Identification of group A rotavirus gene 4 types by polymerase chain reaction.

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J Clin Microbiol. 1992 June; 30(6): 1365-1373

Identification of group A rotavirus gene 4 types by polymerase chain reaction.

J R Gentsch, R I Glass, P Woods, V Gouvea, M Gorziglia, J Flores, B K Das and M K Bhan

Viral Gastroenteritis Unit, Centers for Disease Control, Atlanta, Georgia 30333.

ABSTRACT

Five genetically distinct human rotavirus (HRV) gene 4 groupshave been described on the basis of comparative nucleotide sequencingand the predicted amino acid sequences, and at least four ofthem represent distinct VP4 antigenic types. To identify eachgene 4 type and investigate its distribution in HRV isolatesfrom patients with diarrhea, we developed a polymerase chainreaction (PCR) typing method using sequence information availablefor four genetically distinct gene 4 types. Rotavirus double-strandedRNAs (dsRNAs) isolated from stool samples were first reversetranscribed and amplified by PCR by using two oligonucleotideprimers that correspond to regions that are highly conservedamong all known HRV gene 4 types. The 876-bp dsDNA productswere then reamplified by PCR in the presence of a cocktail containingone conserved plus-sense primer and four type-specific minus-senseprimers (selected from the hypervariable region of gene 4),resulting in products of 345, 483, 267, and 391 bp correspondingto gene 4 types 1, 2, 3, and 4, respectively. This method reliablyidentified the gene 4 types of 16 well-characterized HRV isolates.Our results were independently confirmed for all 16 strainsby reverse transcription and PCR amplification of HRV dsRNAin the presence of alternate type-specific primer pairs. Fordirect gene 4 typing of HRV in stool samples, we developed amethod to extract rotavirus dsRNA from stool specimens by usingglass powder. Our results suggest that gene 4 typing will beuseful in providing more a complete characterization of HRVstrains of epidemiologic or vaccine-related interest.

J Clin Microbiol. 1992 June; 30(6): 1365-1373

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