DETECTION OF GROUP-B AND GROUP-C ROTAVIRUSES BY POLYMERASE CHAIN-REACTION

被引：151

作者：

GOUVEA, V

ALLEN, JR

GLASS, RI

FANG, ZY

BREMONT, M

COHEN, J

MCCRAE, MA

SAIF, LJ

SINARACHATANANT, P

CAUL, EO

机构：

[1] US FDA,WASHINGTON,DC 20204

[2] CHINESE ACAD PREVENT MED,INST VIROL,BEIJING,PEOPLES R CHINA

[3] LAB VIROL & IMMUNOL MOLEC,F-78352 JOUY EN JOSAS,FRANCE

[4] UNIV WARWICK,DEPT BIOL SCI,COVENTRY CV4 7AL,W MIDLANDS,ENGLAND

[5] PUBL HLTH LAB,REG VIRUS LAB,BRISTOL BS2 8EL,ENGLAND

[6] OHIO STATE UNIV,OHIO AGR RES & DEV CTR,WOOSTER,OH 44691

[7] MAHIDOL UNIV,FAC SCI,DEPT MICROBIOL,BANGKOK 10700,THAILAND

来源：

JOURNAL OF CLINICAL MICROBIOLOGY | 1991年 / 29卷 / 03期

关键词：

D O I：

10.1128/JCM.29.3.519-523.1991

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

We adapted the polymerase chain reaction (PCR) to detect the noncultivatable group B and C rotaviruses and introduced a simple and convenient technique to purify viral RNA from stool specimens. Double-stranded RNA present in stool extracts was purified by adsorption to hydrodroxyapatite and was used as the template for reverse transcription and polymerase amplification. Primer pairs specific for group B (gene 8) and group C (gene 6) rotaviruses were selected to amplify group-characteristic sizes of cDNA copies readily identifiable in ethidium bromide-stained agarose gels. These primer pairs were used separately in individual PCR assays or were pooled with a primer pair specific for group A rotavirus (gene 9) in a combined PCR assay for the simultaneous detection of all three rotavirus groups. The method was very sensitive and was used to identify both human and porcine strains of group B and C rotaviruses in stool specimens. A second PCR amplification with internal group-specific primers served to increase further the sensitivity of the test and to confirm the diagnostic results obtained in the first amplification.

引用

页码：519 / 523

页数：5

共 26 条

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