PCR for detection of rubella virus RNA in clinical samples

Author:

Bosma T J1,Corbett K M1,O'Shea S1,Banatvala J E1,Best J M1

Affiliation:

1. Department of Virology, United Medical School, Guys Hospital, London, United Kingdom.

Abstract

A reverse transcription nested PCR (RT-PCR) assay for the detection of rubella virus RNA using primers from the E1 open reading frame was established. This assay was found to be sensitive (detecting approximately two synthetic RNA copies and RNA extracted from 0.1 50% tissue culture infective dose of rubella virus) and specific; five wild-type rubella strains and four vaccine strains were detected, and no nonspecific amplification of 16 other RNA viruses or RNAs from seven cell types occurred. Rubella virus RNA was detected in 12 pharyngeal swabs from patients with serologically confirmed rubella; these RT-PCR results were in complete agreement with virus isolation. Analysis of products of conception obtained after confirmed primary maternal rubella infection by RT-PCR gave 92% agreement (12 of 13 samples) with virus isolation. No false-positive results were obtained. The potential use of this assay for prenatal diagnosis of congenital rubella infection and for investigating aspects of the pathogenesis of chronic disease is discussed.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

Reference27 articles.

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2. Best J. M. 1992. Rubella p. 171-184. In A. Greenough J. Osborne and S. Sutherland (ed.) Congenital perinatal and neonatal infections. Churchill Livingstone London.

3. Best J. M. and J. E. Banatvala. 1990. Rubella p. 337-374. In A. J. Zuckerman J. E. Banatvala and J. R. Pattison (ed.) Principles and practice of clinical virology 2nd ed. John Wiley and Sons Ltd. Chichester.

4. Best J. M. and S. O'Shea. 1989. Rubella virus p. 731-795. In N. J. Schmidt and R. W. Emmons (ed.) Diagnostic procedures for viral rickettsial and chlamydial infections 6th ed. American Public Health Association Washington D.C.

5. Rubella virus strains show no major antigenic differences;Best J. M.;Intervirology,1992

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