Indigenous anti-hepatitis A virus IgM capture ELISA for the diagnosis of hepatitis A.

Chitambar, S D; Murthy-Grewal, S; Bokil, M; Arankalle, V A; Gore, M M; Banerjee, K

Indigenous anti-hepatitis A virus IgM capture ELISA for the diagnosis of hepatitis A.

Date

1994-06-01

Authors

Abstract

Anti-hepatitis A virus IgM capture ELISA was developed by using the reagents produced in the NIV laboratory. The major reagents of the assay were anti-human IgM antibody, hepatitis A virus (HAV) and anti-HAV IgG-horse radish peroxidase (HRP) conjugate. Of these, anti-human IgM antibodies were generated in rabbit against IgM secreted by human hybridoma clone(G3). HAV was derived from buffalo green money kidney cell line infected with HM-175 strain. Virus purified from the cell lysates was used for immunization of rabbits and guinea-pigs. There was very low anti-HAV response. A seropositive rhesus monkey was inoculated with monkey adapted strain of HAV to boost the anti-HAV antibody titre. Anti-HAV IgGs derived from hyperimmune sera of monkey and hepatitis A patient were conjugated with HRP. The preparations of conjugate--particularly human antibody--HRP conjugate yielded highly satisfactory results in anti-HAV capture ELISA. The assay appears to be specific, sensitive and quick and is useful in differentiating acute HAV infection from other acute infections caused by B, E and non-A non-B hepatitis viruses.

Citation

Chitambar SD, Murthy-Grewal S, Bokil M, Arankalle VA, Gore MM, Banerjee K. Indigenous anti-hepatitis A virus IgM capture ELISA for the diagnosis of hepatitis A. Indian Journal of Medical Research. 1994 Jun; 99(): 243-51