POLYMERASE CHAIN-REACTION AMPLIFICATION OF A REPETITIVE DNA-SEQUENCE SPECIFIC FOR MYCOBACTERIUM-TUBERCULOSIS

被引:615
|
作者
EISENACH, KD
CAVE, MD
BATES, JH
CRAWFORD, JT
机构
[1] MCCLELLAN MEM VET HOSP,MED RES SERV 151,4300 W 7TH ST,LITTLE ROCK,AR 72205
[2] UNIV ARKANSAS MED SCI HOSP,DEPT PATHOL,LITTLE ROCK,AR 72205
[3] UNIV ARKANSAS MED SCI HOSP,DEPT ANAT,LITTLE ROCK,AR 72205
[4] UNIV ARKANSAS MED SCI HOSP,DEPT MED,LITTLE ROCK,AR 72205
[5] UNIV ARKANSAS MED SCI HOSP,DEPT MICROBIOL & IMMUNOL,LITTLE ROCK,AR 72205
来源
JOURNAL OF INFECTIOUS DISEASES | 1990年 / 161卷 / 05期
关键词
D O I
10.1093/infdis/161.5.977
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
A segment of DNA repeated in the chromosome of Mycobacterium tuberculosis was sequenced and used as a target for amplification using polymerase chain reaction (PCR). The sequences of the primers (5' to 3') were CCTGCGAGCGTAGGCGTCGG and CTCGTCCAGCGCCGCTTCGG, and a temperature of 68°C was used for annealing the primers in the reaction. Amplification produced a 123-base-pair fragment with an internal SalI site. The specific PCR product was obtained with input DNA from 11 different strains of M. tuberculosis and Mycobacterium bovis and one strain of Mycobacterium simiae. No product was detected with DNA from 28 strains of the Mycobacterium avium complex, Mycobacterium scrofulaceum, Mycobacterium kansasii, Mycobacterium jortuitum, Mycobacterium chelonei, and Mycobacterium gordonae. The PeR product was detected by gel electrophoresis after 30 cycles using 1 fg of input DNA. Amplification of this sequence may provide the basis for an assay to detect M. tuberculosis directly in clinical material. © 1990 by the University of Chicago. All rights reserved.
引用
收藏
页码:977 / 981
页数:5
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