OVERPRODUCTION OF HUMAN-IMMUNODEFICIENCY-VIRUS TYPE-I REVERSE-TRANSCRIPTASE IN ESCHERICHIA-COLI AND PURIFICATION OF THE ENZYME

被引:29
作者
SAITOH, A
IWASAKI, H
NAKATA, A
ADACHI, A
SHINAGAWA, H
机构
[1] OSAKA UNIV,MICROBIAL DIS RES INST,DEPT EXPTL CHEMOTHERAPY,SUITA,OSAKA 565,JAPAN
[2] KYOTO UNIV,INST VIRUS RES,SAKYO KU,KYOTO 606,JAPAN
来源
MICROBIOLOGY AND IMMUNOLOGY | 1990年 / 34卷 / 06期
关键词
D O I
10.1111/j.1348-0421.1990.tb03168.x
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
Overexpression of the reverse transcriptase was designed in E. coli. For a high level of expression, HIV protein was expressed as a protein fusion with β-galactosidase. When the proviral DNA fragment covering the 3’ half of the gag gene and the entire pol gene was ligated to the 3’ end of the lacZ gene to fuse the truncated gag to lacZ in frame, a small quantity of reverse transcriptase was produced, indicating that frameshifting and post-translational processing have occurred. Much more reverse transcriptase was produced when the entire pol region was directly fused to the lacZ gene. From a one liter culture of bacteria, 1 mg of highly purified reverse transcriptase consisting of approximately equimolar amounts of two species (p64 and p51) was obtained. These proteins had identical N-termini consistent with the deduced amino acid sequence and therefore, might be correctly processed from the fusion protein in E. coli by the protease encoded by the pol region. The purified reverse transcriptase was enzymatically as active as the enzyme purified from the virus particles, and immunoreactive to the sera of HIV carriers with high sensitivity and specificity. © 1990, Center For Academic Publications Japan. All rights reserved.
引用
收藏
页码:509 / 521
页数:13
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