Antibodies, Heterophile
Antigens, Heterophile
Infectious Mononucleosis
Forssman Antigen
Antibodies
Immunoconglutinins
Hemagglutination Tests
Latex Fixation Tests
False Positive Reactions
Antibody Specificity
Immunoassay
Immunoglobulin M
Immunoglobulin G
Reagent Kits, Diagnostic
Herpesvirus 4, Human
Antibody Formation
Antibodies, Neutralizing
Antibody Affinity
Fluorescent Antibody Technique
Antibodies, Anti-Idiotypic
Binding Sites, Antibody
When is a heterophile antibody not a heterophile antibody? When it is an antibody against a specific immunogen. (1/250)
Heterophile antibodies are antibodies produced against poorly defined antigens. These are generally weak antibodies with multispecific activities. Human anti-animal antibodies that develop as a result of treatments with animal immunoglobulins are antibodies with strong avidities, produced against well-defined antigens. Although heterophile antibodies and human anti-animal antibodies interfere with immunological assays by similar mechanisms, modes for identifying the sources of the antibodies and for circumventing or retarding the interference may differ. Unfortunately, there has not been a well-organized attempt to encourage correct definition of these antibodies. This problem of inexact definition is highlighted by recent articles in this Journal. In the present discussion, we examine the history leading to this problem and discuss the origins and the reasons that the nature of the antibody is important for rectifying the problem. We propose a simple nomenclature for general usage that should appropriately characterize these antibodies in most cases. (+info)Heterotypic protection and induction of a broad heterotypic neutralization response by rotavirus-like particles. (2/250)
The recognition that rotaviruses are the major cause of life-threatening diarrheal disease and significant morbidity in young children has focused efforts on disease prevention and control of these viruses. Although the correlates of protection in children remain unclear, some studies indicate that serotype-specific antibody is important. Based on this premise, current live attenuated reassortant rotavirus vaccines include the four predominant serotypes of virus. We are evaluating subunit rotavirus vaccines, 2/6/7-VLPs and 2/4/6/7-VLPs, that contain only a single VP7 of serotype G1 or G3. In mice immunized parenterally twice, G3 virus-like particles (VLPs) induced a homotypic, whereas G1 VLPs induced a homotypic and heterotypic (G3) serum neutralizing immune response. Administration of three doses of G1 or G3 VLPs induced serum antibodies that neutralized five of seven different serotype test viruses. The inclusion of VP4 in the VLPs was not essential for the induction of heterotypic neutralizing antibody in mice. To confirm these results in another species, rabbits were immunized parenterally with two doses of 2/4/6/7-VLPs containing a G3 or G1 VP7, sequentially with G3 VLPs followed by G1 (G3/G1) VLPs, or with live or psoralen-inactivated SA11. High-titer homotypic serum neutralizing antibody was induced in all rabbits, and low-level heterotypic neutralizing antibody was induced in a subset of rabbits. The rabbits immunized with the G1 or G3/G1 VLPs in QS-21 were challenged orally with live G3 ALA rotavirus. Protection levels were similar in rabbits immunized with homotypic G3 2/4/6/7-VLPs, heterotypic G1 2/4/6/7-VLPs, or G3/G1 2/4/6/7-VLPs. Therefore, G1 2/4/6/7-VLPs can induce protective immunity against a live heterotypic rotavirus challenge in an adjuvant with potential use in humans. Following challenge, broad serum heterotypic neutralizing antibody responses were detected in rabbits parenterally immunized with G1, G3/G1, or G3 VLPs but not with SA11. Immunization with VLPs may provide sufficient priming of the immune system to induce protective anamnestic heterotypic neutralizing antibody responses upon subsequent rotavirus infection. Therefore, a limited number of serotypes of VLPs may be sufficient to provide a broadly protective subunit vaccine. (+info)Enhancement of haemolysis by Newcastle disease virus (NDV) after pre-treatment with heterophile antibody and complement. (3/250)
Pre-treatment of Newcastle disease virus (NDV) with fresh human plasma enhances its haemolytic (HL) capacity by several factors. The effect is due to complement activation by the heterophile anti-chick antibody present in human plasma. All the adult human plasmas tested were effective, also 91/100 human cord blood sera. The antibody was mainly of the IgM class. The enhanced HL was due to integration and transference of the complement 'holed' virus envelope membrane and subsequent leakage of haemoglobin. High concentration of activated complement destroys the integrity of the virus enevelope. Treatment of chick erythrocytes and fibroblasts with human plasma also produced lysis of the cells. (+info)Heterophile antibodies to bovine and caprine proteins causing false-positive human immunodeficiency virus type 1 and other enzyme-linked immunosorbent assay results. (4/250)
Heterophile antibodies are a well-recognized cause of erroneous results in immunoassays. We describe here a 22-month-old child with heterophile antibodies reactive with bovine serum albumin and caprine proteins causing false-positive results to human immunodeficiency virus type 1 and other infectious serology testing. (+info)Heterophile antibodies segregate in families and are associated with protection from type 1 diabetes. (5/250)
Markedly elevated levels of serum IL-4 were reported previously in 50% of a small group of type 1 diabetes nonprogessors. To determine the patterns of expression for this phenotype, a larger cohort of 58 families containing type 1 diabetic patients was examined. Analysis of the two-site ELISA assay used to measure serum IL-4 revealed evidence for heterophile antibodies, i.e., nonanalyte substances in serum capable of binding antibodies mutivalently and providing erroneous analyte (e.g., IL-4) quantification. Interestingly, relatives without type 1 diabetes were significantly more likely to have this phenotype than were patients with the disease (P = 0.003). In addition, the trait appears to have clustered within certain families and was associated with the protective MHC allele DQB1*0602 (P = 0.008). These results suggest that heterophile antibodies represent an in vivo trait associated with self-tolerance and nonprogression to diabetes. (+info)An immunoadhesin incorporating the molecule OX-2 is a potent immunosuppressant that prolongs allo- and xenograft survival. (6/250)
We have established that, in mice receiving donor-specific immunization by the portal vein, the increased graft survival seen is associated with the increased expression of a molecule (OX-2) on a subpopulation of dendritic cells (DC), and polarization of cytokine production to type 2 cytokines on Ag-specific restimulation of cells from these mice. Furthermore, infusion of a mAb to OX-2 blocks both the increased graft survival and the altered cytokine production seen. We have constructed an immunoadhesin in which the extracellular domain of OX-2 is linked to the murine IgG2a Fc region, and we have expressed this molecule (OX-2:Fc) in a eukaryotic (baculovirus) expression system. Incubation of lymphocytes with 50 ng/ml OX-2:Fc inhibits a primary mixed lymphocyte reaction in vitro, as assayed by proliferation and induction of cytotoxic T cells, and also alters cytokine production with decreased IL-2 (IFN-gamma) production and increased IL-4 (IL-10) production. Similarly, in vivo infusion of OX-2:Fc promotes increased allo- and xenograft (both skin and renal grafts) survival and decreases the Ab response to sheep erythrocytes. Our data suggest this molecule might have clinical importance in allo- and xenotransplantation. (+info)Accelerated development and aging of the immune system in p53-deficient mice. (7/250)
Development and aging of the immune system lead to an accumulation of memory T cells over the long term. The predominance of T cells of the memory phenotype in the T cell population induces an age-related decline in protective immune responses. We found that development and aging of the immune system were accelerated in p53-deficient (p53-/-) mice; the accumulation of memory T cells was spontaneously accelerated, and a strong T cell-dependent Ab response and Th2 cytokine expression (IL-4, IL-6, and IL-10) were induced by Ag stimulation in young p53-/- mice in the developmental stage. The high T cell proliferative response in the young mice rapidly progressed to a depressed proliferative response in adult mice. It was suggested that the loss of regulation of the cell cycle, DNA repair, and apoptosis by p53 deficiency potentially leads to immunosenescence with the accumulation of memory T cells. (+info)Accommodated xenografts survive in the presence of anti-donor antibodies and complement that precipitate rejection of naive xenografts. (8/250)
Hamster hearts transplanted into transiently complement-depleted and continuously cyclosporin A (CyA)-immunosuppressed rats survive long-term despite deposition of anti-donor IgM Abs and complement on the graft vascular endothelium. This phenomenon is referred to as "accommodation." The hypothesis tested here is that accommodated xenografts are resistant to IgM Abs and complement that could result in rejection of naive xenografts. After first hamster hearts had been surviving in cobra venom factor (CVF) + CyA-treated rats for 10 days, a time when the anti-donor IgM Ab level was maximal and complement activity had returned to approximately 50% of pretreatment levels, naive hamster hearts or hamster hearts that had been accommodating in another rat for 14 days were transplanted into those rats carrying the surviving first graft. The naive hearts were all hyperacutely rejected. In contrast, a majority of regrafted accommodating hearts survived long-term. There was widespread Ab and activated complement deposition on the vascular endothelium of accommodating first hearts, second accommodating hearts, and rejected second naive hearts. However, only the rejected naive hearts showed extensive endothelial cell damage, myocardial necrosis, fibrin deposition, and other signs of inflammation. Accommodating first and second hearts but not rejected second naive hearts expressed high levels of the protective genes A20, heme oxygenase-1 (HO-1), bcl-2, and bcl-xL. These data demonstrate that accommodated xenografts become resistant to effects of anti-donor IgM Abs and complement that normally mediate rejection of xenografts. We hypothesize that this resistance involves expression by accommodated xenografts of protective genes. (+info)Heterophile antibodies are a type of antibody that can react with antigens from more than one source, rather than being specific to a single antigen. They are produced in response to an initial infection or immunization, but can also cross-react with antigens from unrelated organisms or substances. A common example of heterophile antibodies are those that are produced in response to Epstein-Barr virus (EBV) infection, which can cause infectious mononucleosis. These antibodies, known as Paul-Bunnell antibodies, can agglutinate (clump together) sheep or horse red blood cells, which is the basis for a diagnostic test for EBV infection called the Monospot test. However, it's important to note that not all cases of infectious mononucleosis are caused by EBV, and other infections or conditions can also cause the production of heterophile antibodies, leading to false-positive results.
Heterophile antigens are a type of antigen that can induce an immune response in multiple species, not just the one they originate from. They are called "heterophile" because they exhibit cross-reactivity with antibodies produced against different antigens from other species. A common example of heterophile antigens is the Forssman antigen, which can be found in various animals such as guinea pigs, rabbits, and humans.
Heterophile antibody tests are often used in diagnostic medicine to detect certain infections or autoimmune disorders. One well-known example is the Paul-Bunnell test, which was historically used to diagnose infectious mononucleosis (IM) caused by the Epstein-Barr virus (EBV). The test detects heterophile antibodies produced against EBV antigens that cross-react with sheep red blood cells. However, this test has been largely replaced by more specific and sensitive EBV antibody tests.
It is important to note that heterophile antibody tests can sometimes produce false positive results due to the presence of these cross-reactive antibodies in individuals who have not been infected with the targeted pathogen. Therefore, it is crucial to interpret test results cautiously and consider them alongside clinical symptoms, medical history, and other diagnostic findings.
Infectious Mononucleosis, also known as "mono" or the "kissing disease," is a common infectious illness caused by the Epstein-Barr virus (EBV). It primarily affects adolescents and young adults. The medical definition of Infectious Mononucleosis includes the following signs and symptoms:
1. Infection: Infectious Mononucleosis is an infection that spreads through saliva, hence the nickname "kissing disease." It can also be transmitted through sharing food, drinks, or personal items such as toothbrushes or utensils with an infected person.
2. Incubation period: The incubation period for Infectious Mononucleosis is typically 4-6 weeks after exposure to the virus.
3. Symptoms: Common symptoms of Infectious Mononucleosis include fever, sore throat (often severe and may resemble strep throat), fatigue, swollen lymph nodes (particularly in the neck and armpits), and skin rash (in some cases).
4. Diagnosis: The diagnosis of Infectious Mononucleosis is typically made based on a combination of clinical symptoms, physical examination findings, and laboratory test results. A complete blood count (CBC) may reveal an increased number of white blood cells, particularly atypical lymphocytes. Additionally, the Paul-Bunnell or Monospot test can detect heterophile antibodies, which are present in about 85% of cases after the first week of illness.
5. Treatment: There is no specific antiviral treatment for Infectious Mononucleosis. Management typically involves supportive care, such as rest, hydration, and pain relief for symptoms like sore throat and fever.
6. Complications: Although most cases of Infectious Mononucleosis resolve without significant complications, some individuals may experience complications such as splenomegaly (enlarged spleen), hepatitis, or neurological issues. Rarely, the virus can cause more severe complications like myocarditis (inflammation of the heart muscle) or hemolytic anemia (destruction of red blood cells).
7. Prevention: Preventing Infectious Mononucleosis is difficult since it is primarily spread through respiratory droplets and saliva. However, practicing good hygiene, such as covering the mouth and nose when coughing or sneezing and avoiding sharing personal items like utensils or drinking glasses, can help reduce the risk of transmission.
The Forssman antigen is a type of heterophile antigen, which is a substance that can stimulate an immune response in animals of different species. It was first discovered by the Swedish bacteriologist, John Forssman, in 1911. The Forssman antigen is found in a variety of tissues and organs, including the kidney, liver, and brain, in many different animal species, including humans.
The Forssman antigen is unique because it can induce the production of antibodies that cross-react with tissues from other species. This means that an immune response to the Forssman antigen in one species can also recognize and react with similar antigens in another species, leading to the possibility of cross-species immune reactions.
The Forssman antigen is a complex glycosphingolipid molecule that is found on the surface of cells. It is not clear what role, if any, the Forssman antigen plays in normal physiological processes. However, its presence has been implicated in various disease processes, including autoimmune disorders and transplant rejection.
In summary, the Forssman antigen is a heterophile antigen found in a variety of tissues and organs in many different animal species, including humans. It can induce cross-reacting antibodies and has been implicated in various disease processes.
Antibodies are proteins produced by the immune system in response to the presence of a foreign substance, such as a bacterium or virus. They are capable of identifying and binding to specific antigens (foreign substances) on the surface of these invaders, marking them for destruction by other immune cells. Antibodies are also known as immunoglobulins and come in several different types, including IgA, IgD, IgE, IgG, and IgM, each with a unique function in the immune response. They are composed of four polypeptide chains, two heavy chains and two light chains, that are held together by disulfide bonds. The variable regions of the heavy and light chains form the antigen-binding site, which is specific to a particular antigen.
Immunoconglutinins are a type of immunoglobulin (a kind of antibody) that can bind to complement components, particularly C3b and C4b, which have been deposited on immune complexes or other structures in the body. They are part of the immune system's response to inflammation and help to remove immune complexes from the bloodstream. Immunoconglutinins can be detected in the serum and are often used as a marker of immune activation, particularly in conditions associated with immune complex formation such as autoimmune diseases or infections.
Antibodies, viral are proteins produced by the immune system in response to an infection with a virus. These antibodies are capable of recognizing and binding to specific antigens on the surface of the virus, which helps to neutralize or destroy the virus and prevent its replication. Once produced, these antibodies can provide immunity against future infections with the same virus.
Viral antibodies are typically composed of four polypeptide chains - two heavy chains and two light chains - that are held together by disulfide bonds. The binding site for the antigen is located at the tip of the Y-shaped structure, formed by the variable regions of the heavy and light chains.
There are five classes of antibodies in humans: IgA, IgD, IgE, IgG, and IgM. Each class has a different function and is distributed differently throughout the body. For example, IgG is the most common type of antibody found in the bloodstream and provides long-term immunity against viruses, while IgA is found primarily in mucous membranes and helps to protect against respiratory and gastrointestinal infections.
In addition to their role in the immune response, viral antibodies can also be used as diagnostic tools to detect the presence of a specific virus in a patient's blood or other bodily fluids.
Hemagglutination tests are laboratory procedures used to detect the presence of antibodies or antigens in a sample, typically in blood serum. These tests rely on the ability of certain substances, such as viruses or bacteria, to agglutinate (clump together) red blood cells.
In a hemagglutination test, a small amount of the patient's serum is mixed with a known quantity of red blood cells that have been treated with a specific antigen. If the patient has antibodies against that antigen in their serum, they will bind to the antigens on the red blood cells and cause them to agglutinate. This clumping can be observed visually, indicating a positive test result.
Hemagglutination tests are commonly used to diagnose infectious diseases caused by viruses or bacteria that have hemagglutinating properties, such as influenza, parainfluenza, and HIV. They can also be used in blood typing and cross-matching before transfusions.
Latex fixation tests are diagnostic procedures used to detect the presence of certain antigens or antibodies in a patient's sample, such as blood or serum. These tests use latex particles that are coated with specific antigens or antibodies that can bind to complementary antigens or antibodies present in the sample. When the sample is added to the latex reagent, if the specific antigen or antibody is present, they will bind to the latex particles, forming an agglutination reaction that can be seen as a visible clumping or agglutination of the latex particles.
Latex fixation tests are commonly used in the diagnosis of infectious diseases, autoimmune disorders, and genetic disorders. For example, a latex fixation test may be used to detect the presence of Streptococcus pneumoniae antigens in a patient's sputum sample or to identify the presence of rheumatoid factor (RF) antibodies in a patient's blood sample. These tests are known for their simplicity, speed, and sensitivity, making them a valuable tool in clinical laboratories.
A "false positive reaction" in medical testing refers to a situation where a diagnostic test incorrectly indicates the presence of a specific condition or disease in an individual who does not actually have it. This occurs when the test results give a positive outcome, while the true health status of the person is negative or free from the condition being tested for.
False positive reactions can be caused by various factors including:
1. Presence of unrelated substances that interfere with the test result (e.g., cross-reactivity between similar molecules).
2. Low specificity of the test, which means it may detect other conditions or irrelevant factors as positive.
3. Contamination during sample collection, storage, or analysis.
4. Human errors in performing or interpreting the test results.
False positive reactions can have significant consequences, such as unnecessary treatments, anxiety, and increased healthcare costs. Therefore, it is essential to confirm any positive test result with additional tests or clinical evaluations before making a definitive diagnosis.
Antibody specificity refers to the ability of an antibody to bind to a specific epitope or antigenic determinant on an antigen. Each antibody has a unique structure that allows it to recognize and bind to a specific region of an antigen, typically a small portion of the antigen's surface made up of amino acids or sugar residues. This highly specific binding is mediated by the variable regions of the antibody's heavy and light chains, which form a pocket that recognizes and binds to the epitope.
The specificity of an antibody is determined by its unique complementarity-determining regions (CDRs), which are loops of amino acids located in the variable domains of both the heavy and light chains. The CDRs form a binding site that recognizes and interacts with the epitope on the antigen. The precise fit between the antibody's binding site and the epitope is critical for specificity, as even small changes in the structure of either can prevent binding.
Antibody specificity is important in immune responses because it allows the immune system to distinguish between self and non-self antigens. This helps to prevent autoimmune reactions where the immune system attacks the body's own cells and tissues. Antibody specificity also plays a crucial role in diagnostic tests, such as ELISA assays, where antibodies are used to detect the presence of specific antigens in biological samples.
An immunoassay is a biochemical test that measures the presence or concentration of a specific protein, antibody, or antigen in a sample using the principles of antibody-antigen reactions. It is commonly used in clinical laboratories to diagnose and monitor various medical conditions such as infections, hormonal disorders, allergies, and cancer.
Immunoassays typically involve the use of labeled reagents, such as enzymes, radioisotopes, or fluorescent dyes, that bind specifically to the target molecule. The amount of label detected is proportional to the concentration of the target molecule in the sample, allowing for quantitative analysis.
There are several types of immunoassays, including enzyme-linked immunosorbent assay (ELISA), radioimmunoassay (RIA), fluorescence immunoassay (FIA), and chemiluminescent immunoassay (CLIA). Each type has its own advantages and limitations, depending on the sensitivity, specificity, and throughput required for a particular application.
Bacterial antibodies are a type of antibodies produced by the immune system in response to an infection caused by bacteria. These antibodies are proteins that recognize and bind to specific antigens on the surface of the bacterial cells, marking them for destruction by other immune cells. Bacterial antibodies can be classified into several types based on their structure and function, including IgG, IgM, IgA, and IgE. They play a crucial role in the body's defense against bacterial infections and provide immunity to future infections with the same bacteria.
Monoclonal antibodies are a type of antibody that are identical because they are produced by a single clone of cells. They are laboratory-produced molecules that act like human antibodies in the immune system. They can be designed to attach to specific proteins found on the surface of cancer cells, making them useful for targeting and treating cancer. Monoclonal antibodies can also be used as a therapy for other diseases, such as autoimmune disorders and inflammatory conditions.
Monoclonal antibodies are produced by fusing a single type of immune cell, called a B cell, with a tumor cell to create a hybrid cell, or hybridoma. This hybrid cell is then able to replicate indefinitely, producing a large number of identical copies of the original antibody. These antibodies can be further modified and engineered to enhance their ability to bind to specific targets, increase their stability, and improve their effectiveness as therapeutic agents.
Monoclonal antibodies have several mechanisms of action in cancer therapy. They can directly kill cancer cells by binding to them and triggering an immune response. They can also block the signals that promote cancer growth and survival. Additionally, monoclonal antibodies can be used to deliver drugs or radiation directly to cancer cells, increasing the effectiveness of these treatments while minimizing their side effects on healthy tissues.
Monoclonal antibodies have become an important tool in modern medicine, with several approved for use in cancer therapy and other diseases. They are continuing to be studied and developed as a promising approach to treating a wide range of medical conditions.
Immunoglobulin M (IgM) is a type of antibody that is primarily found in the blood and lymph fluid. It is the first antibody to be produced in response to an initial exposure to an antigen, making it an important part of the body's primary immune response. IgM antibodies are large molecules that are composed of five basic units, giving them a pentameric structure. They are primarily found on the surface of B cells as membrane-bound immunoglobulins (mlgM), where they function as receptors for antigens. Once an mlgM receptor binds to an antigen, it triggers the activation and differentiation of the B cell into a plasma cell that produces and secretes large amounts of soluble IgM antibodies.
IgM antibodies are particularly effective at agglutination (clumping) and complement activation, which makes them important in the early stages of an immune response to help clear pathogens from the bloodstream. However, they are not as stable or long-lived as other types of antibodies, such as IgG, and their levels tend to decline after the initial immune response has occurred.
In summary, Immunoglobulin M (IgM) is a type of antibody that plays a crucial role in the primary immune response to antigens by agglutination and complement activation. It is primarily found in the blood and lymph fluid, and it is produced by B cells after they are activated by an antigen.
Immunoglobulin G (IgG) is a type of antibody, which is a protective protein produced by the immune system in response to foreign substances like bacteria or viruses. IgG is the most abundant type of antibody in human blood, making up about 75-80% of all antibodies. It is found in all body fluids and plays a crucial role in fighting infections caused by bacteria, viruses, and toxins.
IgG has several important functions:
1. Neutralization: IgG can bind to the surface of bacteria or viruses, preventing them from attaching to and infecting human cells.
2. Opsonization: IgG coats the surface of pathogens, making them more recognizable and easier for immune cells like neutrophils and macrophages to phagocytose (engulf and destroy) them.
3. Complement activation: IgG can activate the complement system, a group of proteins that work together to help eliminate pathogens from the body. Activation of the complement system leads to the formation of the membrane attack complex, which creates holes in the cell membranes of bacteria, leading to their lysis (destruction).
4. Antibody-dependent cellular cytotoxicity (ADCC): IgG can bind to immune cells like natural killer (NK) cells and trigger them to release substances that cause target cells (such as virus-infected or cancerous cells) to undergo apoptosis (programmed cell death).
5. Immune complex formation: IgG can form immune complexes with antigens, which can then be removed from the body through various mechanisms, such as phagocytosis by immune cells or excretion in urine.
IgG is a critical component of adaptive immunity and provides long-lasting protection against reinfection with many pathogens. It has four subclasses (IgG1, IgG2, IgG3, and IgG4) that differ in their structure, function, and distribution in the body.
Reagent kits, diagnostic are prepackaged sets of chemical reagents and other components designed for performing specific diagnostic tests or assays. These kits are often used in clinical laboratories to detect and measure the presence or absence of various biomarkers, such as proteins, antibodies, antigens, nucleic acids, or small molecules, in biological samples like blood, urine, or tissues.
Diagnostic reagent kits typically contain detailed instructions for their use, along with the necessary reagents, controls, and sometimes specialized equipment or supplies. They are designed to simplify the testing process, reduce human error, and increase standardization, ensuring accurate and reliable results. Examples of diagnostic reagent kits include those used for pregnancy tests, infectious disease screening, drug testing, genetic testing, and cancer biomarker detection.
Medical Definition of "Herpesvirus 4, Human" (Epstein-Barr Virus)
"Herpesvirus 4, Human," also known as Epstein-Barr virus (EBV), is a member of the Herpesviridae family and is one of the most common human viruses. It is primarily transmitted through saliva and is often referred to as the "kissing disease."
EBV is the causative agent of infectious mononucleosis (IM), also known as glandular fever, which is characterized by symptoms such as fatigue, sore throat, fever, and swollen lymph nodes. The virus can also cause other diseases, including certain types of cancer, such as Burkitt's lymphoma, Hodgkin's lymphoma, and nasopharyngeal carcinoma.
Once a person becomes infected with EBV, the virus remains in the body for the rest of their life, residing in certain white blood cells called B lymphocytes. In most people, the virus remains dormant and does not cause any further symptoms. However, in some individuals, the virus may reactivate, leading to recurrent or persistent symptoms.
EBV infection is diagnosed through various tests, including blood tests that detect antibodies against the virus or direct detection of the virus itself through polymerase chain reaction (PCR) assays. There is no cure for EBV infection, and treatment is generally supportive, focusing on relieving symptoms and managing complications. Prevention measures include practicing good hygiene, avoiding close contact with infected individuals, and not sharing personal items such as toothbrushes or drinking glasses.
Antibody formation, also known as humoral immune response, is the process by which the immune system produces proteins called antibodies in response to the presence of a foreign substance (antigen) in the body. This process involves several steps:
1. Recognition: The antigen is recognized and bound by a type of white blood cell called a B lymphocyte or B cell, which then becomes activated.
2. Differentiation: The activated B cell undergoes differentiation to become a plasma cell, which is a type of cell that produces and secretes large amounts of antibodies.
3. Antibody production: The plasma cells produce and release antibodies, which are proteins made up of four polypeptide chains (two heavy chains and two light chains) arranged in a Y-shape. Each antibody has two binding sites that can recognize and bind to specific regions on the antigen called epitopes.
4. Neutralization or elimination: The antibodies bind to the antigens, neutralizing them or marking them for destruction by other immune cells. This helps to prevent the spread of infection and protect the body from harmful substances.
Antibody formation is an important part of the adaptive immune response, which allows the body to specifically recognize and respond to a wide variety of pathogens and foreign substances.
Neutralizing antibodies are a type of antibody that defends against pathogens such as viruses or bacteria by neutralizing their ability to infect cells. They do this by binding to specific regions on the surface proteins of the pathogen, preventing it from attaching to and entering host cells. This renders the pathogen ineffective and helps to prevent or reduce the severity of infection. Neutralizing antibodies can be produced naturally in response to an infection or vaccination, or they can be generated artificially for therapeutic purposes.
Antibody affinity refers to the strength and specificity of the interaction between an antibody and its corresponding antigen at a molecular level. It is a measure of how strongly and selectively an antibody binds to its target antigen. A higher affinity indicates a more stable and specific binding, while a lower affinity suggests weaker and less specific interactions. Affinity is typically measured in terms of the dissociation constant (Kd), which describes the concentration of antigen needed to achieve half-maximal binding to an antibody. Generally, a smaller Kd value corresponds to a higher affinity, indicating a tighter and more selective bond. This parameter is crucial in the development of diagnostic and therapeutic applications, such as immunoassays and targeted therapies, where high-affinity antibodies are preferred for improved sensitivity and specificity.
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.
Anti-idiotypic antibodies are a type of immune protein that recognizes and binds to the unique identifying region (idiotype) of another antibody. These antibodies are produced by the immune system as part of a regulatory feedback mechanism, where they can modulate or inhibit the activity of the original antibody. They have been studied for their potential use in immunotherapy and vaccine development.
A binding site on an antibody refers to the specific region on the surface of the antibody molecule that can recognize and bind to a specific antigen. Antibodies are proteins produced by the immune system in response to the presence of foreign substances called antigens. They have two main functions: to neutralize the harmful effects of antigens and to help eliminate them from the body.
The binding site of an antibody is located at the tips of its Y-shaped structure, formed by the variable regions of the heavy and light chains of the antibody molecule. These regions contain unique amino acid sequences that determine the specificity of the antibody for a particular antigen. The binding site can recognize and bind to a specific epitope or region on the antigen, forming an antigen-antibody complex.
The binding between the antibody and antigen is highly specific and depends on non-covalent interactions such as hydrogen bonds, van der Waals forces, and electrostatic attractions. This interaction plays a crucial role in the immune response, as it allows the immune system to recognize and eliminate pathogens and other foreign substances from the body.
HIV antibodies are proteins produced by the immune system in response to the presence of HIV (Human Immunodeficiency Virus) in the body. These antibodies are designed to recognize and bind to specific parts of the virus, known as antigens, in order to neutralize or eliminate it.
There are several types of HIV antibodies that can be produced, including:
1. Anti-HIV-1 and anti-HIV-2 antibodies: These are antibodies that specifically target the HIV-1 and HIV-2 viruses, respectively.
2. Antibodies to HIV envelope proteins: These antibodies recognize and bind to the outer envelope of the virus, which is covered in glycoprotein spikes that allow the virus to attach to and enter host cells.
3. Antibodies to HIV core proteins: These antibodies recognize and bind to the interior of the viral particle, where the genetic material of the virus is housed.
The presence of HIV antibodies in the blood can be detected through a variety of tests, including enzyme-linked immunosorbent assay (ELISA) and Western blot. A positive test result for HIV antibodies indicates that an individual has been infected with the virus, although it may take several weeks or months after infection for the antibodies to become detectable.
Heterophile antibody
Heterophile antibody test
Thyroid-stimulating hormone
Heterophile antigen
Infectious mononucleosis
Cross-reactivity
John Forssman
Pregnancy test
List of MeSH codes (D12.776.124)
List of MeSH codes (D12.776)
Index of immunology articles
Heterophile antibody - Wikipedia
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Graft rejection. Medical search
Antigen11
- Heterophile antigen An immunoassay is a biochemical test, frequently used in medical diagnostic testing, that measures the presence or concentration of a macromolecule in a solution through the use of an antibody or immunoglobulin. (wikipedia.org)
- Here's the basic structure of an antibody (Ab), which is defined as a blood protein produced in response to and counteracting a specific antigen. (aacc.org)
- As you can probably tell from the figure, each antibody has 2 antigen binding sites, which allows the antibody to bind to specific antigens in a lock-and-key-like mechanism. (aacc.org)
- In many cases, heterophile antibodies can arise naturally in the body as the result of antigen diversity. (aacc.org)
- Interpretation of EBV serology for human body material donors : is there a need for early antigen IgG and heterophile antibodies testing? (ugent.be)
- E) Combined HIV-1 antibody and antigen ELISA test. (mhmedical.com)
- Current HIV diagnostic ELISA methods include the option for both antibody and antigen detection. (mhmedical.com)
- or actively by prior immunization of the recipient with graft antigens which evoke specific antibodies and form antigen-antibody complexes which bind to the antigen receptor sites of the T-cells and block their cytotoxic activity. (lookformedical.com)
- The EBV VCA IgG Rapid Test Cassette (Whole Blood/Serum/Plasma) is a rapid chromatographic immunoassay for the qualitative detection of IgG antibody to Viral Capsid Antigen (VCA) of Epstein-Barr virus in human whole blood, serum, or plasma. (custom-monoclonalantibody.com)
- Both IgM and IgG antibodies to the viral capsid antigen (VCA) peak three to four weeks after primary EBV infection. (custom-monoclonalantibody.com)
- The presence or absence of EBV viral capsid antigen (VCA) IgG, VCA IgM and EBV nuclear antigen (EBNA) IgG antibodies was recorded. (who.int)
Antigens2
- Heterophile antibodies are antibodies induced by external antigens (heterophile antigens). (wikipedia.org)
- Antigens stimulating the formation of, or combining with heterophile antibodies. (nih.gov)
Detection10
- Other options include the use of heterophile blocking reagents, steps to remove immunoglobulins, serial dilutions and using non-mammalian capture and/or detection antibodies. (wikipedia.org)
- This is one strategy for heterophile antibody detection. (wikipedia.org)
- They can also bind to antibodies in the immunoassay, such as the capture or the signal antibodies, as well as other components of an immunoassay, such as the conjugate and other parts of a detection system. (aacc.org)
- There is a significant method-specific variation in the detection of dsDNA antibodies in patients receiving TNF antagonists, due in part to the effects of heterophile antibodies. (elsevierpure.com)
- In many people, detection of antibody to EA is a sign of active infection. (cdc.gov)
- B) HIV-1 antibody by rapid detection method. (mhmedical.com)
- Since the antibody to HIV will not develop for at least 2 to 8 weeks after infection and the retroviral syndrome typically occurs before seroconversion, HIV antibody tests, including rapid detection methods ("B"), may well be negative. (mhmedical.com)
- Patients receiving B-cell depleting therapy and those with prior SARS-CoV-2 infection (via detection of nucleocapsid antibodies) were excluded. (bvsalud.org)
- The Fortress Diagnostics Infectious Mononucleosis (IM) test is a rapid slide test for the qualitative detection of heterophile antibodies to IM in human serum. (fortressdiagnostics.com)
- The qualitative detection of heterophile antibodies was determined using the Clearview ® MONO test. (cit.ie)
Interference7
- Heterophile antibodies can cause significant interference in any immunoassay. (wikipedia.org)
- Heterophile antibody interference usually doesn't change linearly with serial dilution, but a true result most often will. (wikipedia.org)
- Blocking heterophile antibody interference can be achieved by removal of immunoglobulins from a sample (such as with PEG), by modifying antibodies which may be present in a sample or by using buffers to reduce interference. (wikipedia.org)
- Heterophile interference accounts for method-specific dsDNA antibodies in patients receiving anti-TNF treatment. (elsevierpure.com)
- Heterophile antibodies in plasma of certain individuals are known to cause interference with immunoassays. (cdc.gov)
- Preliminary data indicate little or no interference by heterophile antibodies. (vub.be)
- Laboratory studies ruled out heterophile antibody interference and hook effect by multiple methods including analysis by different serum hCG assays, treatment with heterophile antibody blocking agents, and dilution studies. (medscape.com)
Immunoassays7
- Sandwich immunoassay = two-site, noncompetitive immunoassays in which the analyte in the unknown sample is bound to the antibody site, then labeled antibody is bound to the analyte. (wikipedia.org)
- However, there are cases where heterophilic antibodies will give a linear response to dilutions, as well as immunoassays that do not change linearly upon dilution, meaning that the method is not fool-proof. (wikipedia.org)
- The Ghost in the assay tube: heterophil antibody interferences in immunoassays - an ever-recurring but often forgotten problem. (wikipedia.org)
- Then we'll quickly review immunoassay and look at some examples of how heterophile antibodies can interfere with immunoassays. (aacc.org)
- For the purpose of this presentation, we'll use "heterophile Ab" as an overarching term to describe Abs that can interfere with clinical immunoassays. (aacc.org)
- So how do these heterophile antibodies interfere with immunoassays? (aacc.org)
- But typically, when we talk about heterophile antibodies interfering with immunoassays, most people tend to think about nonspecific binding to capture and or signaling antibodies in an assay. (aacc.org)
Monospot test1
- You obtain a throat culture, CBC with differential, and heterophile antibody (Monospot) test. (mhmedical.com)
Diagnosis2
- In clinical diagnosis, the heterophile antibody test specifically refers to a rapid test for antibodies produced against the Epstein-Barr virus (EBV), the causative agent of infectious mononucleosis. (wikipedia.org)
- Tests for other EBV antibodies and/or a repeat mono test may be performed to help confirm or rule out the mononucleosis diagnosis. (labtestsonline.org.br)
Anti-VCA antibodies1
- The clinical findings of infectious mononucleosis occur in conjunction with the appearance of IgG and IgM anti-VCA antibodies. (cdc.gov)
Infection17
- EBV infection induces the production of several antibody classes, of which heterophile antibodies are one (others include anti-i, rheumatoid factor and ANA). (wikipedia.org)
- Thus, another possible cause of false positives in a pregnancy test are heterophile antibodies, commonly seen in EBV infection as well as selective IgA deficiency. (wikipedia.org)
- The present study showed that the presence in serum of the thermostable cytolytic anti-sheep red blood cells antibodies is dependent on the Schistosoma mansoni infection, and this is more frequent in adults than in children. (fiocruz.br)
- Antibody to EBNA, determined by the standard immunofluorescent test, is not seen in the acute phase of EBV infection but slowly appears two to four months after onset of symptoms and persists for the rest of a person's life. (cdc.gov)
- However, specific antibody tests may be needed to identify the cause of illness in people who do not have a typical case of infectious mononucleosis or have other illnesses that can be caused by EBV infection. (cdc.gov)
- People are considered susceptible to EBV infection if they do not have antibodies to the VCA. (cdc.gov)
- People are considered to have a primary EBV infection if they have anti-VCA IgM but do not have antibody to EBNA. (cdc.gov)
- Other results that strongly suggest a primary infection are a high or rising level of anti-VCA IgG and no antibody to EBNA after at least four weeks of illness. (cdc.gov)
- The presence of antibodies to both VCA and EBNA suggests past infection (from several months to years earlier). (cdc.gov)
- Since over 90% of adults have been infected with EBV, most adults will show antibodies to EBV from infection years earlier. (cdc.gov)
- High or elevated antibody levels may be present for years and are not diagnostic of recent infection. (cdc.gov)
- In most cases, the antibody response occurs rapidly during primary EBV infection. (cdc.gov)
- Although screening programs that rely on point-of-care HIV antibody testing will reliably identify persons with established infection, these tests fail to detect AHI ( 1 , 5 ). (cdc.gov)
- AHI was defined as having a negative or indeterminate HIV antibody test result in the presence of detectable HIV-1 RNA, corresponding to Fiebig stages I-II, with a mean estimated date of infection within the previous 10 days (95% CI 7-14 days) ( 12 ). (cdc.gov)
- Lower antibody levels before third vaccination correlated with lower antibodies after third immunization.ConclusionPatients with autoimmune rheumatic diseases undergoing combination therapy may be more vulnerable to SARS-CoV-2 infection, due to reduced antibody levels 6 months following two doses of mRNA vaccine. (bvsalud.org)
- The mono test detects heterophile antibodies , which are made by the body in response to an infection by EBV. (labtestsonline.org.br)
- If the mono test is initially negative but the doctor still suspects mono, he may order a repeat test in a week or so to see if Heterophile antibodies have developed and/or order one or more EBV antibodies to help confirm or rule out the presence of a current EBV infection. (labtestsonline.org.br)
Heterophilic antibodies2
- We found naturally heterophilic antibodies (IgG-type) in people without contact with Loxosceles spiders or any clinical history of loxoscelism. (biomedcentral.com)
- People without contact with the spider venom produced heterophilic antibodies capable of generating a cross-reaction against the venom of L. laeta and Sicarius spiders. (biomedcentral.com)
ELISA4
- Sixty serum samples from patients receiving biological anti-TNF medication were assessed for the presence of dsDNA antibodies using three standard diagnostic platforms [ELISA, IIF and multiplex bead array (MBA)], before and after treatment to block heterophile antibodies. (elsevierpure.com)
- dsDNA antibodies were frequent according to ELISA and IIF, but rare according to MBA. (elsevierpure.com)
- The effect of heterophile antibodies in the QuantiFERON ® -TB Gold IT ELISA is minimized by the addition of normal mouse serum to the green diluent and the use of F(ab')2 monoclonal antibody fragments as the IFN-γ capture antibody coated the microplate wells. (cdc.gov)
- A) HIV-1 antibody by ELISA followed by a Western blot. (mhmedical.com)
Monoclonal antibody1
- METHODS: As a model of this approach, we developed a dual-label time-resolved fluorescence immunoassay (TRFIA) to simultaneously measure proinsulin, C-peptide, and the proinsulin-C-peptide ratio (PI/C). A monoclonal antibody captures all C-peptide-containing molecules, and 2 differently labeled antibodies distinguish between proinsulin-like molecules and true C-peptide. (vub.be)
Serum2
- In 1932, Paul and Bunnell discovered that serum from symptomatic patients had antibodies that agglutinate the red blood cells (RBCs) of unrelated species, the "heterophile antibodies. (medscape.com)
- The reagent agglutinates when mixed with serum containing the heterophile antibodies. (fortressdiagnostics.com)
Cross-react1
- Moreover, heterophile antibodies cross-react with PLDs from other Loxosceles species and the venom of Sicarius spider. (biomedcentral.com)
Lymphocytes2
- Mono is also characterized by the presence of atypical white blood cells (usually reported as reactive lymphocytes ) as seen on a blood smear and by the presence of EBV antibodies in an infected person. (labtestsonline.org.br)
- If symptoms and reactive lymphocytes are present but the mono test is negative, then it may be too early to detect the Heterophile antibodies or the affected person may be one of a small percentage of people who do not make heterophile antibodies. (labtestsonline.org.br)
Titer2
- Of key interest is the effect of conventional synthetic (csDMARD) and biological/ targeted drugs (b/tsDMARDs) disease modifying antirheumatic drugs on the time of protection.ObjectivesTo compare antibody titer development in patients with vasculitis and connective tissue disease (CTD) with healthy controls 6 months after two mRNA vaccinations and after third immunization. (bvsalud.org)
- To analyze factors, that affect the velocity of titer decline, well as qualitative humoral response.MethodsPatients with SARD were enrolled and matched for gender and age with healthy control subjects (HC) and the humoral response after 6 months to two doses of mRNA vaccine BNT162b2 in terms of SARS-COV-2 antibody titer was assessed. (bvsalud.org)
Test11
- Heterophile antibody is a fairly specific but insensitive test for EBV. (wikipedia.org)
- This test looks for specific antibodies in the blood. (medlineplus.gov)
- EBV antibody test. (medlineplus.gov)
- This test looks for EBV antibodies, the main cause of mono. (medlineplus.gov)
- So monospot tests are often ordered with an EVB antibody test and other tests that look for infections. (medlineplus.gov)
- If it was negative, but you or your child still has symptoms, your health care provider will probably order an EBV antibody test. (medlineplus.gov)
- If your EBV test was positive, it means EBV antibodies were found in your blood. (medlineplus.gov)
- The test will also show which types of antibodies were found. (medlineplus.gov)
- Heterophite antibody test can be done. (epainassist.com)
- Hep C - The main test is Hep C Antibody. (diagnosis123.com)
- If Antibody negative, and Viral Load positive, they have Acute Hepatitis C. But the viral load test is expensive. (diagnosis123.com)
Immunoassay2
Infectious4
- Heterophile antibodies are of particular importance in clinical medicine for their use in detecting Epstein-Barr Virus (the causative agent of infectious mononucleosis). (wikipedia.org)
- The antibodies detected by Monospot can be caused by conditions other than infectious mononucleosis. (cdc.gov)
- For example, the heterophile antibodies detected by Monospot are often not present in children with infectious mononucleosis. (cdc.gov)
- EBV antibody tests are not usually needed to diagnose infectious mononucleosis. (cdc.gov)
HAMA3
- Human anti-mouse antibodies (HAMA) belong to this category. (wikipedia.org)
- The term "heterophile" antibodies is also often used to refer to human anti-animal antibodies, such as human-anti-mouse antibodies, or HAMA. (aacc.org)
- One important thing to note is that there are papers in the literature that draw a distinction between heterophile antibodies and human anti-animal antibodies such as HAMA, largely because of differences in their origin and binding affinity. (aacc.org)
Assay3
- The presence of a heterophile antibody is characterized by broad reactivity with antibodies of other animal species (which are often the source of the assay antibodies). (wikipedia.org)
- This type is also known as sandwich assay as the analyte is "sandwiched" between two antibodies. (wikipedia.org)
- Antibody in human sera that induces lysis of sheep erythrocytes in hemolytic assay was investigated. (fiocruz.br)
Diagnostic1
- Resolution of the illness may occur before the diagnostic antibody levels appear. (cdc.gov)
Autoimmune2
- Furthermore, the production of heterophile antibodies has been associated with patients with autoimmune or inflammatory conditions. (aacc.org)
- BackgroundPatients suffering from systemic autoimmune rheumatic disease (SARD) display poor antibody development after two doses of mRNA vaccinations leaving these patients with only limited humoral protection against severe SARS-CoV-2 disease courses. (bvsalud.org)
Infections3
- Heterophile antibodies can arise in non-EBV infections. (wikipedia.org)
- In rare cases, people with active EBV infections may not have detectable EBV-specific antibodies. (cdc.gov)
- These antibodies show up during or after during certain infections, including mono. (medlineplus.gov)
Rheumatic1
- For example, in rheumatic fever, antibodies against group A streptococcal cell walls can also react with (and thus damage) human heart tissues. (wikipedia.org)
Bind1
- It will be directly proportional to the concentration of the analyte because labeled antibody will not bind if the analyte is not present in the unknown sample. (wikipedia.org)
Affinity2
- Heterophile antibodies are IgM antibodies with affinity for sheep and horse red blood cells. (wikipedia.org)
- It's been estimated that up to 40% of the general population have antibodies with affinity to animal antibodies, but not all of them will be problematic for laboratory testing. (aacc.org)
Species1
- Antibodies from an individual that react with ISOANTIGENS of another individual of the same species. (lookformedical.com)
Specific3
- We identified significant method-specific discrepancies in the estimation of dsDNA antibodies in patients receiving TNF antagonists. (elsevierpure.com)
- The Nil samples adjust for background, heterophile antibody effects, or non-specific IFN-γ in blood samples. (cdc.gov)
- In addition, most testing programs in nonhealthcare settings continue to rely on routine antibody testing alone, with specific testing for AHI conducted only for persons with signs or symptoms. (cdc.gov)
Patients8
- Overall, it's been estimated that these endogenous heterophile antibodies can be found in more than 10% of patients. (aacc.org)
- To evaluate analytical explanations for the highly reported incidence of antibodies to dsDNA in patients receiving TNF antagonists. (elsevierpure.com)
- 0,001), whereas patients receiving only csDMARD as monotherapy displayed comparable antibody levels to healthy controls. (bvsalud.org)
- Our data strongly recommends antibody measurements in patients receiving combination therapy and individualized earlier booster vaccination.Figure 1.Anti-SARS-Cov-2 S antibody titers. (bvsalud.org)
- A: Antibody titers measured 6 months after two doses of mRNA vaccination in patients with connective tissue disease, vasculitis and healthy controls. (bvsalud.org)
- To the best of our knowledge, no study has evaluated the presence of antibodies against Loxosceles venom in loxoscelism patients without treatment with antivenom immunotherapy. (biomedcentral.com)
- We perform a comparative analysis for the presence of antibodies capable of recognizing Loxosceles venom in a group of patients diagnosed with loxoscelism and in a group of people without loxoscelism. (biomedcentral.com)
- In total, 420 patients had their peripheral bloods tested for heterophil antibodies over a two year period, 2018 and 2019 in the haematology department of the Mercy University Hospital (MUH), Cork. (cit.ie)
Clinical2
- An important clinical pearl for heterophile antibodies is they can also be seen in genetic immunodeficiencies. (wikipedia.org)
- The interpretation of EBV antibody tests requires familiarity with these tests and access to the patient's clinical information. (cdc.gov)
Sera1
- Thermostability of lytic heterophile antibodies from human sera infected with Schistosoma mansoni and geo-helminths. (fiocruz.br)
Mono2
- About 70% to 80% of those with mono produce heterophile antibodies. (labtestsonline.org.br)
- Most infants and young children will not make heterophile antibodies, so they will have negative mono tests even when infected with EBV. (labtestsonline.org.br)
Presence1
- Elevated levels of IFN-γ in the Nil sample may occur with the presence of heterophile antibodies, or to intrinsic IFN-γ secretion. (cdc.gov)
Occur1
- Symptoms occur sooner, and may get better before antibody shows up. (diagnosis123.com)
Rapidly1
- Anti-VCA IgM antibodies decline rapidly and are usually undetectable after 12 weeks. (custom-monoclonalantibody.com)
Symptoms1
- However, the antibody pattern is not stable before symptoms appear. (cdc.gov)
Typically1
- Heterophile antibody can also be found in healthy individuals, but typically to a lesser extent. (aacc.org)
Negative1
- As part of this confidential HIV testing program, routine, individual donation, HIV nucleic acid amplification testing (NAT) has been provided to all rapid antibody-negative participants since June 2007 (samples for NAT are obtained at the time of rapid antibody testing) ( 7 , 10 , 11 ). (cdc.gov)
Human1
- Such antibodies are commonly referred to as human anti-animal antibodies (HAAA). (wikipedia.org)
Children1
- Further, thermostable complement-activating heterophile antibodies were noticed in children in association with massive number of S.mansoni eggs. (fiocruz.br)
