help pathologists identify the presence and distribution of these mucins within the tumor cells, which can aid in making an accurate diagnosis and determining the best course of treatment.

It's worth noting that there are several different types of histological stains that use various dyes to highlight different structures or features within tissues. Azure stains are just one example of these techniques, and they are typically used in conjunction with other staining methods to provide a comprehensive picture of the tissue being examined.

Ubiquitin-Protein Ligase Complexes, also known as E3 ubiquitin ligases, are a group of enzymes that play a crucial role in the ubiquitination process. Ubiquitination is a post-translational modification where ubiquitin molecules are attached to specific target proteins, marking them for degradation by the proteasome or altering their function, localization, or interaction with other proteins.

The ubiquitination process involves three main steps:

1. Ubiquitin activation: Ubiquitin is activated by an E1 ubiquitin-activating enzyme in an ATP-dependent reaction.
2. Ubiquitin conjugation: The activated ubiquitin is then transferred to an E2 ubiquitin-conjugating enzyme.
3. Ubiquitin ligation: Finally, the E2 ubiquitin-conjugating enzyme interacts with a specific E3 ubiquitin ligase complex, which facilitates the transfer and ligation of ubiquitin to the target protein.

Ubiquitin-Protein Ligase Complexes are responsible for recognizing and binding to specific substrate proteins, ensuring that ubiquitination occurs on the correct targets. They can be divided into three main categories based on their structural features and mechanisms of action:

1. Really Interesting New Gene (RING) finger E3 ligases: These E3 ligases contain a RING finger domain, which directly interacts with both the E2 ubiquitin-conjugating enzyme and the substrate protein. They facilitate the transfer of ubiquitin from the E2 to the target protein by bringing them into close proximity.
2. Homologous to E6-AP C terminus (HECT) E3 ligases: These E3 ligases contain a HECT domain, which interacts with the E2 ubiquitin-conjugating enzyme and forms a thioester bond with ubiquitin before transferring it to the substrate protein.
3. RING-between-RING (RBR) E3 ligases: These E3 ligases contain both RING finger and HECT-like domains, which allow them to function similarly to both RING finger and HECT E3 ligases. They first form a thioester bond with ubiquitin using their RING1 domain before transferring it to the substrate protein via their RING2 domain.

Dysregulation of Ubiquitin-Protein Ligase Complexes has been implicated in various diseases, including cancer and neurodegenerative disorders. Understanding their mechanisms and functions can provide valuable insights into disease pathogenesis and potential therapeutic strategies.

The Anaphase-Promoting Complex/Cyclosome (APC/C) is a large E3 ubiquitin ligase complex that plays a crucial role in the regulation of the cell cycle. It is responsible for targeting specific proteins for degradation by the proteasome, which is a multi-subunit protein complex that mediates the controlled breakdown of ubiquitinated proteins.

During anaphase, the final stage of mitosis, the APC/C becomes active and triggers the degradation of several key regulatory proteins, including securin and cyclin B. The destruction of these proteins allows for the separation of chromosomes and the completion of cell division.

The APC/C is composed of multiple subunits, including a catalytic core that binds to ubiquitin-conjugating enzymes (E2s) and several coactivators that regulate its activity. The activation of the APC/C requires the binding of one of two coactivators, Cdc20 or CDH1, which recognize specific substrates for degradation.

Dysregulation of the APC/C has been implicated in various human diseases, including cancer and neurodegenerative disorders. Therefore, understanding the mechanisms that regulate its activity is an important area of research with potential therapeutic implications.

Kinesin is not a medical term per se, but a term from the field of cellular biology. However, understanding how kinesins work is important in the context of medical and cellular research.

Kinesins are a family of motor proteins that play a crucial role in transporting various cargoes within cells, such as vesicles, organelles, and chromosomes. They move along microtubule filaments, using the energy derived from ATP hydrolysis to generate mechanical force and motion. This process is essential for several cellular functions, including intracellular transport, mitosis, and meiosis.

In a medical context, understanding kinesin function can provide insights into various diseases and conditions related to impaired intracellular transport, such as neurodegenerative disorders (e.g., Alzheimer's disease, Parkinson's disease, and Huntington's disease) and certain genetic disorders affecting motor neurons. Research on kinesins can potentially lead to the development of novel therapeutic strategies targeting these conditions.

Fluorescence microscopy is a type of microscopy that uses fluorescent dyes or proteins to highlight and visualize specific components within a sample. In this technique, the sample is illuminated with high-energy light, typically ultraviolet (UV) or blue light, which excites the fluorescent molecules causing them to emit lower-energy, longer-wavelength light, usually visible light in the form of various colors. This emitted light is then collected by the microscope and detected to produce an image.

Fluorescence microscopy has several advantages over traditional brightfield microscopy, including the ability to visualize specific structures or molecules within a complex sample, increased sensitivity, and the potential for quantitative analysis. It is widely used in various fields of biology and medicine, such as cell biology, neuroscience, and pathology, to study the structure, function, and interactions of cells and proteins.

There are several types of fluorescence microscopy techniques, including widefield fluorescence microscopy, confocal microscopy, two-photon microscopy, and total internal reflection fluorescence (TIRF) microscopy, each with its own strengths and limitations. These techniques can provide valuable insights into the behavior of cells and proteins in health and disease.

Sperm-ovum interactions, also known as sperm-egg interactions, refer to the specific series of events that occur between a spermatozoon (sperm) and an oocyte (egg or ovum) during fertilization in sexual reproduction.

The process begins with the sperm's attachment to the zona pellucida, a glycoprotein layer surrounding the oocyte. This interaction is mediated by specific proteins on the surface of both the sperm and the zona pellucida. Following attachment, the sperm undergoes the acrosome reaction, during which enzymes are released from the sperm's head to help digest and penetrate the zona pellucida.

Once the sperm has successfully traversed the zona pellucida, it makes contact with the oocyte's plasma membrane, triggering the fusion of the sperm and egg membranes. This results in the release of the sperm's genetic material into the oocyte's cytoplasm and the initiation of a series of intracellular signaling events within the oocyte that ultimately lead to its completion of meiosis II and formation of a zygote, marking the beginning of embryonic development.

Proper sperm-ovum interactions are crucial for successful fertilization and subsequent embryonic development, and any disruptions in these processes can result in infertility or early pregnancy loss.

I'm sorry for any confusion, but "Protamine Kinase" is not a widely recognized or established term in medical or biological sciences. Protamines are small, arginine-rich proteins found in the sperm cells of many organisms, and they play a crucial role in the packaging and protection of DNA during spermatogenesis.

Kinases, on the other hand, are enzymes that catalyze the transfer of phosphate groups from ATP to specific amino acids in proteins, thereby modulating their function, localization, or stability.

A search of scientific literature reveals only a few instances where "protamine kinase" is mentioned, usually in the context of potential regulatory mechanisms during sperm maturation or fertilization. However, there is no widely accepted or well-characterized enzyme known as "protamine kinase." Therefore, it would be challenging to provide a concise and accurate medical definition for this term.

A centrosome is a microtubule-organizing center found in animal cells. It consists of two barrel-shaped structures called centrioles, which are surrounded by a protein matrix called the pericentriolar material. The centrosome plays a crucial role in organizing the microtubules that form the cell's cytoskeleton and help to shape the cell, as well as in separating the chromosomes during cell division.

During mitosis, the two centrioles of the centrosome separate and move to opposite poles of the cell, where they nucleate the formation of the spindle fibers that pull the chromosomes apart. The centrosome also helps to ensure that the genetic material is equally distributed between the two resulting daughter cells.

It's worth noting that while centrioles are present in many animal cells, they are not always present in all types of cells. For example, plant cells do not have centrioles or centrosomes, and instead rely on other mechanisms to organize their microtubules.

Securin is not a medical term, but rather a biological concept related to cell division. It's a protein that plays a crucial role in the regulation of chromosome separation during cell division (mitosis).

During mitosis, sister chromatids (identical copies of a chromosome) are held together by cohesin proteins until it's time for them to separate and move to opposite ends of the cell. Securin is one of the proteins that helps regulate this process. Specifically, securin inhibits an enzyme called separase, which is responsible for cleaving the cohesin rings that hold sister chromatids together.

Once the cell is ready to separate its chromosomes, a protease called separase is activated and degrades securin. This allows separase to cleave the cohesin rings, leading to the separation of sister chromatids and the continuation of mitosis. If securin function is disrupted, it can lead to errors in chromosome segregation, which can contribute to genomic instability and diseases like cancer.

Chromosome painting is a molecular cytogenetic technique used to identify and visualize the specific chromosomes or chromosomal regions that are present in an abnormal location or number in a cell. This technique uses fluorescent probes that bind specifically to different chromosomes or chromosomal regions, allowing for their identification under a fluorescence microscope.

The process of chromosome painting involves labeling different chromosomes or chromosomal regions with fluorescent dyes of distinct colors. The labeled probes are then hybridized to the metaphase chromosomes of a cell, and any excess probe is washed away. The resulting fluorescent pattern allows for the identification of specific chromosomes or chromosomal regions that have been gained, lost, or rearranged in the genome.

Chromosome painting has numerous applications in medical genetics, including prenatal diagnosis, cancer cytogenetics, and constitutional genetic disorders. It can help to identify chromosomal abnormalities such as translocations, deletions, and duplications that may contribute to disease or cancer development.

Spermatozoa are the male reproductive cells, or gametes, that are produced in the testes. They are microscopic, flagellated (tail-equipped) cells that are highly specialized for fertilization. A spermatozoon consists of a head, neck, and tail. The head contains the genetic material within the nucleus, covered by a cap-like structure called the acrosome which contains enzymes to help the sperm penetrate the female's egg (ovum). The long, thin tail propels the sperm forward through fluid, such as semen, enabling its journey towards the egg for fertilization.

Medical Definition:
Microtubule-associated proteins (MAPs) are a diverse group of proteins that bind to microtubules, which are key components of the cytoskeleton in eukaryotic cells. MAPs play crucial roles in regulating microtubule dynamics and stability, as well as in mediating interactions between microtubules and other cellular structures. They can be classified into several categories based on their functions, including:

1. Microtubule stabilizers: These MAPs promote the assembly of microtubules and protect them from disassembly by enhancing their stability. Examples include tau proteins and MAP2.
2. Microtubule dynamics regulators: These MAPs modulate the rate of microtubule polymerization and depolymerization, allowing for dynamic reorganization of the cytoskeleton during cell division and other processes. Examples include stathmin and XMAP215.
3. Microtubule motor proteins: These MAPs use energy from ATP hydrolysis to move along microtubules, transporting various cargoes within the cell. Examples include kinesin and dynein.
4. Adapter proteins: These MAPs facilitate interactions between microtubules and other cellular structures, such as membranes, organelles, or signaling molecules. Examples include MAP4 and CLASPs.

Dysregulation of MAPs has been implicated in several diseases, including neurodegenerative disorders like Alzheimer's disease (where tau proteins form abnormal aggregates called neurofibrillary tangles) and cancer (where altered microtubule dynamics can contribute to uncontrolled cell division).

I'm sorry for any confusion, but "Potoroidae" is not a medical term. It is a taxonomic family within the order Diprotodontia, which includes several species of rat-kangaroos that are native to Australia. These small marsupials are known for their hopping locomotion and nocturnal behavior. If you have any questions about veterinary or medical terminology, I would be happy to help with those!

The cleavage stage of an ovum, also known as a fertilized egg, refers to the series of rapid cell divisions that occur after fertilization. During this stage, the single cell (zygote) divides into multiple cells, forming a blastomere. This process occurs in the fallopian tube and continues until the blastocyst reaches the uterus, typically around 5-6 days after fertilization. The cleavage stage is a critical period in early embryonic development, as any abnormalities during this time can lead to implantation failure or developmental defects.

Nuclear transfer techniques are scientific procedures that involve the transfer of the nucleus of a cell, containing its genetic material, from one cell to another. The most well-known type of nuclear transfer is somatic cell nuclear transfer (SCNT), which is used in therapeutic cloning and reproductive cloning.

In SCNT, the nucleus of a somatic cell (a body cell, not an egg or sperm cell) is transferred into an enucleated egg cell (an egg cell from which the nucleus has been removed). The egg cell with the new nucleus is then stimulated to divide and grow, creating an embryo that is genetically identical to the donor of the somatic cell.

Nuclear transfer techniques have various potential applications in medicine, including the creation of patient-specific stem cells for use in regenerative medicine, drug development and testing, and the study of genetic diseases. However, these procedures are also associated with ethical concerns, particularly in relation to reproductive cloning and the creation of human embryos for research purposes.

"Primed In Situ Labeling" (PRINS) is not a widely recognized medical term, but it is a technique used in molecular biology and pathology. Here's a definition of the PRINS technique:

Primed In Situ Labeling (PRINS) is a cytogenetic method that allows for the detection and visualization of specific DNA sequences within chromosomes or interphase nuclei through fluorescence in situ hybridization (FISH). The technique involves denaturing double-stranded DNA in fixed cells, followed by annealing a primer to a specific target sequence. A DNA polymerase then extends the primer, incorporating labeled nucleotides that can be visualized under a fluorescence microscope.

The PRINS technique offers several advantages over traditional FISH methods, including higher sensitivity and specificity, lower background signal, and the ability to analyze multiple targets simultaneously using different colored probes. It is commonly used in the diagnosis and monitoring of various genetic disorders, cancer, and infectious diseases.

Cyclin B1 is a type of cyclin protein that regulates the cell cycle, specifically the transition from G2 phase to mitosis (M phase) in eukaryotic cells. It forms a complex with and acts as a regulatory subunit of cyclin-dependent kinase 1 (CDK1), also known as CDC2. During the G2 phase, Cyclin B1 levels accumulate and upon reaching a certain threshold, it binds to CDK1 to form the maturation promoting factor (MPF). The activation of MPF triggers the onset of mitosis by promoting nuclear envelope breakdown, chromosome condensation, and other events required for cell division. After the completion of mitosis, Cyclin B1 is degraded by the ubiquitin-proteasome system, allowing the cell cycle to progress back into G1 phase.

Colchicine is a medication that is primarily used to treat gout, a type of arthritis characterized by sudden and severe attacks of pain, swelling, redness, and tenderness in the joints. It works by reducing inflammation and preventing the formation of uric acid crystals that cause gout symptoms.

Colchicine is also used to treat familial Mediterranean fever (FMF), a genetic disorder that causes recurrent fevers and inflammation in the abdomen, chest, and joints. It can help prevent FMF attacks and reduce their severity.

The medication comes in the form of tablets or capsules that are taken by mouth. Common side effects of colchicine include diarrhea, nausea, vomiting, and abdominal pain. In rare cases, it can cause more serious side effects such as muscle weakness, nerve damage, and bone marrow suppression.

It is important to follow the dosage instructions carefully when taking colchicine, as taking too much of the medication can be toxic. People with certain health conditions, such as liver or kidney disease, may need to take a lower dose or avoid using colchicine altogether.

Meiotic Prophase I is a stage in the meiotic division of cellular reproduction that results in the formation of gametes or sex cells (sperm and egg). It is the first of five stages in Meiosis I, which is a type of cell division that reduces the chromosome number by half.

During Meiotic Prophase I, homologous chromosomes pair and form tetrads (four-stranded structures), which then undergo genetic recombination or crossing over, resulting in new combinations of alleles on the chromatids of each homologous chromosome. This stage can be further divided into several substages: leptonema, zygonema, pachynema, diplonema, and diakinesis. These substages are characterized by distinct changes in chromosome structure and behavior, including the condensation and movement of the chromosomes, as well as the formation and dissolution of the synaptonemal complex, a protein structure that holds the homologous chromosomes together during crossing over.

Overall, Meiotic Prophase I is a critical stage in meiosis that ensures genetic diversity in offspring by shuffling the genetic material between homologous chromosomes and creating new combinations of alleles.

A blastocyst is a stage in the early development of a fertilized egg, or embryo, in mammals. It occurs about 5-6 days after fertilization and consists of an outer layer of cells called trophoblasts, which will eventually form the placenta, and an inner cell mass, which will give rise to the fetus. The blastocyst is characterized by a fluid-filled cavity called the blastocoel. This stage is critical for the implantation of the embryo into the uterine lining.

Nuclear proteins are a category of proteins that are primarily found in the nucleus of a eukaryotic cell. They play crucial roles in various nuclear functions, such as DNA replication, transcription, repair, and RNA processing. This group includes structural proteins like lamins, which form the nuclear lamina, and regulatory proteins, such as histones and transcription factors, that are involved in gene expression. Nuclear localization signals (NLS) often help target these proteins to the nucleus by interacting with importin proteins during active transport across the nuclear membrane.

The Nucleolus Organizer Region (NOR) is a specific region within the chromosomes, primarily in the short arm of the acrocentric chromosomes (chromosomes 13, 14, 15, 21, and 22). It consists of clusters of repetitive DNA sequences that encode ribosomal RNA (rRNA) genes. During interphase, these regions form the nucleolus, a distinct structure within the nucleus where rRNA transcription, processing, and ribosome assembly occur. The number of NORs in an individual can vary, which has implications in certain genetic conditions and aging processes.

I believe you may be mistakenly using the term "starfish" to refer to a medical condition. If so, the correct term is likely " asterixis," which is a medical sign characterized by rapid, rhythmic flapping or tremulous movements of the hands when they are extended and the wrist is dorsiflexed (held with the back of the hand facing upwards). This is often seen in people with certain neurological conditions such as liver failure or certain types of poisoning.

However, if you are indeed referring to the marine animal commonly known as a "starfish," there isn't a specific medical definition for it. Starfish, also known as sea stars, are marine animals belonging to the class Asteroidea in the phylum Echinodermata. They have a distinctive shape with five or more arms radiating from a central disc, and they move slowly along the ocean floor using their tube feet. Some species of starfish have the ability to regenerate lost body parts, including entire limbs or even their central disc.

Aurora Kinase B is a type of enzyme that plays a crucial role in the regulation of cell division and mitosis. It is a member of the Aurora kinase family, which includes three different isoforms (Aurora A, B, and C). Among these, Aurora Kinase B is specifically involved in the proper alignment and separation of chromosomes during cell division.

During mitosis, Aurora Kinase B forms a complex with other proteins to form the chromosomal passenger complex (CPC), which plays a critical role in ensuring accurate chromosome segregation. The CPC is responsible for regulating various events during mitosis, including the attachment of microtubules to kinetochores (protein structures that connect chromosomes to spindle fibers), the correction of erroneous kinetochore-microtubule attachments, and the regulation of the anaphase promoting complex/cyclosome (APC/C), which targets specific proteins for degradation during mitosis.

Dysregulation of Aurora Kinase B has been implicated in various human diseases, including cancer. Overexpression or amplification of this kinase can lead to chromosomal instability and aneuploidy, contributing to tumorigenesis and cancer progression. As a result, Aurora Kinase B is considered a promising target for the development of anti-cancer therapies, with several inhibitors currently being investigated in preclinical and clinical studies.

Chromosome disorders are a group of genetic conditions caused by abnormalities in the number or structure of chromosomes. Chromosomes are thread-like structures located in the nucleus of cells that contain most of the body's genetic material, which is composed of DNA and proteins. Normally, humans have 23 pairs of chromosomes, for a total of 46 chromosomes.

Chromosome disorders can result from changes in the number of chromosomes (aneuploidy) or structural abnormalities in one or more chromosomes. Some common examples of chromosome disorders include:

1. Down syndrome: a condition caused by an extra copy of chromosome 21, resulting in intellectual disability, developmental delays, and distinctive physical features.
2. Turner syndrome: a condition that affects only females and is caused by the absence of all or part of one X chromosome, resulting in short stature, lack of sexual development, and other symptoms.
3. Klinefelter syndrome: a condition that affects only males and is caused by an extra copy of the X chromosome, resulting in tall stature, infertility, and other symptoms.
4. Cri-du-chat syndrome: a condition caused by a deletion of part of the short arm of chromosome 5, resulting in intellectual disability, developmental delays, and a distinctive cat-like cry.
5. Fragile X syndrome: a condition caused by a mutation in the FMR1 gene on the X chromosome, resulting in intellectual disability, behavioral problems, and physical symptoms.

Chromosome disorders can be diagnosed through various genetic tests, such as karyotyping, chromosomal microarray analysis (CMA), or fluorescence in situ hybridization (FISH). Treatment for these conditions depends on the specific disorder and its associated symptoms and may include medical interventions, therapies, and educational support.

Sister chromatid exchange (SCE) is a type of genetic recombination that takes place between two identical sister chromatids during the DNA repair process in meiosis or mitosis. It results in an exchange of genetic material between the two chromatids, creating a new combination of genes on each chromatid. This event is a normal part of cell division and helps to increase genetic variability within a population. However, an increased rate of SCEs can also be indicative of exposure to certain genotoxic agents or conditions that cause DNA damage.

Blastomeres are early stage embryonic cells that result from the initial rounds of cell division in a fertilized egg, also known as a zygote. These cells are typically smaller and have a more simple organization compared to more mature cells. They are important for the normal development of the embryo and contribute to the formation of the blastocyst, which is an early stage embryonic structure that will eventually give rise to the fetus. The process of cell division that produces blastomeres is called cleavage.

CDC20 proteins are a type of regulatory protein that play a crucial role in the cell cycle, which is the process by which cells grow and divide. Specifically, CDC20 proteins are involved in the transition from metaphase to anaphase during mitosis, the phase of the cell cycle where chromosomes are separated and distributed to two daughter cells.

CDC20 proteins function as part of a larger complex called the anaphase-promoting complex/cyclosome (APC/C), which targets specific proteins for degradation by the proteasome. During metaphase, CDC20 binds to the APC/C and helps to activate it, leading to the degradation of securin and cyclin B, two proteins that are essential for maintaining the proper attachment of chromosomes to the spindle apparatus.

Once these proteins are degraded, the sister chromatids can be separated and moved to opposite poles of the cell, allowing for the completion of mitosis and the formation of two genetically identical daughter cells. In addition to their role in mitosis, CDC20 proteins have also been implicated in other cellular processes, including meiosis, DNA damage repair, and apoptosis.

Translocation, genetic, refers to a type of chromosomal abnormality in which a segment of a chromosome is transferred from one chromosome to another, resulting in an altered genome. This can occur between two non-homologous chromosomes (non-reciprocal translocation) or between two homologous chromosomes (reciprocal translocation). Genetic translocations can lead to various clinical consequences, depending on the genes involved and the location of the translocation. Some translocations may result in no apparent effects, while others can cause developmental abnormalities, cancer, or other genetic disorders. In some cases, translocations can also increase the risk of having offspring with genetic conditions.

M Phase cell cycle checkpoints are control mechanisms that ensure the proper completion of the M phase (mitosis or meiosis) of the cell cycle. These checkpoints verify that certain conditions are met before the cell proceeds to the next phase of the cell cycle, thus helping to maintain genomic stability and prevent errors such as chromosomal mutations or aneuploidy.

There are two main M Phase cell cycle checkpoints:

1. The G2/M Checkpoint: This checkpoint is activated at the end of the G2 phase and verifies that all DNA has been replicated accurately, and that there are no DNA damages or other issues that could interfere with mitosis. If any problems are detected, the cell cycle is halted until they can be resolved.
2. The Mitotic Spindle Checkpoint: This checkpoint ensures that all chromosomes have attached properly to the spindle apparatus and that they will be equally distributed to the two resulting daughter cells during mitosis. If any chromosomes are not properly attached or if there is an issue with the spindle apparatus, the cell cycle is paused until these problems are corrected.

These checkpoints play a crucial role in maintaining genomic stability and preventing the development of cancer and other diseases.

Protein-Serine-Threonine Kinases (PSTKs) are a type of protein kinase that catalyzes the transfer of a phosphate group from ATP to the hydroxyl side chains of serine or threonine residues on target proteins. This phosphorylation process plays a crucial role in various cellular signaling pathways, including regulation of metabolism, gene expression, cell cycle progression, and apoptosis. PSTKs are involved in many physiological and pathological processes, and their dysregulation has been implicated in several diseases, such as cancer, diabetes, and neurodegenerative disorders.

Cytoplasm is the material within a eukaryotic cell (a cell with a true nucleus) that lies between the nuclear membrane and the cell membrane. It is composed of an aqueous solution called cytosol, in which various organelles such as mitochondria, ribosomes, endoplasmic reticulum, Golgi apparatus, lysosomes, and vacuoles are suspended. Cytoplasm also contains a variety of dissolved nutrients, metabolites, ions, and enzymes that are involved in various cellular processes such as metabolism, signaling, and transport. It is where most of the cell's metabolic activities take place, and it plays a crucial role in maintaining the structure and function of the cell.

"Xenopus" is not a medical term, but it is a genus of highly invasive aquatic frogs native to sub-Saharan Africa. They are often used in scientific research, particularly in developmental biology and genetics. The most commonly studied species is Xenopus laevis, also known as the African clawed frog.

In a medical context, Xenopus might be mentioned when discussing their use in research or as a model organism to study various biological processes or diseases.

Intracytoplasmic Sperm Injection (ICSI) is a specialized form of assisted reproductive technology (ART), specifically used in the context of in vitro fertilization (IVF). It involves the direct injection of a single sperm into the cytoplasm of a mature egg (oocyte) to facilitate fertilization. This technique is often used when there are issues with male infertility, such as low sperm count or poor sperm motility, to increase the chances of successful fertilization. The resulting embryos can then be transferred to the uterus in hopes of achieving a pregnancy.

Chromosome pairing, also known as chromosome synapsis, is a process that occurs during meiosis, which is the type of cell division that results in the formation of sex cells or gametes (sperm and eggs).

In humans, each cell contains 23 pairs of chromosomes, for a total of 46 chromosomes. Of these, 22 pairs are called autosomal chromosomes, and they are similar in size and shape between the two copies in a pair. The last pair is called the sex chromosomes (X and Y), which determine the individual's biological sex.

During meiosis, homologous chromosomes (one from each parent) come together and pair up along their lengths in a process called synapsis. This pairing allows for the precise alignment of corresponding genes and genetic regions between the two homologous chromosomes. Once paired, the chromosomes exchange genetic material through a process called crossing over, which increases genetic diversity in the resulting gametes.

After crossing over, the homologous chromosomes separate during meiosis I, followed by the separation of sister chromatids (the two copies of each chromosome) during meiosis II. The end result is four haploid cells, each containing 23 chromosomes, which then develop into sperm or eggs.

Chromosome pairing is a crucial step in the process of sexual reproduction, ensuring that genetic information is accurately passed from one generation to the next while also promoting genetic diversity through recombination and independent assortment of chromosomes.

Polar bodies are small, non-functional cells that are produced during the process of female meiosis, which results in the formation of an egg cell. They are formed when cytoplasmic divisions occur without subsequent cytokinesis, resulting in the separation of a small amount of cytoplasm and organelles from the main cell.

In the first meiotic division, a primary oocyte divides into a larger secondary oocyte and a smaller polar body, which contains half the number of chromosomes as the original cell. During the second meiotic division, the secondary oocyte divides into a larger ovum (egg) and another smaller polar body, again with half the number of chromosomes.

Polar bodies are typically extruded from the main cell and eventually disintegrate or are absorbed by surrounding cells. They do not contribute to the genetic makeup of the resulting egg or any offspring that may be produced from it. The formation of polar bodies helps ensure that the egg contains the correct number of chromosomes for normal development.

"Xenopus proteins" refer to the proteins that are expressed or isolated from the Xenopus species, which are primarily used as model organisms in biological and biomedical research. The most commonly used Xenopus species for research are the African clawed frogs, Xenopus laevis and Xenopus tropicalis. These proteins play crucial roles in various cellular processes and functions, and they serve as valuable tools to study different aspects of molecular biology, developmental biology, genetics, and biochemistry.

Some examples of Xenopus proteins that are widely studied include:

1. Xenopus Histones: These are the proteins that package DNA into nucleosomes, which are the fundamental units of chromatin in eukaryotic cells. They play a significant role in gene regulation and epigenetic modifications.
2. Xenopus Cyclins and Cyclin-dependent kinases (CDKs): These proteins regulate the cell cycle and control cell division, differentiation, and apoptosis.
3. Xenopus Transcription factors: These proteins bind to specific DNA sequences and regulate gene expression during development and in response to various stimuli.
4. Xenopus Signaling molecules: These proteins are involved in intracellular signaling pathways that control various cellular processes, such as cell growth, differentiation, migration, and survival.
5. Xenopus Cytoskeletal proteins: These proteins provide structural support to the cells and regulate their shape, motility, and organization.
6. Xenopus Enzymes: These proteins catalyze various biochemical reactions in the cell, such as metabolic pathways, DNA replication, transcription, and translation.

Overall, Xenopus proteins are essential tools for understanding fundamental biological processes and have contributed significantly to our current knowledge of molecular biology, genetics, and developmental biology.

Cell division is the process by which a single eukaryotic cell (a cell with a true nucleus) divides into two identical daughter cells. This complex process involves several stages, including replication of DNA, separation of chromosomes, and division of the cytoplasm. There are two main types of cell division: mitosis and meiosis.

Mitosis is the type of cell division that results in two genetically identical daughter cells. It is a fundamental process for growth, development, and tissue repair in multicellular organisms. The stages of mitosis include prophase, prometaphase, metaphase, anaphase, and telophase, followed by cytokinesis, which divides the cytoplasm.

Meiosis, on the other hand, is a type of cell division that occurs in the gonads (ovaries and testes) during the production of gametes (sex cells). Meiosis results in four genetically unique daughter cells, each with half the number of chromosomes as the parent cell. This process is essential for sexual reproduction and genetic diversity. The stages of meiosis include meiosis I and meiosis II, which are further divided into prophase, prometaphase, metaphase, anaphase, and telophase.

In summary, cell division is the process by which a single cell divides into two daughter cells, either through mitosis or meiosis. This process is critical for growth, development, tissue repair, and sexual reproduction in multicellular organisms.

Embryonic development is the series of growth and developmental stages that occur during the formation and early growth of the embryo. In humans, this stage begins at fertilization (when the sperm and egg cell combine) and continues until the end of the 8th week of pregnancy. During this time, the fertilized egg (now called a zygote) divides and forms a blastocyst, which then implants into the uterus. The cells in the blastocyst begin to differentiate and form the three germ layers: the ectoderm, mesoderm, and endoderm. These germ layers will eventually give rise to all of the different tissues and organs in the body.

Embryonic development is a complex and highly regulated process that involves the coordinated interaction of genetic and environmental factors. It is characterized by rapid cell division, migration, and differentiation, as well as programmed cell death (apoptosis) and tissue remodeling. Abnormalities in embryonic development can lead to birth defects or other developmental disorders.

It's important to note that the term "embryo" is used to describe the developing organism from fertilization until the end of the 8th week of pregnancy in humans, after which it is called a fetus.

"Cells, cultured" is a medical term that refers to cells that have been removed from an organism and grown in controlled laboratory conditions outside of the body. This process is called cell culture and it allows scientists to study cells in a more controlled and accessible environment than they would have inside the body. Cultured cells can be derived from a variety of sources, including tissues, organs, or fluids from humans, animals, or cell lines that have been previously established in the laboratory.

Cell culture involves several steps, including isolation of the cells from the tissue, purification and characterization of the cells, and maintenance of the cells in appropriate growth conditions. The cells are typically grown in specialized media that contain nutrients, growth factors, and other components necessary for their survival and proliferation. Cultured cells can be used for a variety of purposes, including basic research, drug development and testing, and production of biological products such as vaccines and gene therapies.

It is important to note that cultured cells may behave differently than they do in the body, and results obtained from cell culture studies may not always translate directly to human physiology or disease. Therefore, it is essential to validate findings from cell culture experiments using additional models and ultimately in clinical trials involving human subjects.

Micromanipulation is a term used in the field of medicine, specifically in assisted reproductive technologies (ARTs) such as in vitro fertilization (IVF). It refers to a technique that involves the manipulation of oocytes (human eggs), sperm, and/or embryos under a microscope using micromanipulative tools and equipment.

The most common form of micromanipulation is intracytoplasmic sperm injection (ICSI), where a single sperm is selected and injected directly into the cytoplasm of an oocyte to facilitate fertilization. Other forms of micromanipulation include assisted hatching (AH), where a small opening is made in the zona pellucida (the protective layer surrounding the embryo) to help the embryo hatch and implant into the uterus, and embryo biopsy, which involves removing one or more cells from an embryo for genetic testing.

Micromanipulation requires specialized training and equipment and is typically performed in IVF laboratories by experienced embryologists. The goal of micromanipulation is to improve the chances of successful fertilization, implantation, and pregnancy, particularly in cases where conventional methods have been unsuccessful or when there are specific fertility issues, such as male factor infertility or genetic disorders.

Chromosome mapping, also known as physical mapping, is the process of determining the location and order of specific genes or genetic markers on a chromosome. This is typically done by using various laboratory techniques to identify landmarks along the chromosome, such as restriction enzyme cutting sites or patterns of DNA sequence repeats. The resulting map provides important information about the organization and structure of the genome, and can be used for a variety of purposes, including identifying the location of genes associated with genetic diseases, studying evolutionary relationships between organisms, and developing genetic markers for use in breeding or forensic applications.

Nuclear matrix-associated proteins (NMAPs) are a group of structural and functional proteins that are associated with the nuclear matrix, a network of fibers within the nucleus of a eukaryotic cell. The nuclear matrix provides support to the nuclear envelope and plays a role in DNA replication, transcription, and repair. NMAPs can be categorized into several groups based on their functions, including:

1. Scaffold proteins: These proteins provide structural support to the nuclear matrix and help maintain its architecture.
2. Enzymes: These proteins are involved in various biochemical reactions, such as DNA replication and repair, RNA processing, and chromatin remodeling.
3. Transcription factors: These proteins regulate gene expression by binding to specific DNA sequences and interacting with the transcription machinery.
4. Chromatin-associated proteins: These proteins are involved in the organization and regulation of chromatin structure and function.
5. Signal transduction proteins: These proteins transmit signals from the extracellular environment to the nucleus, regulating gene expression and other nuclear functions.

NMAPs have been implicated in various cellular processes, including cell cycle regulation, differentiation, apoptosis, and oncogenesis. Therefore, understanding the structure and function of NMAPs is crucial for elucidating the mechanisms underlying these processes and developing novel therapeutic strategies for various diseases, including cancer.

Mammalian chromosomes are thread-like structures that exist in the nucleus of mammalian cells, consisting of DNA, hist proteins, and RNA. They carry genetic information that is essential for the development and function of all living organisms. In mammals, each cell contains 23 pairs of chromosomes, for a total of 46 chromosomes, with one set inherited from the mother and the other from the father.

The chromosomes are typically visualized during cell division, where they condense and become visible under a microscope. Each chromosome is composed of two identical arms, separated by a constriction called the centromere. The short arm of the chromosome is labeled as "p," while the long arm is labeled as "q."

Mammalian chromosomes play a critical role in the transmission of genetic information from one generation to the next and are essential for maintaining the stability and integrity of the genome. Abnormalities in the number or structure of mammalian chromosomes can lead to various genetic disorders, including Down syndrome, Turner syndrome, and Klinefelter syndrome.

Sex chromosomes, often denoted as X and Y, are one of the 23 pairs of human chromosomes found in each cell of the body. Normally, females have two X chromosomes (46,XX), and males have one X and one Y chromosome (46,XY). The sex chromosomes play a significant role in determining the sex of an individual. They contain genes that contribute to physical differences between men and women. Any variations or abnormalities in the number or structure of these chromosomes can lead to various genetic disorders and conditions related to sexual development and reproduction.

The Fluorescent Antibody Technique (FAT) is a type of immunofluorescence assay used in laboratory medicine and pathology for the detection and localization of specific antigens or antibodies in tissues, cells, or microorganisms. In this technique, a fluorescein-labeled antibody is used to selectively bind to the target antigen or antibody, forming an immune complex. When excited by light of a specific wavelength, the fluorescein label emits light at a longer wavelength, typically visualized as green fluorescence under a fluorescence microscope.

The FAT is widely used in diagnostic microbiology for the identification and characterization of various bacteria, viruses, fungi, and parasites. It has also been applied in the diagnosis of autoimmune diseases and certain cancers by detecting specific antibodies or antigens in patient samples. The main advantage of FAT is its high sensitivity and specificity, allowing for accurate detection and differentiation of various pathogens and disease markers. However, it requires specialized equipment and trained personnel to perform and interpret the results.

Human chromosomes are the thread-like structures located in the nucleus of human cells, which carry genetic information in the form of DNA. Humans have a total of 46 chromosomes arranged in 23 pairs. The first 22 pairs are called autosomes, and the last pair are the sex chromosomes, X and Y.

Chromosomes 1-3 are the largest human chromosomes, and they contain a significant portion of the human genome. Here is a brief overview of each:

1. Chromosome 1: This is the largest human chromosome, spanning about 8% of the human genome. It contains approximately 2,800 genes that are responsible for various functions such as cell growth and division, nerve function, and response to stimuli.
2. Chromosome 2: The second largest human chromosome, spanning about 7% of the human genome. It contains approximately 2,300 genes that are involved in various functions such as metabolism, development, and immune response.
3. Chromosome 3: This is the third largest human chromosome, spanning about 6% of the human genome. It contains approximately 1,900 genes that are responsible for various functions such as DNA repair, cell signaling, and response to stress.

It's worth noting that while these chromosomes contain a large number of genes, they also have significant amounts of non-coding DNA, which means that not all of the genetic material on these chromosomes is responsible for encoding proteins or other functional elements.

The v-mos oncogene protein is derived from the retrovirus called Moloney murine sarcoma virus (Mo-MSV). This oncogene encodes for a serine/threonine protein kinase, which is involved in cell proliferation and differentiation. When incorporated into the host genome during viral infection, the v-mos oncogene can cause unregulated cell growth and tumor formation, leading to sarcomas in mice. The normal cellular homolog of v-mos is called c-mos, which plays a crucial role in regulating cell division and is tightly controlled in normal cells. However, mutations or aberrant activation of c-mos can also contribute to oncogenic transformation and tumorigenesis.

A cell line is a culture of cells that are grown in a laboratory for use in research. These cells are usually taken from a single cell or group of cells, and they are able to divide and grow continuously in the lab. Cell lines can come from many different sources, including animals, plants, and humans. They are often used in scientific research to study cellular processes, disease mechanisms, and to test new drugs or treatments. Some common types of human cell lines include HeLa cells (which come from a cancer patient named Henrietta Lacks), HEK293 cells (which come from embryonic kidney cells), and HUVEC cells (which come from umbilical vein endothelial cells). It is important to note that cell lines are not the same as primary cells, which are cells that are taken directly from a living organism and have not been grown in the lab.

A karyotype is a method used in genetics to describe the number and visual appearance of chromosomes in the nucleus of a cell. It includes the arrangement of the chromosomes by length, position of the centromeres, and banding pattern. A karyotype is often represented as a photograph or image of an individual's chromosomes, arranged in pairs from largest to smallest, that has been stained to show the bands of DNA. This information can be used to identify genetic abnormalities, such as extra or missing chromosomes, or structural changes, such as deletions, duplications, or translocations. A karyotype is typically obtained by culturing cells from a sample of blood or tissue, then arresting the cell division at metaphase and staining the chromosomes to make them visible for analysis.

Human chromosomes 13-15 are part of a set of 23 pairs of chromosomes found in the cells of the human body. Chromosomes are thread-like structures that contain genetic material, or DNA, that is inherited from each parent. They are responsible for the development and function of all the body's organs and systems.

Chromosome 13 is a medium-sized chromosome and contains an estimated 114 million base pairs of DNA. It is associated with several genetic disorders, including cri du chat syndrome, which is caused by a deletion on the short arm of the chromosome. Chromosome 13 also contains several important genes, such as those involved in the production of enzymes and proteins that help regulate growth and development.

Chromosome 14 is a medium-sized chromosome and contains an estimated 107 million base pairs of DNA. It is known to contain many genes that are important for the normal functioning of the brain and nervous system, as well as genes involved in the production of immune system proteins. Chromosome 14 is also associated with a number of genetic disorders, including Wolf-Hirschhorn syndrome, which is caused by a deletion on the short arm of the chromosome.

Chromosome 15 is a medium-sized chromosome and contains an estimated 102 million base pairs of DNA. It is associated with several genetic disorders, including Prader-Willi syndrome and Angelman syndrome, which are caused by abnormalities in the expression of genes on the chromosome. Chromosome 15 also contains important genes involved in the regulation of growth and development, as well as genes that play a role in the production of neurotransmitters, the chemical messengers of the brain.

It is worth noting that while chromosomes 13-15 are important for normal human development and function, abnormalities in these chromosomes can lead to a variety of genetic disorders and developmental issues.

Polyploidy is a condition in which a cell or an organism has more than two sets of chromosomes, unlike the typical diploid state where there are only two sets (one from each parent). Polyploidy can occur through various mechanisms such as errors during cell division, fusion of egg and sperm cells that have an abnormal number of chromosomes, or through the reproduction process in plants.

Polyploidy is common in the plant kingdom, where it often leads to larger size, increased biomass, and sometimes hybrid vigor. However, in animals, polyploidy is less common and usually occurs in only certain types of cells or tissues, as most animals require a specific number of chromosomes for normal development and reproduction. In humans, polyploidy is typically not compatible with life and can lead to developmental abnormalities and miscarriage.

Cytokinesis is the part of the cell division process (mitosis or meiosis) in which the cytoplasm of a single eukaryotic cell divides into two daughter cells. It usually begins after telophase, and it involves the constriction of a contractile ring composed of actin filaments and myosin motor proteins that forms at the equatorial plane of the cell. This results in the formation of a cleavage furrow, which deepens and eventually leads to the physical separation of the two daughter cells. Cytokinesis is essential for cell reproduction and growth in multicellular organisms, and its failure can lead to various developmental abnormalities or diseases.

Deoxyribonucleic acid (DNA) is the genetic material present in the cells of organisms where it is responsible for the storage and transmission of hereditary information. DNA is a long molecule that consists of two strands coiled together to form a double helix. Each strand is made up of a series of four nucleotide bases - adenine (A), guanine (G), cytosine (C), and thymine (T) - that are linked together by phosphate and sugar groups. The sequence of these bases along the length of the molecule encodes genetic information, with A always pairing with T and C always pairing with G. This base-pairing allows for the replication and transcription of DNA, which are essential processes in the functioning and reproduction of all living organisms.

Molecular sequence data refers to the specific arrangement of molecules, most commonly nucleotides in DNA or RNA, or amino acids in proteins, that make up a biological macromolecule. This data is generated through laboratory techniques such as sequencing, and provides information about the exact order of the constituent molecules. This data is crucial in various fields of biology, including genetics, evolution, and molecular biology, allowing for comparisons between different organisms, identification of genetic variations, and studies of gene function and regulation.

Chromosome fragility refers to the susceptibility of specific regions on chromosomes to break or become unstable during cell division. These fragile sites are prone to forming gaps or breaks in the chromosome structure, which can lead to genetic rearrangements, including deletions, duplications, or translocations.

Chromosome fragility is often associated with certain genetic disorders and syndromes. For example, the most common fragile site in human chromosomes is FRAXA, located on the X chromosome, which is linked to Fragile X Syndrome, a leading cause of inherited intellectual disability and autism.

Environmental factors such as exposure to chemicals or radiation can also increase chromosome fragility, leading to an increased risk of genetic mutations and diseases.

Cumulus cells are a type of specialized cell that surround and support the egg (oocyte) in the ovary of female mammals, including humans. These cells are located in the cumulus oophorus, which is a cluster of cells that surrounds and protects the mature egg within the follicle.

Cumulus cells play an important role in the process of fertilization by providing nutrients to the developing egg and helping to regulate its growth and development. They also help to facilitate communication between the egg and the surrounding follicular cells, which is necessary for the release of the mature egg from the ovary during ovulation.

In addition to their role in reproduction, cumulus cells have been studied for their potential use in various medical applications, including as a source of stem cells for therapeutic purposes. However, more research is needed to fully understand the properties and potential uses of these cells.

Electron microscopy (EM) is a type of microscopy that uses a beam of electrons to create an image of the sample being examined, resulting in much higher magnification and resolution than light microscopy. There are several types of electron microscopy, including transmission electron microscopy (TEM), scanning electron microscopy (SEM), and reflection electron microscopy (REM).

In TEM, a beam of electrons is transmitted through a thin slice of the sample, and the electrons that pass through the sample are focused to form an image. This technique can provide detailed information about the internal structure of cells, viruses, and other biological specimens, as well as the composition and structure of materials at the atomic level.

In SEM, a beam of electrons is scanned across the surface of the sample, and the electrons that are scattered back from the surface are detected to create an image. This technique can provide information about the topography and composition of surfaces, as well as the structure of materials at the microscopic level.

REM is a variation of SEM in which the beam of electrons is reflected off the surface of the sample, rather than scattered back from it. This technique can provide information about the surface chemistry and composition of materials.

Electron microscopy has a wide range of applications in biology, medicine, and materials science, including the study of cellular structure and function, disease diagnosis, and the development of new materials and technologies.

Heterochromatin is a type of chromatin (the complex of DNA, RNA, and proteins that make up chromosomes) that is characterized by its tightly packed structure and reduced genetic activity. It is often densely stained with certain dyes due to its high concentration of histone proteins and other chromatin-associated proteins. Heterochromatin can be further divided into two subtypes: constitutive heterochromatin, which is consistently highly condensed and transcriptionally inactive throughout the cell cycle, and facultative heterochromatin, which can switch between a condensed, inactive state and a more relaxed, active state depending on the needs of the cell. Heterochromatin plays important roles in maintaining the stability and integrity of the genome by preventing the transcription of repetitive DNA sequences and protecting against the spread of transposable elements.

"Silver staining" is a histological term that refers to a technique used to selectively stain various components of biological tissues, making them more visible under a microscope. This technique is often used in the study of histopathology and cytology. The most common type of silver staining is known as "silver impregnation," which is used to demonstrate the presence of argyrophilic structures, such as nerve fibers and neurofibrillary tangles, in tissues.

The process of silver staining involves the use of silver salts, which are reduced by a developer to form metallic silver that deposits on the tissue components. The intensity of the stain depends on the degree of reduction of the silver ions, and it can be modified by adjusting the concentration of the silver salt, the development time, and other factors.

Silver staining is widely used in diagnostic pathology to highlight various structures such as nerve fibers, axons, collagen, basement membranes, and microorganisms like fungi and bacteria. It has also been used in research to study the distribution and organization of these structures in tissues. However, it's important to note that silver staining is not specific for any particular substance, so additional tests are often needed to confirm the identity of the stained structures.

I'm assuming you are asking for a definition of "gene" in the context of mosquitoes (Culicidae).

A gene is a hereditary unit that carries genetic information from one generation to the next. Genes are segments of DNA that contain the instructions for the development and function of an organism. In mosquitoes, genes play crucial roles in various biological processes such as growth, development, reproduction, behavior, and resistance to insecticides.

Mosquitoes have a relatively small genome size compared to other insects, with approximately 278 million base pairs organized into three chromosomes. The mosquito genome has been sequenced for several species, including the malaria vector Anopheles gambiae and the dengue fever vector Aedes aegypti, which has facilitated the identification of genes associated with various traits and diseases.

Understanding the genetic basis of mosquito biology is essential for developing effective strategies to control mosquito-borne diseases, such as malaria, dengue fever, yellow fever, Zika virus, and chikungunya.

Nondisjunction is a genetic term that refers to the failure of homologous chromosomes or sister chromatids to properly separate during cell division, resulting in an abnormal number of chromosomes in the daughter cells. This can occur during either mitosis (resulting in somatic mutations) or meiosis (leading to gametes with an incorrect number of chromosomes).

In humans, nondisjunction of chromosome 21 during meiosis is the most common cause of Down syndrome, resulting in three copies of chromosome 21 (trisomy 21) in the affected individual. Nondisjunction can also result in other aneuploidies, such as Turner syndrome (X monosomy), Klinefelter syndrome (XXY), and Edwards syndrome (trisomy 18).

Nondisjunction is typically a random event, although maternal age has been identified as a risk factor for nondisjunction during meiosis. In some cases, structural chromosomal abnormalities or genetic factors may predispose an individual to nondisjunction events.

Phosphorylation is the process of adding a phosphate group (a molecule consisting of one phosphorus atom and four oxygen atoms) to a protein or other organic molecule, which is usually done by enzymes called kinases. This post-translational modification can change the function, localization, or activity of the target molecule, playing a crucial role in various cellular processes such as signal transduction, metabolism, and regulation of gene expression. Phosphorylation is reversible, and the removal of the phosphate group is facilitated by enzymes called phosphatases.

Cryopreservation is a medical procedure that involves the preservation of cells, tissues, or organs by cooling them to very low temperatures, typically below -150°C. This is usually achieved using liquid nitrogen. The low temperature slows down or stops biological activity, including chemical reactions and cellular metabolism, which helps to prevent damage and decay.

The cells, tissues, or organs that are being cryopreserved must be treated with a cryoprotectant solution before cooling to prevent the formation of ice crystals, which can cause significant damage. Once cooled, the samples are stored in specialized containers or tanks until they are needed for use.

Cryopreservation is commonly used in assisted reproductive technologies, such as the preservation of sperm, eggs, and embryos for fertility treatments. It is also used in research, including the storage of cell lines and stem cells, and in clinical settings, such as the preservation of skin grafts and corneas for transplantation.

Embryo transfer is a medical procedure that involves the transfer of an embryo, which is typically created through in vitro fertilization (IVF), into the uterus of a woman with the aim of establishing a pregnancy. The embryo may be created using the intended parent's own sperm and eggs or those from donors. After fertilization and early cell division, the resulting embryo is transferred into the uterus of the recipient mother through a thin catheter that is inserted through the cervix. This procedure is typically performed under ultrasound guidance to ensure proper placement of the embryo. Embryo transfer is a key step in assisted reproductive technology (ART) and is often used as a treatment for infertility.

In vitro oocyte maturation (IVM) techniques refer to the process of stimulating and promoting the development and maturation of immature oocytes (eggs) outside of the human body, in a laboratory setting. This procedure is often used in assisted reproductive technology (ART) for individuals or couples who may have difficulty conceiving due to various reasons such as premature ovarian failure, polycystic ovary syndrome (PCOS), or those undergoing cancer treatment.

The IVM process involves the retrieval of immature oocytes from the ovaries, usually through a minor surgical procedure called transvaginal oocyte retrieval. The immature oocytes are then cultured in a laboratory and exposed to specific hormones and nutrients that stimulate their growth and maturation. Once the oocytes have reached full maturity, they can be fertilized with sperm through intracytoplasmic sperm injection (ICSI) or other methods, and the resulting embryos can be transferred to a woman's uterus in the hope of achieving a successful pregnancy.

IVM techniques offer several advantages over traditional in vitro fertilization (IVF) procedures, including reduced medication doses, shorter treatment durations, and lower costs. Additionally, IVM may help minimize the risk of ovarian hyperstimulation syndrome (OHSS), a potentially serious complication associated with conventional ART treatments. However, IVM is still considered an experimental procedure in many countries and requires further research to establish its safety and efficacy for widespread clinical use.

In the field of medicine, "time factors" refer to the duration of symptoms or time elapsed since the onset of a medical condition, which can have significant implications for diagnosis and treatment. Understanding time factors is crucial in determining the progression of a disease, evaluating the effectiveness of treatments, and making critical decisions regarding patient care.

For example, in stroke management, "time is brain," meaning that rapid intervention within a specific time frame (usually within 4.5 hours) is essential to administering tissue plasminogen activator (tPA), a clot-busting drug that can minimize brain damage and improve patient outcomes. Similarly, in trauma care, the "golden hour" concept emphasizes the importance of providing definitive care within the first 60 minutes after injury to increase survival rates and reduce morbidity.

Time factors also play a role in monitoring the progression of chronic conditions like diabetes or heart disease, where regular follow-ups and assessments help determine appropriate treatment adjustments and prevent complications. In infectious diseases, time factors are crucial for initiating antibiotic therapy and identifying potential outbreaks to control their spread.

Overall, "time factors" encompass the significance of recognizing and acting promptly in various medical scenarios to optimize patient outcomes and provide effective care.

Dyneins are a type of motor protein that play an essential role in the movement of cellular components and structures within eukaryotic cells. They are responsible for generating force and motion along microtubules, which are critical components of the cell's cytoskeleton. Dyneins are involved in various cellular processes, including intracellular transport, organelle positioning, and cell division.

There are several types of dyneins, but the two main categories are cytoplasmic dyneins and axonemal dyneins. Cytoplasmic dyneins are responsible for moving various cargoes, such as vesicles, organelles, and mRNA complexes, toward the minus-end of microtubules, which is usually located near the cell center. Axonemal dyneins, on the other hand, are found in cilia and flagella and are responsible for their movement by sliding adjacent microtubules past each other.

Dyneins consist of multiple subunits, including heavy chains, intermediate chains, light-intermediate chains, and light chains. The heavy chains contain the motor domain that binds to microtubules and hydrolyzes ATP to generate force. Dysfunction in dynein proteins has been linked to various human diseases, such as neurodevelopmental disorders, ciliopathies, and cancer.

Nucleic acid hybridization is a process in molecular biology where two single-stranded nucleic acids (DNA, RNA) with complementary sequences pair together to form a double-stranded molecule through hydrogen bonding. The strands can be from the same type of nucleic acid or different types (i.e., DNA-RNA or DNA-cDNA). This process is commonly used in various laboratory techniques, such as Southern blotting, Northern blotting, polymerase chain reaction (PCR), and microarray analysis, to detect, isolate, and analyze specific nucleic acid sequences. The hybridization temperature and conditions are critical to ensure the specificity of the interaction between the two strands.

Brachiaria is a genus of tropical and subtropical grasses that are native to Africa, but have since been introduced and naturalized in many other parts of the world. They are important pasture grasses for grazing livestock, particularly in areas with low soil fertility and high temperatures. Some species of Brachiaria have also been found to have potential as cover crops and for erosion control.

There is no medical definition of 'Brachiaria' as it is a term used in botany and agriculture, not medicine.

Birefringence is a property of certain materials, such as crystals and some plastics, to split a beam of light into two separate beams with different polarization states and refractive indices when the light passes through the material. This phenomenon arises due to the anisotropic structure of these materials, where their physical properties vary depending on the direction of measurement.

When a unpolarized or partially polarized light beam enters a birefringent material, it gets separated into two orthogonally polarized beams called the ordinary and extraordinary rays. These rays propagate through the material at different speeds due to their distinct refractive indices, resulting in a phase delay between them. Upon exiting the material, the recombination of these two beams can produce various optical effects, such as double refraction or interference patterns, depending on the thickness and orientation of the birefringent material and the polarization state of the incident light.

Birefringence has numerous applications in optics, including waveplates, polarizing filters, stress analysis, and microscopy techniques like phase contrast and differential interference contrast imaging.

A nonmammalian embryo refers to the developing organism in animals other than mammals, from the fertilized egg (zygote) stage until hatching or birth. In nonmammalian species, the developmental stages and terminology differ from those used in mammals. The term "embryo" is generally applied to the developing organism up until a specific stage of development that is characterized by the formation of major organs and structures. After this point, the developing organism is referred to as a "larva," "juvenile," or other species-specific terminology.

The study of nonmammalian embryos has played an important role in our understanding of developmental biology and evolutionary developmental biology (evo-devo). By comparing the developmental processes across different animal groups, researchers can gain insights into the evolutionary origins and diversification of body plans and structures. Additionally, nonmammalian embryos are often used as model systems for studying basic biological processes, such as cell division, gene regulation, and pattern formation.

Histones are highly alkaline proteins found in the chromatin of eukaryotic cells. They are rich in basic amino acid residues, such as arginine and lysine, which give them their positive charge. Histones play a crucial role in packaging DNA into a more compact structure within the nucleus by forming a complex with it called a nucleosome. Each nucleosome contains about 146 base pairs of DNA wrapped around an octamer of eight histone proteins (two each of H2A, H2B, H3, and H4). The N-terminal tails of these histones are subject to various post-translational modifications, such as methylation, acetylation, and phosphorylation, which can influence chromatin structure and gene expression. Histone variants also exist, which can contribute to the regulation of specific genes and other nuclear processes.

Cricetinae is a subfamily of rodents that includes hamsters, gerbils, and relatives. These small mammals are characterized by having short limbs, compact bodies, and cheek pouches for storing food. They are native to various parts of the world, particularly in Europe, Asia, and Africa. Some species are popular pets due to their small size, easy care, and friendly nature. In a medical context, understanding the biology and behavior of Cricetinae species can be important for individuals who keep them as pets or for researchers studying their physiology.

Bivalvia is a class of mollusks, also known as "pelecypods," that have a laterally compressed body and two shells or valves. These valves are hinged together on one side and can be opened and closed to allow the animal to feed or withdraw into its shell for protection.

Bivalves include clams, oysters, mussels, scallops, and numerous other species. They are characterized by their simple body structure, which consists of a muscular foot used for burrowing or anchoring, a soft mantle that secretes the shell, and gills that serve both as respiratory organs and feeding structures.

Bivalves play an important role in aquatic ecosystems as filter feeders, helping to maintain water quality by removing particles and organic matter from the water column. They are also commercially important as a source of food for humans and other animals, and their shells have been used historically for various purposes such as tools, jewelry, and building materials.

Salamandridae is not a medical term, but a taxonomic designation in the field of biology. It refers to a family of amphibians commonly known as newts and salamanders. These creatures are characterized by their slender bodies, moist skin, and four legs. Some species have the ability to regenerate lost body parts, including limbs, spinal cord, heart, and more.

If you're looking for a medical term, please provide more context or check if you may have made a typo in your question.

Cell extracts refer to the mixture of cellular components that result from disrupting or breaking open cells. The process of obtaining cell extracts is called cell lysis. Cell extracts can contain various types of molecules, such as proteins, nucleic acids (DNA and RNA), carbohydrates, lipids, and metabolites, depending on the methods used for cell disruption and extraction.

Cell extracts are widely used in biochemical and molecular biology research to study various cellular processes and pathways. For example, cell extracts can be used to measure enzyme activities, analyze protein-protein interactions, characterize gene expression patterns, and investigate metabolic pathways. In some cases, specific cellular components can be purified from the cell extracts for further analysis or application, such as isolating pure proteins or nucleic acids.

It is important to note that the composition of cell extracts may vary depending on the type of cells, the growth conditions, and the methods used for cell disruption and extraction. Therefore, it is essential to optimize the experimental conditions to obtain representative and meaningful results from cell extract studies.

Human chromosomes are thread-like structures that contain genetic material, composed of DNA and proteins, present in the nucleus of human cells. Each chromosome is a single, long DNA molecule that carries hundreds to thousands of genes.

Chromosomes 21, 22, and Y are three of the 23 pairs of human chromosomes. Here's what you need to know about each:

* Chromosome 21 is the smallest human autosomal chromosome, with a total length of about 47 million base pairs. It contains an estimated 200-300 genes and is associated with several genetic disorders, most notably Down syndrome, which occurs when there is an extra copy of this chromosome (trisomy 21).
* Chromosome 22 is the second smallest human autosomal chromosome, with a total length of about 50 million base pairs. It contains an estimated 500-600 genes and is associated with several genetic disorders, including DiGeorge syndrome and cat-eye syndrome.
* The Y chromosome is one of the two sex chromosomes (the other being the X chromosome) and is found only in males. It is much smaller than the X chromosome, with a total length of about 59 million base pairs and an estimated 70-200 genes. The Y chromosome determines maleness by carrying the gene for the testis-determining factor (TDF), which triggers male development in the embryo.

It's worth noting that while we have a standard set of 23 pairs of chromosomes, there can be variations and abnormalities in the number or structure of these chromosomes that can lead to genetic disorders.

Cell nucleus division, also known as nuclear division, is the process by which the genetic material within the cell nucleus, referred to as chromosomes, is separated into two equal sets in preparation for cell division. This process results in the formation of two daughter nuclei, each with a complete set of chromosomes.

There are two types of nuclear division: mitosis and meiosis.

Mitosis is the type of nuclear division that occurs in somatic cells (cells other than sex cells) during growth, repair, and maintenance of tissues. It results in the formation of two genetically identical daughter nuclei. The process of mitosis can be divided into several stages: prophase, prometaphase, metaphase, anaphase, and telophase.

Meiosis, on the other hand, is the type of nuclear division that occurs in sex cells (sperm and egg cells) during sexual reproduction. It results in the formation of four genetically unique daughter nuclei, each with half the number of chromosomes as the parent cell. Meiosis consists of two consecutive divisions: meiosis I and meiosis II.

Both types of nuclear division are essential for the growth, development, and reproduction of living organisms.

A ring chromosome is a structurally abnormal chromosome that has formed a circle or ring shape. This occurs when both ends of the chromosome break off and the resulting fragments join together to form a circular structure. Ring chromosomes can vary in size, and the loss of genetic material during the formation of the ring can lead to genetic disorders and developmental delays. The effects of a ring chromosome depend on the location of the breakpoints and the amount of genetic material lost. Some individuals with ring chromosomes may have mild symptoms, while others may have severe disabilities or health problems.

I'm sorry for any confusion, but "hybrid cells" is not a standard medical term with a widely accepted or specific definition in the field of medicine. The term "hybrid" is used in various scientific and medical contexts to describe combinations or mixtures of different elements, such as hybridoma cells (a type of fusion cell used in research, created by combining a B cell and a tumor cell) or hybridization (in genetics, the process of combining DNA from two different sources).

Without more specific context, it's difficult to provide an accurate medical definition for "hybrid cells." If you could provide more information about the context in which this term was used, I would be happy to help you further!

The synaptonemal complex is a protein structure that forms between two homologous chromosomes during meiosis, the type of cell division that leads to the production of gametes (sex cells). The synaptonemal complex consists of two lateral elements, which are associated with each of the homologous chromosomes, and a central element that runs parallel to the length of the complex and connects the two lateral elements.

The synaptonemal complex plays a crucial role in the process of genetic recombination, which occurs during meiosis. Genetic recombination is the exchange of genetic material between two homologous chromosomes that results in new combinations of genes on the chromosomes. This process helps to increase genetic diversity and is essential for the proper segregation of chromosomes during meiosis.

The synaptonemal complex also helps to ensure that the correct number of chromosomes are distributed to each gamete by holding the homologous chromosomes together until they can be properly aligned and separated during meiosis. Mutations in genes involved in the formation and maintenance of the synaptonemal complex can lead to fertility problems, developmental abnormalities, and other genetic disorders.

... accounts for approximately 4% of the cell cycle's duration.[citation needed] In metaphase, microtubules from both ... "Metaphase plate". Biology Dictionary. Biology Online. Retrieved 9 December 2012. "Metaphase". Nature Education. Retrieved 9 ... The analysis of metaphase chromosomes is one of the main tools of classical cytogenetics and cancer studies. Chromosomes are ... Normal metaphase spreads are used in methods like FISH and as a hybridization matrix for comparative genomic hybridization (CGH ...
ISBN 978-0-671-53136-2. Metaphase. OCLC 26432028. Retrieved August 6, 2020 - via WorldCat. "In Memoriam - Vonda N. McIntyre". ...
The zygote metaphase revisited". BioEssays. 39 (4). doi:10.1002/bies.201600226. PMID 28247957. S2CID 3813188. (Cell anatomy, ...
Cremer T, Lichter P, Borden J, Ward DC, Manuelidis L (November 1988). "Detection of chromosome aberrations in metaphase and ... Distribution in interphase and metaphase". Exp. Cell Res. 124 (1): 111-9. CiteSeerX 10.1.1.490.8109. doi:10.1016/0014-4827(79) ... Lichter the concept of comparative genomic hybridization to metaphase chromosomes and to a matrix with DNA spots representing ...
Paulson JR, Laemmli UK (November 1977). "The structure of histone-depleted metaphase chromosomes". Cell. 12 (3): 817-828. doi: ...
Earnshaw, W. C.; Laemmli, U. K. (1983). "Architecture of metaphase chromosomes and chromosome scaffolds". The Journal of Cell ...
The oocyte now enters meiosis II and remains arrested in metaphase II until fertilization where sister chromatids will separate ... Missegregation of sister chromatids during Metaphase II. Age dependent weakening of sister chromatid cohesion. Matt (2019-09-25 ...
Zhai Y, Kronebusch PJ, Borisy GG (November 1995). "Kinetochore microtubule dynamics and the metaphase-anaphase transition". The ...
It begins with the regulated triggering of the metaphase-to-anaphase transition. Metaphase ends with the destruction of B ... Interphase Prophase Prometaphase Metaphase Telophase Cytoskeleton Anaphase I Anaphase II Cdc20 "Chromosome condensation through ... is the stage of mitosis after the process of metaphase, when replicated chromosomes are split and the newly-copied chromosomes ... which is required for the function of metaphase cyclin-dependent kinases (M-Cdks). In essence, Activation of the Anaphase- ...
A single metaphase cell is isolated from solution. The chromosomes are then released from the nucleus, and the cytoplasm is ... In addition, this method is only applicable to cells in metaphase, which inherently limits the technique to cell types and ... As with the above technique microdissection begins with metaphase cells. The nucleus is lysed mechanically on a glass slide and ... Microfluidic whole genome haplotyping is a technique for the physical separation of individual chromosomes from a metaphase ...
"Infrared nanospectroscopic mapping of a single metaphase chromosome". Nucleic Acids Research. 47 (18): e108. doi:10.1093/nar/ ...
Metaphase: The centrosomes have moved to the poles of the cell and have established the mitotic spindle. The chromosomes have ... The resulting tension causes the chromosomes to align along the metaphase plate or equatorial plane, an imaginary line that is ... In animal cells, a cleavage furrow (pinch) containing a contractile ring, develops where the metaphase plate used to be, ... If the cell successfully passes through the metaphase checkpoint, it proceeds to anaphase. During anaphase A, the cohesins that ...
Thus at metaphase, when all chromosomes are aligned at the metaphase plate, all checkpoint proteins are released from the ... At metaphase, CENP-E, Bub3 and Bub1 levels diminish by a factor of about three to four as compared with free kinetochores, ... At metaphase, CENP-E, Bub3 and Bub1 levels decreases 3 to 4 fold as compared to the levels at unattached kinetochores, whereas ... Following the transition from metaphase to anaphase, the sister chromatids separate from each other, and the individual ...
Zech, Lore (December 1969). "Investigation of metaphase chromosomes with DNA-binding flurochromes". Exp Cell Res. 58 (2-3): 463 ... first reported intense fluorescence of the A T-rich distal half of the long arm of the Y chromosome in the nuclei of metaphase ...
The independent orientation of homologous chromosome pairs along the metaphase plate during metaphase I and orientation of ... The new equatorial metaphase plate is rotated by 90 degrees when compared to meiosis I, perpendicular to the previous plate. ... In metaphase II, the centromeres contain two kinetochores that attach to spindle fibers from the centrosomes at opposite poles ... During this process, the maturing oocytes resume meiosis and continue until metaphase II of meiosis II, where they are again ...
In an alternative technique to interphase or metaphase preparations, fiber FISH, interphase chromosomes are attached to a slide ... Then, an interphase or metaphase chromosome preparation is produced. The chromosomes are firmly attached to a substrate, ... A traditional exam involving metaphase chromosome analysis is often unable to identify features that distinguish one disease ... a trained technologist is required to distinguish subtle differences in banding patterns on bent and twisted metaphase ...
The meiotic cycle of the oocyte was suspended in metaphase of the second meiotic division. Once PLCζ is introduced into the ... Chromosomes then orientate on the metaphase spindle for mitosis. This combination of the two genomes is called syngamy. The ...
During metaphase, the chromosomes line up using the spindle apparatus in the middle of the cell along the equatorial plate. The ... Mitosis includes four phases: prophase, metaphase, anaphase, and telophase. Prophase is the initial phase when spindle fibers ...
Prophase Prometaphase Metaphase Anaphase Telophase Cytoskeleton Marieb E (2000). Essentials of human anatomy and physiology. ...
Upon fertilization, the metaphase arrest is released by the action of Ca2+ ions released from the endoplasmic reticulum, ... The cell cycle of unfertilized eggs of X. laevis is arrested highly synchronously at metaphase of meiosis II. ... "Insights into the micromechanical properties of the metaphase spindle". Cell. 145 (7): 767-778. doi:10.1016/j.cell.2011.05.038 ...
Pflumm, M.F.; Bochtan, M.R. (2001). "Orc mutants arrest in metaphase with abnormally condensed chromosomes". Development. 128 ( ...
The routine chromosome analysis (Karyotyping) refers to analysis of metaphase chromosomes which have been banded using trypsin ... Because prophase and prometaphase chromosomes are more extended than metaphase chromosomes, the number of bands observable for ... High-resolution banding involves the staining of chromosomes during prophase or early metaphase (prometaphase), before they ... For congenital problems usually 20 metaphase cells are scored. Advances now focus on molecular cytogenetics including automated ...
... the metaphase checkpoint, or the mitotic checkpoint, is a cell cycle checkpoint during metaphase of mitosis or meiosis that ... The beginning of metaphase is characterized by the connection of the microtubules to the kinetochores of the chromosomes, as ... Yet in the same study it was shown that, once the transition from metaphase to anaphase is initiated in one part of the cell, ... At the metaphase to anaphase transition, this cohesion between sister chromatids is dissolved, and the separated chromatids are ...
In metaphase, the nucleus takes on a cylindrical shape. Centric mitotic spindles do not reach the poles of the nucleus. The ...
Lau YF, Pfeiffer RA, Arrighi FE, Hsu TC (January 1978). "Combination of silver and fluorescent staining for metaphase ...
At metaphase, when the chromosomes align at the middle plate and are pulled with high tension to either pole by the kinetochore ... At prophase and metaphase, survivin is mainly nuclear in location. During prophase, as the chromatin condenses so that it is ... Moreover, survivin has been shown to localize to components of the mitotic spindle during metaphase and anaphase of mitosis. ...
High Cdc28-Clb levels also initiate DNA replication and duplication of the spindle pole bodies (SPBs). Then the metaphase ...
Wee is a protein that operates at the G2 to metaphase checkpoint. Wee becomes active if errors occur in the DNA synthesis phase ... It blocks entry into metaphase until the problem is resolved. Like Rb, Wee becomes inactive when hyperphosphorylated. In ... Cdc2, part of the metaphase entry checkpoint, is active depending on the pattern of phosphorylation. (Articles lacking sources ...
The product, Metaphase, eventually became the sole property of SDRC. On September 14, 1994, SDRC announced that it would be ... Metaphase is now published under the Teamcenter Enterprise name by Siemens Digital Industries Software. SEC citation (Articles ... I-DEAS is still published by Siemens Digital Industries Software (formerly known as UGS Corp). Metaphase was SDRC's product ...
In conventional CGH, the target is a reference metaphase spread. In array CGH, these targets can be genomic fragments cloned in ... In array CGH, the metaphase chromosomes are replaced by cloned DNA fragments (+100-200 kb) of which the exact chromosomal ... The implementation of array CGH, whereby DNA microarrays are used instead of the traditional metaphase chromosome preparation, ... Because of the limited resolution of metaphase chromosomes, aberrations smaller than 5-10 Mb cannot be detected using ...
Metaphase accounts for approximately 4% of the cell cycles duration.[citation needed] In metaphase, microtubules from both ... "Metaphase plate". Biology Dictionary. Biology Online. Retrieved 9 December 2012. "Metaphase". Nature Education. Retrieved 9 ... The analysis of metaphase chromosomes is one of the main tools of classical cytogenetics and cancer studies. Chromosomes are ... Normal metaphase spreads are used in methods like FISH and as a hybridization matrix for comparative genomic hybridization (CGH ...
Metaphase spread of normal human male chromosomes, showing Y-banding. Light microscope. ... Normal human male metaphase, Y banding. .. Wessex Reg. Genetics Centre. . Attribution 4.0 International (CC BY 4.0). . Source: ... Metaphase spread of normal human male chromosomes, showing Y-banding. Light microscope. ...
Metaphase Technologies LED Backlights ideal for machine vision and systems with limited space, feature no warm-up time, and are ... With twice the brightness, Metaphase Technologies LED Backlights offer a great alternative to Cold Cathode Fluorescent ...
Metaphase Technologies Inc. will have its new dark field line light called the Eclipser on display at Automate 2015. ... Contact:Metaphase Technologies Inc.. Headquarters: Bristol, PA, USA. Product: Eclipser dark field line light. Key features: ... Metaphase Technologies Inc. will have its new dark field line light called the "Eclipser" on display at Automate 2015. ... What Metaphase Technologies says:. View more information on the Eclipser dark field line light. ...
Solo Traveler PlusBryce Rutter2022-06-30T13:26:59-05:00 ...
Infrared nanospectroscopic mapping of a single metaphase chromosome. Nucleic Acids Research. 2019 Oct 10;47(18):e108. doi: ... Infrared nanospectroscopic mapping of a single metaphase chromosome. In: Nucleic Acids Research. 2019 ; Vol. 47, No. 18. ... However, there are no reliable tools to decipher the molecular composition of metaphase chromosomes. Here, we have applied ... We demonstrate the ability of our methodology to locate spatially the presence of anticancer drug sites in metaphase ...
... Asian Journal of Biological Sciences, 3 ... Oocyte metaphase II stages with first polar bodies were separated and then randomly divided into three groups randomly. All ... The effect of osmotic stress on the cell volume, metaphase II spindle and developmental potential of in vitro matured porcine ... Use of Open Pulled Straw as a Carrier in Vitrification of Metaphase II Oocyte in Mice table, th, td { border: 0px solid #ececec ...
It scans the entire slide, locating and capturing the best metaphases and remembering their coordinates, often completing a ... The automatic Metaphase Finder is also supported b ... The automatic Metaphase Finder is also supported by ASIs ... ASIs automatic Metaphase Finder improves workflow efficiency. It scans the entire slide, locating and capturing the best ... ASIs automatic Metaphase Finder improves workflow efficiency. It scans the entire slide, locating and capturing the best ...
The Metabright™ Area Backlight is a high performance and uniform light source for silhouetting and transmissive applications. Using a Full Array LED layout, we can pack more LEDs per square inch to provide greater intensity, uniformity, and performance.. ...
... spindles of vertebrate oocytes must remain stable and correctly organized during the arrest in metaphase II of meiosis. Using ... DOC1R: a MAP kinase substrate that control microtubule organization of metaphase II mouse oocytes. Development (2003) 130 (21 ... Possible involvement of mitogen- and stress-activated protein kinase 1, MSK1, in metaphase-II arrest through phosphorylation of ... Possible Role of p38 MAPK-MNK1-EMI2 Cascade in Metaphase-II Arrest of Mouse Oocytes1 ...
General, 77 to 127 total metaphases of every indicated genotype had been analyzed. * Post author By exposed ... General, 77 to 127 total metaphases of every indicated genotype had been analyzed. We discovered that in Bretazenil individual ...
Rad51cko/neo oocytes at metaphase I and II. (A-C) Centromeric cohesion appears to be normal in mutant oocytes at metaphase I. ... Rad51cko/neo oocytes at metaphase I and II. (A-C) Centromeric cohesion appears to be normal in mutant oocytes at metaphase I. ... A late role for RAD51C in meiotic recombination is revealed at metaphase II. (A and B) Metaphase I chromosomes in control (A) ... A late role for RAD51C in meiotic recombination is revealed at metaphase II. (A and B) Metaphase I chromosomes in control (A) ...
Metaphase➦. Metaphase (from the Greek μετά, "adjacent" and φάσις, "stage") is a stage of mitosis in the eukaryotic cell cycle ... Metaphase➦. (biology) The stage of mitosis and meiosis, that follows prophase and comes before anaphase, during which condensed ... Metaphase➦. The stage of mitosis and meiosis, following prophase and preceding anaphase, during which the chromosomes are ...
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Here is a second possible arrangement of the chromosomes at metaphase. Homologous pair number 1 has aligned itself so that the ... imagine this is the situation in metaphase I. All three maternal chromosomes are attached to the spindle nearer to the lower ... This is a cell during metaphase I. For each pair of chromosomes, any gamete produced by this cell could contain either the ... Tags: metaphase I maternal chromosomes paternal chromosomes gamete homologous chromosomes Metaphase I ANIMATION ...
Metaphase spreads were prepared as described and hybridized to Y-chromosome paint probes (MetaSystems). Metaphases with ... h) Quantification of metaphase fragment dispersion from (g). Data represent individual metaphase spreads with an intact or ... 79 metaphases from 3 independent experiments. j) CIP2A KO cells exhibit increased fragment dispersion on metaphase chromosome ... 44 metaphases from 3 independent experiments. k) CIP2A or TOPBP1 depletion increases fragment dispersion on metaphase ...
Home Tag: Metaphase. Tagged By Metaphase Similarities Between Binary Fission and Cell Division November 14, 2017. , Dr. Mariam ...
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Speak to the children of Israel and you shall say to them that they shall make for themselves fringes on the corners of their garments, throughout their generations, and they shall affix a thread of sky blue [wool] on the fringe of each corner." (Num. 15:38) At the end of the weekly Torah portion Shelach (Num. 13:1-15:41), Torah commands us to attached tzitzit, "tassels," to the four corners of the garment. Reading about the white and blue strings of the tzitzit brought back childhood memories of how I first invented a naïve form of the string theory. It was 1970, as I recall, and I was about 13 years old at the time. Growing up in Russia, alas, I didnt have a Bar Mitzvah, so I wasnt busy studying Torah or preparing for [...]. ...
A previous study showed that pretreatment of mouse oocytes with 3% (0.09 M) sucrose allowed visualization of the metaphase ... Staining of DNA with Hoechst 33342 revealed that these projections coincided with the position of the metaphase chromosomes in ... This study demonstrated that 0.3 M sucrose treatment of bovine oocytes facilitates the localization of metaphase chromosomes ... Oocytes enucleated at the second metaphase stage (MII) are often used as recipient cytoplasts for nuclear transfer. The ...
Metaphase chromatin and division[edit]. See also: mitosis and meiosis. Human chromosomes during metaphase. Stages of early ... During metaphase the X-shaped structure is called a metaphase chromosome, which is highly condensed and thus easiest to ... Arresting mitosis in metaphase by a solution of colchicine. *Pretreating cells in a hypotonic solution 0.075 M KCl, which ... Cells can be locked part-way through division (in metaphase) in vitro (in a reaction vial) with colchicine. These cells are ...
Metaphase Technologies has extensive expertise in engineering flexible lighting solutions for ease of integration into vision ... Metaphase (Lights). For more than two decades, Metaphase Technologies has been developing products that advance "The Quality of ... Metaphase has extensive expertise in engineering flexible lighting solutions for ease of integration into vision systems design ... Metaphase LED illuminators currently profit thousands of applications throughout the world including vision guided robotics, ...
It shows the metaphase plate just about to separate the chromosomes. The chromosomes are white (DAPI stain for DNA), and the ... A deconvolved wide-field fluorescence microscope image of human HeLa cancer cells in metaphase of mitosis. ... It shows the metaphase plate just about to separate the chromosomes. The chromosomes are white (DAPI stain for DNA), and the ... Human HeLa cancer cells, metaphase. by Paul Andrews/Univ. Dundee.. A deconvolved wide-field fluorescence microscope image of ...
他为他的公司带来了超过25年的技术和咨询经验, where he is focused on developing MetaPhases Digital Transformation, 技术现代化和数据分析能力,并共同领导中期创新实验室- ... Prior to MetaPhase, 布雷特曾在包括博思艾伦咨询公司和CGI在内的联邦咨询公司支持大规模的联邦IT项目. He holds a B.A. 在James Madison University获得计算机
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the HANABI-PII More reduces the uptime of the entire harvesting process by 75%, leaving time for other specialized tasks, providing increased throughput for your lab. Capable of processing up to 24 samples per run, eliminates variability compared to manual processing methods.. the HANABI-PII More can be integrated with additional options such as reagent sensors, waste liquid reservoir sensors, additional fixation line and the HANABI-SPI (self-fixing mixer). ...
The HANABI-PII Plus benchmark technology fully automates the multi-step process of preparing and harvesting metaphase cells ... The HANABI-PII Plus Metaphase Chromosome Harvester is designed for todays cytogenetic laboratories that require increased ...
... Wang Xue, Guo Shi-yi, Song Lin-sheng, Fan Ting-yu, Wang ... Abstract: Chromosomal ultrastructure and ribonucleoproteins (RNP) at mitotic metaphase in garlic (Allium sativum L. ) were ... Chromosomal Ribonucleoproteins at Mitotic Metaphase in Allium sativum[J]. J Integr Plant Biol., 1994, 36(7): -. ...
In metaphase, chromosomes align at the metaphase plate.. The most important and critical phase is anaphase which makes sure the ... Metaphase. In metaphase chromosome is a duplicated structure having two sister chromatids, connected at a point called ... Mitosis - Definition, Prophase, Metaphase & More. February 21, 2021. September 24, 2020. by Nimar_geek ... These vesicles originate actually during metaphase, line up in the center of the dividing cell, where they fuse to form ...
  • Metaphase (from Ancient Greek μετα- (meta-) beyond, above, transcending and from Ancient Greek φάσις (phásis) 'appearance') is a stage of mitosis in the eukaryotic cell cycle in which chromosomes are at their second-most condensed and coiled stage (they are at their most condensed in anaphase). (wikipedia.org)
  • Metaphase (from the Greek μετά, "adjacent" and φάσις, "stage") is a stage of mitosis in the eukaryotic cell cycle in which chromosomes are at their second-most condensed and coiled stage (they are at their most condensed in anaphase). (askdifference.com)
  • The stage of mitosis and meiosis, following prophase and preceding anaphase, during which the chromosomes are aligned along the metaphase plate. (askdifference.com)
  • A deconvolved wide-field fluorescence microscope image of human HeLa cancer cells in metaphase of mitosis. (mitosispictures.com)
  • Metaphase: What Happens in this Stage of Mitosis & Meiosis? (sciencing.com)
  • Metaphase is one of the stages of mitosis which is characterized by the appearance of chromosomes due to condensation of duplicated genetic material (chromatin/genomic DNA). (laboratorynotes.com)
  • Mitosis includes prophase, prometaphase, metaphase, and anaphase, as well as telophase, during which chromosome copies are carefully separated in preparation for cytokinesis, where the cytoplasm divides. (coursehero.com)
  • The HANABI-PII Plus Metaphase Chromosome Harvester is designed for today's cytogenetic laboratories that require increased productivity and throughput - plus it delivers the consistent, professional quality you demand every time. (adsbiotec.com)
  • Karyokinesis can further be divided into prophase, metaphase, anaphase, and telophase for thorough understanding, though it is a constant process. (guyhowto.com)
  • Analysis of the mechanism(s) of metaphase I-arrest in strain LT mouse oocytes: delay in the acquisition of competence to undergo the metaphase I/anaphase transition. (jax.org)
  • However, it was found that LT oocytes do not acquire competence to undergo the metaphase I/anaphase transition in response to 6-DMAP until 50-60 min after normal oocytes. (jax.org)
  • MOS-null LT oocytes also exhibit a delay in acquisition of competence to undergo the metaphase I/anaphase transition. (jax.org)
  • Thus, a delay in competence to undergo the metaphase I/anaphase transition in response to 6-DMAP-treatment correlates with metaphase I-arrest. (jax.org)
  • It is therefore hypothesized that the observed delay in acquisition of competence to enter anaphase I may instigate the sustained metaphase I-arrest in LT oocytes by allowing CSF activity to rise to a level that prevents cyclin B degradation and maintains high MPF activity before anaphase can be initiated by normal triggering mechanisms. (jax.org)
  • Chromosomes are normally visible under a light microscope only during the metaphase of cell division (where all chromosomes are aligned in the center of the cell in their condensed form). (wikipedia.org)
  • At the end of metaphase, chromosomes are aligned at the metaphase plate. (laboratorynotes.com)
  • Hypertonic medium treatment for localization of nuclear material in bovine metaphase II oocytes. (ox.ac.uk)
  • Oocytes enucleated at the second metaphase stage (MII) are often used as recipient cytoplasts for nuclear transfer. (ox.ac.uk)
  • A previous study showed that pretreatment of mouse oocytes with 3% (0.09 M) sucrose allowed visualization of the metaphase spindle and chromosomes under standard light microscopy and led to a 100% enucleation rate. (ox.ac.uk)
  • Staining of DNA with Hoechst 33342 revealed that these projections coincided with the position of the metaphase chromosomes in 100% of sucrose-treated oocytes, whereas only 31% of oocytes showed alignment of the position of Pb1 with their nuclear materials. (ox.ac.uk)
  • This study demonstrated that 0.3 M sucrose treatment of bovine oocytes facilitates the localization of metaphase chromosomes under normal light microscopy and hence increases enucleation efficiency without compromising the in vitro development potential of cloned embryos by nuclear transfer. (ox.ac.uk)
  • In this study, we investigated the role of Cdc25B during metaphase II (MII) arrest in mouse oocytes. (molcells.org)
  • Primary spermatocytes are the male germ cells before meiosis I. To examine whether these 4n diploid cells are genetically competent to fertilize oocytes and support full embryo development, we introduced the nuclei of pachytene/diplotene spermatocytes into oocytes that were arrested in prophase I (germinal vesicle stage), metaphase I, or metaphase II (Met II). (elsevierpure.com)
  • After activation of the Met II oocytes that were produced, those microfertilized at metaphase I showed the best developmental ability in vitro, and three of these embryos developed into full-term offspring after embryo transfer. (elsevierpure.com)
  • Fully grown oocytes of most laboratory mice progress without interruption from the germinal vesicle (GV) stage to metaphase II, where meiosis is arrested until fertilization. (jax.org)
  • In contrast, many oocytes of strain LT mice arrest precociously at metaphase I and often undergo subsequent spontaneous parthenogenetic activation. (jax.org)
  • Cytostatic factor (CSF), which prevents the degradation of cyclin B and maintains high maturation-promoting factor (MPF) activity, is required for maintenance of metaphase I-arrest in LT oocytes, similar to its requirement for maintaining metaphase II-arrest in normal oocytes. (jax.org)
  • However, CSF does not instigate metaphase I-arrest since a temporary metaphase I-arrest occurs in MOS-null LT oocytes. (jax.org)
  • A similar delay was observed in strain CX8-4 oocytes, which also have a high incidence of metaphase I-arrest, but not in strain CX8-11 oocytes, which exhibit a low incidence of metaphase I-arrest. (jax.org)
  • First, imagine this is the situation in metaphase I. All three maternal chromosomes are attached to the spindle nearer to the lower pole while the three paternal chromosomes are attached to the spindle nearer to the upper pole. (homeworkclinic.com)
  • The kinetochore fibers of the spindle connect to the kinetochore region at the centromere of the chromosome and align them at the equator of the spindle forming an equatorial plate or metaphase plate. (guyhowto.com)
  • The alignment of chromosomes at the metaphase plate (spindle equator), a plane halfway between the poles of the spindle. (planteome.org)
  • Colcemid, an inhibitor of the mitotic spindle, inhibits the formation of mitotic spindles, thus stopping the segregation of chromosomes and cells remain in the metaphase. (laboratorynotes.com)
  • Tension from spindle fibers aligns chromosomes at the metaphase plate. (cellsalive.com)
  • Cryo-electron tomography and small-angle X-ray scattering were used to investigate the chromatin folding in metaphase chromosomes. (unibas.ch)
  • Chromosomal ultrastructure and ribonucleoproteins (RNP) at mitotic metaphase in garlic (Allium sativum L. ) were studied. (jipb.net)
  • B: First meiotic metaphase. (cdc.gov)
  • E: First meiotic metaphase of the same insect shown in 2D. (cdc.gov)
  • The analysis of metaphase chromosomes is one of the main tools of classical cytogenetics and cancer studies. (wikipedia.org)
  • Preparation of metaphase chromosome spread is an important technique in cytogenetics. (laboratorynotes.com)
  • citation needed] In metaphase, microtubules from both duplicated centrosomes on opposite poles of the cell have completed attachment to kinetochores on condensed chromosomes. (wikipedia.org)
  • In metaphase chromosome is a duplicated structure having two sister chromatids, connected at a point called centromere or primary constriction . (guyhowto.com)
  • Intensity Integrated Laplacian Based Thickness Measurement for Detecting Human Metaphase Chromosome Centromere Location. (cytognomix.com)
  • Accurate detection of the human metaphase chromosome centromere is an important step in many chromosome analysis and medical diagnosis algorithms. (cytognomix.com)
  • The centromeres of the chromosomes convene themselves on the metaphase plate (or equatorial plate), an imaginary line that is equidistant from the two centrosome poles. (wikipedia.org)
  • Three chromosome-specific repetitive probes labeled with either amino acetyl fluorene (AAF), mercury, or biotin were hybridized simultaneously to metaphase chromosomes prepared from human blood lymphocytes or to interphase tumor nuclei. (nih.gov)
  • Cohesin holds the sister CHROMATIDS together during METAPHASE and its cleavage results in chromosome segregation. (bvsalud.org)
  • There's no better place to meet thought leaders," declares speaker Bryce Rutter, PhD, IDSA, of Metaphase in a new video. (core77.com)
  • With twice the brightness, Metaphase Technologies LED Backlights offer a great alternative to Cold Cathode Fluorescent illumination. (edmundoptics.com)
  • Normal metaphase spreads are used in methods like FISH and as a hybridization matrix for comparative genomic hybridization (CGH) experiments. (wikipedia.org)
  • It shows the metaphase plate just about to separate the chromosomes. (mitosispictures.com)
  • In metaphase, chromosomes align at the metaphase plate. (guyhowto.com)
  • Link to all annotated objects annotated to metaphase plate congression. (planteome.org)
  • Link to all direct and indirect annotations to metaphase plate congression. (planteome.org)
  • The metaphase plate depicts strong speckled pattern with some coarse speckles standing out. (cdc.gov)
  • For classical cytogenetic analyses, cells are grown in short term culture and arrested in metaphase using mitotic inhibitor. (wikipedia.org)
  • Malignant cells from solid tumors or leukemia samples can also be used for cytogenetic analysis to generate metaphase preparations. (wikipedia.org)
  • The HANABI-PII Plus benchmark technology fully automates the multi-step process of preparing and harvesting metaphase cells derived from blood and bone marrow cell cultures and from other cell suspension cultures for cytogenetic analysis. (adsbiotec.com)
  • Inspection of the stained metaphase chromosomes allows the determination of numerical and structural changes in the tumor cell genome, for example, losses of chromosomal segments or translocations, which may lead to chimeric oncogenes, such as bcr-abl in chronic myelogenous leukemia. (wikipedia.org)
  • Cells burst when they hit the slide surface, resulting in the release of chromosomes due to lack of nuclear membrane in metaphase cells. (laboratorynotes.com)
  • For more than two decades, Metaphase Technologies has been developing products that advance "The Quality of Light" through engineering and manufacture of uniform diffuse high brightness and ultra brightness LED illuminators for machine vision, military, and specialty lighting applications. (saber1.com)
  • Here, we have applied infrared nanospectroscopy (AFM-IR) to demonstrate molecular difference between eu- and heterochromatin and generate infrared maps of single metaphase chromosomes revealing detailed information on their molecular composition, with nanometric lateral spatial resolution. (monash.edu)
  • Metaphase chromosome spread is used for karyotyping including analysis of numerical or structural changes in chromosomes. (laboratorynotes.com)
  • Metaphase Technologies Inc. will have its new dark field line light called the "Eclipser" on display at Automate 2015. (vision-systems.com)
  • Metaphase Technologies Inc. (vision-systems.com)
  • First, to standardize built-in constant current drivers, Metaphase continues to synergize cutting-edge machine vision LED lighting & control technologies in an effort to simplify innovation and increase customer return on investment. (saber1.com)
  • MetaPhase Consulting was named a 2023 Elev8 GovCon Honoree by Orange Slices AI. (metaphaseconsulting.com)
  • MetaPhase Consulting won SECAF's 2022 Government Contractor of the Year Award in the $27.5M - $50M in revenue category. (metaphaseconsulting.com)
  • As the CEO at MetaPhase Consulting, 弗雷德负责通过"敬业团队"来实现公司的目标, Meaningful Work (faceoff-6.com)
  • Brett McLaren is the Chief Strategy Officer of MetaPhase Consulting. (faceoff-6.com)
  • Prior to MetaPhase, Andy was a Senior Director at Eagle Hill Consulting, Vice President at ICF International, and Managing Consultant at IBM. (faceoff-6.com)
  • Danielle Toole is a Vice President at MetaPhase Consulting. (faceoff-6.com)
  • This is a cell during metaphase I. For each pair of chromosomes, any gamete produced by this cell could contain either the maternal chromosome or the paternal chromosome. (homeworkclinic.com)
  • These metaphase cells are lysed in a controlled manner on a slide that causes the release and spread of chromosomes from individual cells that remain close to each other, thus making it possible to analyze chromosomes from individual cells. (laboratorynotes.com)
  • To lyse metaphase cells in a controlled manner, cells are treated with a hypotonic solution that results in an increase in the volume of cells and cells become prone to lyse upon mechanical stress. (laboratorynotes.com)
  • MDI-GSH also increased the number of cells in metaphase. (cdc.gov)
  • Here is a second possible arrangement of the chromosomes at metaphase. (homeworkclinic.com)
  • The proposed method was observed to be more accurate and statistically significant compared to a centerline based method when tested with 226 human metaphase chromosomes. (cytognomix.com)
  • Methods available in literature yield unreliable results mainly due to high variability of morphology in metaphase chromosomes and boundary noise present in the image. (cytognomix.com)
  • However, there are no reliable tools to decipher the molecular composition of metaphase chromosomes. (monash.edu)
  • Metaphase has extensive expertise in engineering flexible lighting solutions for ease of integration into vision systems design. (saber1.com)
  • Chromosomes are condensed (thickened) and highly coiled in metaphase, which makes them most suitable for visual analysis. (wikipedia.org)
  • The automatic Metaphase Finder is also supported by ASI's robotic tray loader, allowing 81 slides to be loaded in a single batch, reloaded without disrupting system operation, and providing labs with 24x7 continuous scanning and analysis. (dssimage.com)
  • MetaPhase works at the intersection of business-to-IT partnerships-creating, deploying, and supporting practical solutions that serve as a force multiplier for government. (metaphaseconsulting.com)
  • Metaphase is the third of the five phases of biological cell division, or more specifically, the division of what is inside that cell's nucleus. (sciencing.com)
  • and fluorescent in, situ hybridization (FISH) to metaphase chromosomes revealed an insertion of part of chromosome 16 on chromosome 11. (lu.se)
  • During metaphase the X-shaped structure is called a metaphase chromosome, which is highly condensed and thus easiest to distinguish and study. (wikipedia.org)
  • Each of these in turn includes its own metaphase, appropriately named metaphase I and metaphase II. (sciencing.com)
  • This is a general protocol for the preparation of metaphase chromosomes spread from any adherent cell lines. (laboratorynotes.com)