A Serological Assay for the Detection of Antibodies Generated Against California Serogroup Virus Infection

The California serogroup (CSG) viruses are orthobunyaviruses endemic in North America and responsible for the second most common cause of mosquito-borne viral encephalitis in the United States. As the CSG viruses have been neglected and are poorly studied, there are no commercial diagnostic serologi...

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Vydané v:	Methods in molecular biology (Clifton, N.J.) Ročník 2893; s. 25
Hlavní autori:	Stulberg, Alyssa, Barry, Christina, Robinson, Alyssia, Mueller, Nicole, Bello, Alexander, Wood, Heidi
Médium:	Journal Article
Jazyk:	English
Vydavateľské údaje:	United States 2025
Predmet:	Animals Antibodies, Viral - blood Antibodies, Viral - immunology Antigens, Viral - immunology Encephalitis Virus, California - immunology Encephalitis, California - diagnosis Encephalitis, California - immunology Encephalitis, California - virology Enzyme-Linked Immunosorbent Assay - methods Humans Immunoglobulin M - blood Immunoglobulin M - immunology Neutralization Tests - methods Serogroup Serologic Tests - methods Virus antigen purification P/N ratio California serogroup virus MAC-ELISA
ISSN:	1940-6029, 1940-6029
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Abstract	The California serogroup (CSG) viruses are orthobunyaviruses endemic in North America and responsible for the second most common cause of mosquito-borne viral encephalitis in the United States. As the CSG viruses have been neglected and are poorly studied, there are no commercial diagnostic serological assays or reagents available for detection. Therefore, diagnostic laboratories have had to rely on the development of their own in-house serological assays. To develop serological assays, antigenic materials such as recombinant protein, virus-like particles (VLP), or inactivated virus can be used in the IgM antibody capture enzyme-linked immunosorbent assay (MAC-ELISA) to detect CSG virus-specific IgM antibodies. All positive MAC-ELISA results should be confirmed by a well-defined gold standard test method such as the plaque-reduction neutralization test (PRNT).
AbstractList	The California serogroup (CSG) viruses are orthobunyaviruses endemic in North America and responsible for the second most common cause of mosquito-borne viral encephalitis in the United States. As the CSG viruses have been neglected and are poorly studied, there are no commercial diagnostic serological assays or reagents available for detection. Therefore, diagnostic laboratories have had to rely on the development of their own in-house serological assays. To develop serological assays, antigenic materials such as recombinant protein, virus-like particles (VLP), or inactivated virus can be used in the IgM antibody capture enzyme-linked immunosorbent assay (MAC-ELISA) to detect CSG virus-specific IgM antibodies. All positive MAC-ELISA results should be confirmed by a well-defined gold standard test method such as the plaque-reduction neutralization test (PRNT).The California serogroup (CSG) viruses are orthobunyaviruses endemic in North America and responsible for the second most common cause of mosquito-borne viral encephalitis in the United States. As the CSG viruses have been neglected and are poorly studied, there are no commercial diagnostic serological assays or reagents available for detection. Therefore, diagnostic laboratories have had to rely on the development of their own in-house serological assays. To develop serological assays, antigenic materials such as recombinant protein, virus-like particles (VLP), or inactivated virus can be used in the IgM antibody capture enzyme-linked immunosorbent assay (MAC-ELISA) to detect CSG virus-specific IgM antibodies. All positive MAC-ELISA results should be confirmed by a well-defined gold standard test method such as the plaque-reduction neutralization test (PRNT). The California serogroup (CSG) viruses are orthobunyaviruses endemic in North America and responsible for the second most common cause of mosquito-borne viral encephalitis in the United States. As the CSG viruses have been neglected and are poorly studied, there are no commercial diagnostic serological assays or reagents available for detection. Therefore, diagnostic laboratories have had to rely on the development of their own in-house serological assays. To develop serological assays, antigenic materials such as recombinant protein, virus-like particles (VLP), or inactivated virus can be used in the IgM antibody capture enzyme-linked immunosorbent assay (MAC-ELISA) to detect CSG virus-specific IgM antibodies. All positive MAC-ELISA results should be confirmed by a well-defined gold standard test method such as the plaque-reduction neutralization test (PRNT).
Author	Barry, Christina Stulberg, Alyssa Robinson, Alyssia Wood, Heidi Bello, Alexander Mueller, Nicole
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SubjectTerms	Animals Antibodies, Viral - blood Antibodies, Viral - immunology Antigens, Viral - immunology Encephalitis Virus, California - immunology Encephalitis, California - diagnosis Encephalitis, California - immunology Encephalitis, California - virology Enzyme-Linked Immunosorbent Assay - methods Humans Immunoglobulin M - blood Immunoglobulin M - immunology Neutralization Tests - methods Serogroup Serologic Tests - methods
Title	A Serological Assay for the Detection of Antibodies Generated Against California Serogroup Virus Infection
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