DETECTION OF HPV-16 IN CELL-LINES AND CERVICAL LAVAGE SPECIMENS BY A POLYMERASE CHAIN-REACTION ENZYME-IMMUNOASSAY ASSAY

被引:10
作者
COUTLEE, F
BOBO, L
ABBASS, H
DALABETTA, G
HOOK, NE
SHAH, K
VISCIDI, RP
机构
[1] UNIV MONTREAL, DEPT MICROBIOL & IMMUNOL, MONTREAL H3C 3J7, QUEBEC, CANADA
[2] JOHNS HOPKINS UNIV, SCH MED, DEPT MED, DIV INFECT DIS, BALTIMORE, MD 21205 USA
[3] JOHNS HOPKINS UNIV, SCH MED, DEPT PEDIAT, EUDOWOOD DIV INFECT DIS, BALTIMORE, MD 21205 USA
[4] JOHNS HOPKINS UNIV, SCH HYG & PUBL HLTH, DEPT IMMUNOL & INFECT DIS, BALTIMORE, MD 21218 USA
[5] BALTIMORE CITY DEPT HLTH, BALTIMORE, MD USA
关键词
PCR; HPV; GENITAL CANCER; BIOTIN; NONISOTOPIC;
D O I
10.1002/jmv.1890370105
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
A gene amplification method that combines the polymerase chain reaction with detection of amplified DNA in a solution hybridization/enzyme immunoassay (PCR-EIA) was developed for HPV-16 DNA. Samples were amplified with primers for the E7-E1 region of HPV-16. Amplified DNA products were identified and quantiated by hybridization in solution with a biotinylated RNA probe. Labeled DNA/RNA hybrids were measured semiquantitatively in an enzyme immunoassay using solid phase anti-biotin antibody and liquid phase B-d galactosidase labeled monoclonal antibody against DNA-RNA hybrids. Enzyme bound to the solid phase was quantitated with a fluorogenic substrate. The assay was linear over 2 log10 dilutions of SiHa cells and the detection limit was three copies of HPV-16 genome. The sensitivity of PCR-EIA for detection of PCR amplified products compared favorably with slot and Southern blots using a P-32-labeled RNA probe. The assay was used to assess HPV-16 infection of uterine cervix in women attending a clinic for sexually transmitted diseases. Twenty-one of the 81 specimens (25.9%), obtained by cervicovaginal lavage, were positive for HPV-16 by PCR-EIA. The assay provides a convenient means to objectively measure HPV DNA amplified with PCR.
引用
收藏
页码:22 / 29
页数:8
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