POLYMERASE CHAIN-REACTION (PCR) AMPLIFICATION FOR THE DETECTION OF PORCINE PARVOVIRUS

被引：52

作者：

MOLITOR, TW ^{[1
]}

ORAVEERAKUL, K ^{[1
]}

ZHANG, QQ ^{[1
]}

CHOI, CS ^{[1
]}

LUDEMANN, LR ^{[1
]}

机构：

[1] USDA,APHIS,S&T,NATL VET SERV LABS,BIOL VIROL LAB,AMES,IA 50010

来源：

JOURNAL OF VIROLOGICAL METHODS | 1991年 / 32卷 / 2-3期

关键词：

PORCINE PARVOVIRUS; POLYMERASE CHAIN REACTION; DETECTION OF VIRAL DNA;

D O I：

10.1016/0166-0934(91)90051-Z

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

A polymerase chain reaction (PCR) amplification method was developed and evaluated to detect porcine parvovirus (PPV). A pair of 20-base primers and an oligonucleotide probe were derived from the DNA sequences common to two isolates of PPV, NADL-8 and NADL-2. The primers flanked 118-bp nucleotides within the region coding for the major structural protein VP2. After DNA amplification of PPV replicative form (RF), a 158-bp fragment was detected in agarose gels. This amplified fragment was shown to be specific for PPV DNA after Southern transfer and hybridization to a 20-base internal probe. The amplified fragment also contained a single EcoRI cleavage site. Various conditions, such as number of cycles and annealing temperature, were examined to optimize the conditions for detecting viral DNAs from infected cell cultures and swine fetal tissues. Four different isolates of PPV, NADL-8, NADL-2, KBSH and Kresse, and two other viruses, canine parvovirus (CPV) and pseudorabies virus (PRV), were included to determine specificity of amplification. Slot blot hybridization with a radiolabeled probe was used to evaluated the sensitivity of PCR amplification. The optimized protocol was specific for PPV detecting equally all four strains of PPV, but failing to amplify CPV or PRV sequences. The PCR method could detect at least 100 fg of viral replicative form (RF) DNA or the equivalent of 1 PFU of infectious virus. The applications of this method include routine detection of PPV in clinical samples and as a contaminant in mammalian cell lines.

引用

页码：201 / 211

页数：11

共 26 条

[1] POLYMERASE CHAIN-REACTION ASSAY OF PARVOVIRUS B19 DNA IN CLINICAL SPECIMENS
CLEWLEY, JP
[J]. JOURNAL OF CLINICAL MICROBIOLOGY, 1989, 27 (12) : 2647 - 2651
[2] THE AUTONOMOUSLY REPLICATING PARVOVIRUSES OF VERTEBRATES
COTMORE, SF
TATTERSALL, P
[J]. ADVANCES IN VIRUS RESEARCH, 1987, 33 : 91 - 174
[3] CSIZA CK, 1971, AM J VET RES, V32, P419
[4] DEA S, 1985, CAN J COMP MED, V49, P343
[5] PERSISTENCE OF PARVOVIRUS H-1 DNA IN HUMAN B-LYMPHOMA AND T-LYMPHOMA CELLS
FAISST, S
BARTNITZKE, S
SCHLEHOFER, JR
HAUSEN, HZ
[J]. VIRUS RESEARCH, 1990, 16 (02) : 211 - 224
[6] PERSISTENCE OF PORCINE PARVOVIRUS IN SWINE INFECTED INUTERO AND FOLLOWED THROUGH MATURITY
GRADIL, CM
JOO, HS
MOLITOR, TW
[J]. JOURNAL OF VETERINARY MEDICINE SERIES B-ZENTRALBLATT FUR VETERINARMEDIZIN REIHE B-INFECTIOUS DISEASES AND VETERINARY PUBLIC HEALTH, 1990, 37 (04): : 309 - 316
[7] PARVOVIRUSES AS CONTAMINANTS OF PERMANENT HUMAN CELL LINES .1. VIRUS ISOLATIONS FROM 1960-1970
HALLAUER, C
KRONAUER, G
SIEGL, G
[J]. ARCHIV FUR DIE GESAMTE VIRUSFORSCHUNG, 1971, 35 (01): : 80 - &
[8] PATHOGENESIS OF PORCINE PARVOVIRUS INFECTION - PATHOLOGY AND IMMUNOFLUORESCENCE IN FETUS
JOO, HS
DONALDSONWOOD, CR
JOHNSON, RH
CAMPBELL, RSF
[J]. JOURNAL OF COMPARATIVE PATHOLOGY, 1977, 87 (03) : 383 - 391
[9] RAPID DIAGNOSTIC TECHNIQUES FOR DETECTION OF PORCINE PARVOVIRUS INFECTION IN MUMMIFIED FETUSES
JOO, HS
DONALDSONWOOD, CR
JOHNSON, RH
[J]. AUSTRALIAN VETERINARY JOURNAL, 1976, 52 (01) : 51 - 52
[10] OBSERVATIONS ON PATHOGENESIS OF PORCINE PARVOVIRUS INFECTION
JOO, HS
DONALDSONWOOD, CR
JOHNSON, RH
[J]. ARCHIVES OF VIROLOGY, 1976, 51 (1-2) : 123 - 129

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