HIV-1反式激活因子蛋白可独立于病毒启动子序列和反式激活应答元件反式激活异源TATAA元件。

HIV-1 Tat protein can transactivate a heterologous TATAA element independent of viral promoter sequences and the trans-activation response element.

作者信息

Roebuck K A, Rabbi M F, Kagnoff M F

机构信息

Department of Immunology and Microbiology, Rush Presbyterian-St Luke's Medical Center, Chicago, Illinois 60612, USA.

出版信息

AIDS. 1997 Feb;11(2):139-46. doi: 10.1097/00002030-199702000-00002.

DOI:10.1097/00002030-199702000-00002

PMID:9030359

Abstract

OBJECTIVE

To determine whether the HIV-1 transactivator protein Tat acts as a DNA sequence-specific transcription factor and activates transcription from a heterologous TATAA element in the absence of the trans-activation response (TAR) element and other sequences in the HIV-1 long terminal repeat (LTR).

DESIGN

Activating protein-1 (AP-1) and Tat-induced transcription were assessed using Jun and hybrid Tat/Jun-expression plasmids and reporter gene constructs which contained AP-1 binding sites upstream of the rat prolactin TATAA element or an HIV-1 LTR construct in which AP-1 binding sites replaced the TAR element.

METHODS

Tat-induced transcription was determined following transient transfection of colon epithelial cell lines with reporter gene constructs and Tat/Jun-expression plasmids in which Tat was fused to the DNA binding domain of Jun. Activation of prolactin (PL) and LTR reporter genes was assessed by luciferase (LUC) or chloramphenicol acetyltransferase (CAT) activity in cellular extracts.

RESULTS

Cotransfection of cells with Tat/Jun and the AP-1 PL LUC or LTR AP-1 CAT reporter plasmid resulted in a marked increase in reporter gene activity which was comparable with that induced by transfection of cells with several different AP-1 expression plasmids (e.g., JunD, JunB, c-Fos), or that elicited by stimulation of the cells transfected with LTR AP-1 CAT plasmids with phorbol ester or tumor necrosis factor-alpha. Tat-induced transcription was DNA-mediated since both a Jun DNA binding domain fused to Tat as well as AP-1 binding sites within the promoter were required for the induction of CAT expression.

CONCLUSIONS

Tat-activated transcriptor can occur strictly through a heterologous TATAA element independent of TAR and Sp1 binding sites or other HIV-1 LTR sequences. Tat appears to increase transcription initiated through the TATAA element by mechanisms similar to that of DNA sequence-specific transcription factors.

摘要

目的

确定人类免疫缺陷病毒1型（HIV-1）反式激活蛋白Tat是否作为一种DNA序列特异性转录因子，在缺乏反式激活应答（TAR）元件及HIV-1长末端重复序列（LTR）中的其他序列的情况下，激活来自异源TATAA元件的转录。

设计

使用Jun和Tat/Jun杂交表达质粒以及报告基因构建体评估激活蛋白-1（AP-1）和Tat诱导的转录，这些构建体在大鼠催乳素TATAA元件上游含有AP-1结合位点，或者是一个AP-1结合位点取代了TAR元件的HIV-1 LTR构建体。

方法

用报告基因构建体和Tat/Jun表达质粒瞬时转染结肠上皮细胞系后，测定Tat诱导的转录，其中Tat与Jun的DNA结合结构域融合。通过细胞提取物中的荧光素酶（LUC）或氯霉素乙酰转移酶（CAT）活性评估催乳素（PL）和LTR报告基因的激活情况。

结果

将Tat/Jun与AP-1 PL LUC或LTR AP-1 CAT报告质粒共转染细胞，导致报告基因活性显著增加，这与用几种不同的AP-1表达质粒（如JunD、JunB、c-Fos）转染细胞所诱导的活性相当，或者与用佛波酯或肿瘤坏死因子-α刺激转染了LTR AP-1 CAT质粒的细胞所引发的活性相当。Tat诱导的转录是由DNA介导的，因为诱导CAT表达既需要与Tat融合的Jun DNA结合结构域，也需要启动子内的AP-1结合位点。