QUANTITATION OF ENTEROVIRAL RNA BY COMPETITIVE POLYMERASE CHAIN-REACTION

被引：29

作者：

MARTINO, TA

SOLE, MJ

PENN, LZ

LIEW, CC

LIU, P

机构：

[1] TORONTO HOSP,CTR CARDIOVASC RES,TORONTO M5G 2C4,ON,CANADA

[2] HOSP SICK CHILDREN,RES INST,DEPT MICROBIOL,TORONTO M5G 1X8,ONTARIO,CANADA

[3] UNIV TORONTO,DEPT MED,TORONTO M5S 1A1,ONTARIO,CANADA

[4] UNIV TORONTO,DEPT CLIN BIOCHEM,TORONTO M5S 1A1,ONTARIO,CANADA

[5] UNIV TORONTO,DEPT MICROBIOL,TORONTO M5S 1A1,ONTARIO,CANADA

来源：

JOURNAL OF CLINICAL MICROBIOLOGY | 1993年 / 31卷 / 10期

关键词：

D O I：

10.1128/JCM.31.10.2634-2640.1993

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

The polymerase chain reaction (PCR) is a new diagnostic technique for the detection of enteroviral infection; however, it currently provides only qualitative results. The aim of this study was to adapt PCR for the accurate quantitation of enteroviral RNA in clinical specimens. For this purpose, we designed a standard RNA which was homologous to sequences at the 5' end of the coxsackie B3 enterovirus genome but contained a single-base-pair mutation which created a novel internal restriction site. Serial dilutions of this standard template RNA were mixed with a fixed concentration of coxsackie B3 enterovirus RNA. The viral and standard templates were reverse transcribed to cDNA and coamplified by PCR, and a comparison of the radioactive PCR products was made. Since the templates were both present in a single reaction tube and competed for the same primers, the ratio of products remained proportional throughout the amplification process. By this approach, a fourfold difference in viral titer was clearly distinguishable. Moreover, we were able to accurately quantitate as few as 15 50% tissue culture infectious doses, which reflects common clinical viral titers. This study lays the foundation for quantitation of enteroviral RNA in clinical specimens and establishes a technique that can readily be applied to the diagnosis of enteroviral infection.

引用

页码：2634 / 2640

页数：7

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