Pneumovirus
Pneumovirus Infections
Turkeys
Metapneumovirus
Paramyxoviridae Infections
Poultry Diseases
Paramyxoviridae
Respiratory Syncytial Viruses
Respiratory Syncytial Virus, Human
Detection and characterization of proteins encoded by the second ORF of the M2 gene of pneumoviruses. (1/39)
The nucleotide sequence of the M2 gene of pneumonia virus of mice (PVM) was determined. The sequence showed that the gene encoded a protein of 176 amino acids with a predicted molecular mass of 20165 Da from a major ORF, which is smaller than the equivalent proteins encoded by human, bovine and ovine respiratory syncytial (RS) viruses. The PVM M2 protein is conserved, having 41% similarity to the equivalent human RS virus protein. In common with the M2 genes of the RS viruses and avian pneumovirus (APV), the PVM mRNA also contained a second ORF (ORF2) that partially overlaps the first ORF and which is capable of encoding a 98 residue polypeptide. No significant sequence identity could be detected between the putative M2 ORF2 proteins of PVM, APV and the RS viruses. The expression of the M2 ORF2 proteins of the pneumoviruses was investigated by using monospecific antisera raised against GST fusion proteins. Western blot analysis demonstrated the presence of polypeptides encoded by M2 ORF2 of PVM and RS virus corresponding with those predicted by in vitro translation studies, but this was not the case for APV. The PVM polypeptide was present as three distinct products in vivo. The PVM and RS virus polypeptides were also detected in cells by immunofluorescence, which showed that both were present in the cytoplasm with a degree of localization in inclusion bodies. No APV M2 ORF2 protein could be detected in vivo. The RS virus M2 ORF2 polypeptide was shown to accumulate during infection and the potential implications of this are discussed. (+info)Isolation of avian pneumovirus from an outbreak of respiratory illness in Minnesota turkeys. (2/39)
Antibodies to avian pneumovirus (APV) were first detected in Minnesota turkeys in 1997. Virus isolation was attempted on 32 samples (28 tracheal swabs, 4 pools of trachea and turbinates) that were positive for APV by reverse transcriptase polymerase chain reaction (RT-PCR). The cell cultures used were chicken embryo fibroblast (CEF), Vero cells, and QT-35 cells. Five virus isolates were obtained from these samples, and the identity of the isolates was confirmed by RT-PCR. Four isolates were obtained by inoculation of CEF cells, and 1 isolate was obtained in QT-35 cells after 3-7 blind passages in cell cultures. Vero cells did not yield any isolate on primary isolation; however, all 5 isolates could be adapted to grow in Vero cells following primary isolation in CEF or QT-35 cells. This is the first report of isolation of APV in Minnesota and also the first report of primary isolation of APV in QT-35 cells. (+info)A modified enzyme-linked immunosorbent assay for the detection of avian pneumovirus antibodies. (3/39)
Avian pneumovirus (APV) infection of turkeys in Minnesota was first confirmed in March 1997. Serum samples (n = 5,194) from 539 submissions to Minnesota Veterinary Diagnostic Laboratory were tested by a modified enzyme-linked immunosorbent assay (ELISA). Of these, 2,528 (48.7%) samples from 269 submissions were positive and 2,666 (51.3%) samples from 270 submissions were negative for APV antibodies. Most positive samples were from Kandiyohi, Stearns, Morrison, and Meeker counties in Minnesota. In addition, 10 samples from South Dakota were positive. The sensitivity and specificity of the ELISA test with anti-chicken and anti-turkey conjugates were compared by testing field and experimental sera. The ELISA test with anti-turkey conjugate was more sensitive than that with anti-chicken conjugate. The ELISA tests with antigens prepared with APV strains isolated from Colorado and Minnesota were also compared. No difference was detectable. Currently, the Minnesota Veterinary Diagnostic Laboratory uses an antigen prepared from the Colorado isolate of APV and a goat anti-turkey conjugate in the ELISA test. (+info)The chemokine macrophage-inflammatory protein-1 alpha and its receptor CCR1 control pulmonary inflammation and antiviral host defense in paramyxovirus infection. (4/39)
In this work, we explore the responses of specific gene-deleted mice to infection with the paramyxovirus pneumonia virus of mice (PVM). We have shown previously that infection of wild type mice with PVM results in pulmonary neutrophilia and eosinophilia accompanied by local production of macrophage-inflammatory protein-1 alpha (MIP-1 alpha). Here we examine the role of MIP-1 alpha in the pathogenesis of this disease using mice deficient in MIP-1 alpha or its receptor, CCR1. The inflammatory response to PVM in MIP-1 alpha-deficient mice was minimal, with approximately 10-60 neutrophils/ml and no eosinophils detected in bronchoalveolar lavage fluid. Higher levels of infectious virus were recovered from lung tissue excised from MIP-1 alpha-deficient than from fully competent mice, suggesting that the inflammatory response limits the rate of virus replication in vivo. PVM infection of CCR1-deficient mice was also associated with attenuated inflammation, with enhanced recovery of infectious virus, and with accelerated mortality. These results suggest that the MIP-1 alpha/CCR1-mediated acute inflammatory response protects mice by delaying the lethal sequelae of infection. (+info)Nucleotide sequences of the F, L and G protein genes of two non-A/non-B avian pneumoviruses (APV) reveal a novel APV subgroup. (5/39)
Sequence analysis was performed of all or part of the genes encoding the fusion (F), polymerase (L) and attachment (G) proteins of two French non-A/non-B avian pneumovirus (APV) isolates (Fr/85/1 and Fr/85/2). The two isolates shared at least 99.7% nt and 99.0% aa sequence identity. Comparison with the F genes from subgroup A, subgroup B or Colorado APVs revealed nt and aa identities of 70.0-80. 5% and 77.6-97.2%, respectively, with the L gene sharing 76.1% nt and 85.3% aa identity with that of a subgroup A isolate. The Fr/85/1 and Fr/85/2 G genes comprised 1185 nt, encoding a protein of 389 aa. Common features with subgroup A and subgroup B G proteins included an amino-terminal membrane anchor, a high serine and threonine content, conservation of cysteine residues and a single extracellular region of highly conserved sequence proposed to be the functional domain involved in virus attachment to cellular receptors. However, the Fr/85/1 and Fr/85/2 G sequences shared at best 56.6% nt and 31.2% aa identity with subgroup A and B APVs, whereas these isolates share 38% aa identity. Phylogenetic analysis of the F, G and L genes of pneumoviruses suggested that isolates Fr/85/1 and Fr/85/2 belong to a previously unrecognized APV subgroup, tentatively named D. G-based oligonucleotide primers were defined for the specific molecular identification of subgroup D. These are the first G protein sequences of non-A/non-B APVs to be determined. (+info)Development of a highly sensitive and specific enzyme-linked immunosorbent assay based on recombinant matrix protein for detection of avian pneumovirus antibodies. (6/39)
The matrix (M) protein of avian pneumovirus (APV) was evaluated for its antigenicity and reliability in an enzyme-linked immunosorbent assay (ELISA) for diagnosis of APV infection, a newly emergent disease of turkeys in United States. Sera from APV-infected turkeys consistently contained antibodies to a 30-kDa protein (M protein). An ELISA based on recombinant M protein generated in Escherichia coli was compared with the routine APV ELISA that utilizes inactivated virus as antigen. Of 34 experimentally infected turkeys, 33 (97.1%) were positive by M protein ELISA whereas only 18 (52.9%) were positive by routine APV ELISA 28 days after infection. None of the serum samples from 41 uninfected experimental turkeys were positive by M protein ELISA. Of 184 field sera from turkey flocks suspected of having APV infection, 133 (72.3%) were positive by M protein ELISA whereas only 99 (53.8%) were positive by routine APV ELISA. Twelve serum samples, which were negative by M protein ELISA but positive by routine APV ELISA, were not reactive with either recombinant M protein or denatured purified APV proteins by Western analysis. This indicates that the samples had given false-positive results by routine APV ELISA. The M protein ELISA was over six times more sensitive than virus isolation (11.5%) in detecting infections from samples obtained from birds showing clinical signs of APV infection. Taken together, these results show that ELISA based on recombinant M protein is a highly sensitive and specific test for detecting antibodies to APV. (+info)Avian pneumovirus (APV) RNA from wild and sentinel birds in the United States has genetic homology with RNA from APV isolates from domestic turkeys. (7/39)
Nasal turbinates or swabs were collected from wild ducks, geese, owls, sparrows, swallows, and starlings and from sentinel ducks placed next to turkey farms experiencing avian pneumovirus (APV) infections and were analyzed for APV genome and infectious particles. APV RNA was detected in samples examined from geese, sparrows, and starlings. APV RNA and antibodies were also detected in two different groups of sentinel ducks. Infectious APV was recovered from sentinel duck samples. The APV M gene isolated from the wild birds had over 96% predicted amino acid identity with APV/Minnesota 2A, which was isolated earlier from domestic turkeys showing respiratory illness, suggesting that wild birds may be involved in spreading APV infection. (+info)Serological monitoring on layer farms with specific pathogen-free chickens. (8/39)
To monitor the existence of avian pathogens in laying chicken flocks, specific pathogen-free (SPF) chickens were introduced into two layer farms and reared with laying hens for 12 months. SPF chickens were bled several times after their introduction and examined for their sero-conversion to avian pathogens. As a result, antibodies to eight or ten kinds of pathogens were detected in SPF chickens on each farm. Antibodies to infectious bronchitis virus (IBV), avian nephritis virus, Mycoplasma gallisepticum and M. synoviae were detected early within the first month. Antibody titer to IBV suggested that the laying chickens were infected with IBV repeatedly during the experiment on both farms. However, antibodies to infectious bursal disease virus and 6 pathogens were not detected. (+info)Pneumovirus is a genus of viruses in the family Pneumoviridae, order Mononegavirales. It includes several species that can cause respiratory infections in humans and animals. The most well-known species that infect humans is Human Respiratory Syncytial Virus (HRSV), which is a major cause of bronchiolitis and pneumonia in young children, the elderly, and immunocompromised individuals. Other human pneumoviruses include Human Metapneumovirus (HMPV) and Avian Metapneumovirus subtype C (AMPV-C). These viruses can cause similar respiratory symptoms, ranging from mild to severe.
Pneumoviruses are enveloped, negative-sense, single-stranded RNA viruses that replicate in the cytoplasm of infected cells. They have a nonsegmented genome and encode several structural proteins, including an attachment protein, fusion protein, matrix protein, and nucleocapsid protein. The virions are typically pleomorphic, with a diameter of 150-250 nm.
Transmission of pneumoviruses occurs through respiratory droplets or direct contact with contaminated surfaces. Preventive measures include good hygiene practices, such as hand washing and covering the mouth and nose when coughing or sneezing. There are currently no vaccines available for human pneumoviruses, but several candidates are in development. Treatment is primarily supportive and may include oxygen therapy, mechanical ventilation, and antiviral medications in severe cases.
Pneumovirus infections refer to respiratory illnesses caused by viruses belonging to the Pneumoviridae family, specifically human respirovirus (hRSV) and human metapneumovirus (hMPV). These viruses primarily infect the respiratory tract and can cause a wide range of symptoms, from mild upper respiratory tract infections to severe lower respiratory tract illnesses such as bronchiolitis and pneumonia.
Human respirovirus (hRSV) is a leading cause of bronchiolitis and pneumonia in infants and young children, while human metapneumovirus (hMPV) tends to infect older children and adults, causing similar respiratory symptoms. Both viruses can also cause more severe disease in immunocompromised individuals, the elderly, and those with underlying medical conditions.
Transmission of these viruses typically occurs through close contact with infected individuals or contaminated surfaces, and they are highly contagious. Preventive measures include good hygiene practices, such as frequent handwashing and avoiding close contact with sick individuals. Currently, there are no vaccines available to prevent pneumovirus infections, but antiviral treatments and supportive care can help manage the symptoms and reduce the risk of complications.
Murine pneumonia virus (MPV) is not a widely recognized or officially established medical term. However, it may refer to the Pneumonia Virus of Mice (PVM), which is a pathogen that affects mice and can cause interstitial pneumonia.
PVM is an enveloped, single-stranded, negative-sense RNA virus belonging to the family Paramyxoviridae and the genus Pneumovirus. It primarily infects laboratory mice but has also been found in wild mouse populations. The virus replicates in the respiratory epithelium, leading to interstitial pneumonia and inflammation of the airways.
It is essential to note that Murine Pneumonia Virus should not be confused with Hantavirus Pulmonary Syndrome (HPS), which is also known as "mouse-related pulmonary syndrome." HPS is a severe, sometimes fatal, respiratory disease in humans caused by exposure to hantaviruses, which are found in rodents.
I'm not aware of any recognized medical term or condition specifically referred to as "turkeys." The term "turkey" is most commonly used in a non-medical context to refer to the large, bird-like domesticated fowl native to North America, scientifically known as Meleagris gallopavo.
However, if you are referring to a medical condition called "turkey neck," it is a colloquial term used to describe sagging or loose skin around the neck area, which can resemble a turkey's wattle. This condition is not a formal medical diagnosis but rather a descriptive term for an aesthetic concern some people may have about their appearance.
If you meant something else by "turkeys," please provide more context so I can give you a more accurate answer.
Metapneumovirus is a type of virus that can cause respiratory infections in humans and animals. The human metapneumovirus (HMPV) is a leading cause of acute respiratory infection (ARI), particularly in young children, the elderly, and people with weakened immune systems. It is associated with a wide range of clinical manifestations, ranging from mild upper respiratory symptoms to severe bronchiolitis and pneumonia.
HMPV is an enveloped, single-stranded RNA virus that belongs to the Pneumoviridae family, subfamily Pneumovirinae, and genus Metapneumovirus. It was first identified in 2001, although it is believed to have been circulating in humans for at least 50 years before its discovery. HMPV is transmitted through respiratory droplets and direct contact with infected individuals or contaminated surfaces.
The incubation period of HMPV ranges from 3 to 6 days, after which symptoms such as cough, fever, nasal congestion, sore throat, and difficulty breathing may appear. In severe cases, HMPV can lead to bronchitis, bronchiolitis, or pneumonia, requiring hospitalization, especially in high-risk populations. Currently, there is no specific antiviral treatment for HMPV infections, and management typically involves supportive care, such as oxygen therapy, hydration, and respiratory support if necessary. Prevention measures include good hand hygiene, wearing masks, and avoiding close contact with infected individuals.
Paramyxoviridae is a family of viruses that includes several important pathogens causing respiratory infections in humans and animals. According to the medical perspective, Paramyxoviridae infections refer to the diseases caused by these viruses.
Some notable human paramyxovirus infections include:
1. Respiratory Syncytial Virus (RSV) Infection: RSV is a common cause of respiratory tract infections, particularly in young children and older adults. It can lead to bronchiolitis and pneumonia, especially in infants and patients with compromised immune systems.
2. Measles (Rubeola): Measles is a highly contagious viral disease characterized by fever, cough, coryza (runny nose), conjunctivitis, and a maculopapular rash. It can lead to severe complications such as pneumonia, encephalitis, and even death, particularly in malnourished children and individuals with weakened immune systems.
3. Parainfluenza Virus Infection: Parainfluenza viruses are responsible for upper and lower respiratory tract infections, including croup, bronchitis, and pneumonia. They mainly affect young children but can also infect adults, causing mild to severe illnesses.
4. Mumps: Mumps is a contagious viral infection that primarily affects the salivary glands, causing painful swelling. It can lead to complications such as meningitis, encephalitis, deafness, and orchitis (inflammation of the testicles) in rare cases.
5. Human Metapneumovirus (HMPV) Infection: HMPV is a respiratory virus that can cause upper and lower respiratory tract infections, similar to RSV and parainfluenza viruses. It mainly affects young children and older adults, leading to bronchitis, pneumonia, and exacerbations of chronic lung diseases.
Prevention strategies for Paramyxoviridae infections include vaccination programs, practicing good personal hygiene, and implementing infection control measures in healthcare settings.
Poultry diseases refer to a wide range of infectious and non-infectious disorders that affect domesticated birds, particularly those raised for meat, egg, or feather production. These diseases can be caused by various factors including viruses, bacteria, fungi, parasites, genetic predisposition, environmental conditions, and management practices.
Infectious poultry diseases are often highly contagious and can lead to significant economic losses in the poultry industry due to decreased production, increased mortality, and reduced quality of products. Some examples of infectious poultry diseases include avian influenza, Newcastle disease, salmonellosis, colibacillosis, mycoplasmosis, aspergillosis, and coccidiosis.
Non-infectious poultry diseases can be caused by factors such as poor nutrition, environmental stressors, and management issues. Examples of non-infectious poultry diseases include ascites, fatty liver syndrome, sudden death syndrome, and various nutritional deficiencies.
Prevention and control of poultry diseases typically involve a combination of biosecurity measures, vaccination programs, proper nutrition, good management practices, and monitoring for early detection and intervention. Rapid and accurate diagnosis of poultry diseases is crucial to implementing effective treatment and prevention strategies, and can help minimize the impact of disease outbreaks on both individual flocks and the broader poultry industry.
Paramyxoviridae is a family of negative-sense, single-stranded RNA viruses that include several medically important pathogens. These viruses are characterized by their enveloped particles and helical symmetry. The paramyxoviruses can cause respiratory infections, neurological disorders, and other systemic diseases in humans, animals, and birds.
Some notable members of the Paramyxoviridae family include:
* Human respirovirus (also known as human parainfluenza virus): causes upper and lower respiratory tract infections in children and adults.
* Human orthopneumovirus (also known as respiratory syncytial virus, or RSV): a major cause of bronchiolitis and pneumonia in infants and young children.
* Measles morbillivirus: causes measles, a highly contagious viral disease characterized by fever, rash, and cough.
* Mumps virus: causes mumps, an acute infectious disease that primarily affects the salivary glands.
* Hendra virus and Nipah virus: zoonotic paramyxoviruses that can cause severe respiratory and neurological disease in humans and animals.
Effective vaccines are available for some paramyxoviruses, such as measles and mumps, but there are currently no approved vaccines for others, such as RSV and Nipah virus. Antiviral therapies are also limited, with only a few options available for the treatment of severe paramyxovirus infections.
Respiratory Syncytial Viruses (RSV) are a common type of virus that cause respiratory infections, particularly in young children and older adults. They are responsible for inflammation and narrowing of the small airways in the lungs, leading to breathing difficulties and other symptoms associated with bronchiolitis and pneumonia.
The term "syncytial" refers to the ability of these viruses to cause infected cells to merge and form large multinucleated cells called syncytia, which is a characteristic feature of RSV infections. The virus spreads through respiratory droplets when an infected person coughs or sneezes, and it can also survive on surfaces for several hours, making transmission easy.
RSV infections are most common during the winter months and can cause mild to severe symptoms depending on factors such as age, overall health, and underlying medical conditions. While RSV is typically associated with respiratory illnesses in children, it can also cause significant disease in older adults and immunocompromised individuals. Currently, there is no vaccine available for RSV, but antiviral medications and supportive care are used to manage severe infections.
Respiratory Syncytial Virus (RSV) is a highly contagious virus that causes infections in the respiratory system. In humans, it primarily affects the nose, throat, lungs, and bronchioles (the airways leading to the lungs). It is a major cause of lower respiratory tract infections and bronchiolitis (inflammation of the small airways in the lung) in young children, but can also infect older children and adults.
Human Respiratory Syncytial Virus (hRSV) belongs to the family Pneumoviridae and is an enveloped, single-stranded, negative-sense RNA virus. The viral envelope contains two glycoproteins: the G protein, which facilitates attachment to host cells, and the F protein, which mediates fusion of the viral and host cell membranes.
Infection with hRSV typically occurs through direct contact with respiratory droplets from an infected person or contaminated surfaces. The incubation period ranges from 2 to 8 days, after which symptoms such as runny nose, cough, sneezing, fever, and wheezing may appear. In severe cases, particularly in infants, young children, older adults, and individuals with weakened immune systems, hRSV can cause pneumonia or bronchiolitis, leading to hospitalization and, in rare cases, death.
Currently, there is no approved vaccine for hRSV; however, passive immunization with palivizumab, a monoclonal antibody, is available for high-risk infants to prevent severe lower respiratory tract disease caused by hRSV. Supportive care and prevention of complications are the mainstays of treatment for hRSV infections.
Respiratory Syncytial Virus (RSV), bovine refers to a species-specific strain of the Respiratory Syncytial Virus that primarily infects cattle. It is a member of the Pneumoviridae family and Orthopneumovirus genus. This virus is closely related to human RSV, and it can cause respiratory infections in young calves, leading to symptoms such as nasal discharge, coughing, difficulty breathing, and pneumonia.
Bovine RSV shares many similarities with its human counterpart, including the ability to form syncytia (multinucleated giant cells) in infected tissues. However, bovine RSV is not known to infect humans or cause disease in humans. It is primarily studied as a model organism for understanding the biology and pathogenesis of RSV infections in general.