Detection of mouse hepatitis virus by the polymerase chain reaction and its application to the rapid diagnosis of infection

Eight different strains of mouse hepatitis virus (MHV) were analyzed by the polymerase chain reaction (PCR) to see whether two sets of oligonucleotides, which were synthesized based on the published nucleotide sequence of MHV-JHM mRNAs 6 and 7, could be used as universal primers for amplification. T...

Full description

Saved in:
Bibliographic Details
Published inLaboratory animal science (Chicago) Vol. 43; no. 4; p. 285
Main Authors Yamada, Y K, Yabe, M, Yamada, A, Taguchi, F
Format Journal Article
LanguageEnglish
Published United States 01.08.1993
Subjects
Animals
Base Sequence
Coronavirus Infections - diagnosis
Coronavirus Infections - microbiology
Coronavirus Infections - veterinary
DNA Primers - genetics
DNA, Viral - genetics
Female
Mice
Mice, Inbred BALB C
Molecular Sequence Data
Murine hepatitis virus - genetics
Murine hepatitis virus - isolation & purification
Polymerase Chain Reaction - methods
Polymerase Chain Reaction - veterinary
RNA, Messenger - genetics
RNA, Viral - genetics
Rodent Diseases - diagnosis
Rodent Diseases - microbiology
Online AccessGet more information

Cover

More Information
Summary:Eight different strains of mouse hepatitis virus (MHV) were analyzed by the polymerase chain reaction (PCR) to see whether two sets of oligonucleotides, which were synthesized based on the published nucleotide sequence of MHV-JHM mRNAs 6 and 7, could be used as universal primers for amplification. Total RNA extracted from virus-infected cells or virus-infected culture fluids was transcribed into cDNA by using reverse transcriptase and oligo(dT) as primer, then the cDNA transcripts were amplified by PCR. The MHV-specific fragments of 199-bp and 241-bp were obtained from all eight strains irrespective of nucleotide differences in the primer regions. The same fragments were also amplified from RNA derived from the liver and brain of MHV-JHM-infected mice as soon as day 1 after intraperitoneal injection, even from the liver from which the virus was not detected. Results of PCR amplification from the liver RNA extracts became positive when more than 10(-2)PFU of MHV-JHM was contained in the PCR reaction mixture. In contrast, anti-MHV antibody was not detected by enzyme-linked immunosorbent assay until day 6 after inoculation. These results suggest that PCR is a very sensitive method to identify a variety of MHV infections in laboratory animals, especially at the early phase of infection.
ISSN:0023-6764