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酿酒酵母中Tat对HIV-1启动子高效反式激活的限制步骤鉴定。

Identification of limiting steps for efficient trans-activation of HIV-1 promoter by Tat in Saccharomyces cerevisiae.

作者信息

Daviet L, Bois F, Battisti P L, Gatignol A

机构信息

Unité 332, INSERM, Institut Cochin de Génétique Moléculaire, 22, rue Méchain, 75014 Paris, France.

出版信息

J Biol Chem. 1998 Oct 23;273(43):28219-28. doi: 10.1074/jbc.273.43.28219.

Abstract

Cellular context is an important determinant for the activity of Tat, the trans-activator of human immunodeficiency virus (HIV). We have investigated HIV-1 promoter expression and trans-activation in Saccharomyces cerevisiae to provide clues about the limiting steps for Tat activity in this organism. A minimal 43-nucleotide HIV promoter (HIV43) has the activity of a weak yeast promoter in the presence or absence of various enhancer binding sites (bs), whereas the entire long terminal repeat is not expressed. None of these constructs could be trans-activated by Tat. Fusion proteins Gal4 binding domain (BD)-Tat48 and Gal4BD-Tat72 are active with different efficiencies on various yeast promoters that have Gal4 bs. They have 70 and 50% of Gal4 wild type activity on hybrid HIV promoters fused to Gal4 bs only in the presence of AP1 bs. This study shows that trans-activation of the HIV-1 promoter by Tat occurs in yeast when Tat is targeted to the promoter and a functional enhancer activity is present. Sp1 function and Tat transfer from the RNA to the promoter are two major elements for in vivo trans-activation of HIV-1 that are defective in S. cerevisiae but can be replaced by functional equivalents.

摘要

细胞环境是人类免疫缺陷病毒(HIV)反式激活因子Tat活性的重要决定因素。我们研究了HIV-1启动子在酿酒酵母中的表达及反式激活作用,以探寻该生物体中Tat活性的限制步骤。一个最小的43个核苷酸的HIV启动子(HIV43),无论是否存在各种增强子结合位点(bs),都具有弱酵母启动子的活性,而整个长末端重复序列则不表达。这些构建体均不能被Tat反式激活。融合蛋白Gal4结合结构域(BD)-Tat48和Gal4BD-Tat72对具有Gal4 bs的各种酵母启动子具有不同效率的活性。仅在存在AP1 bs的情况下,它们在与Gal4 bs融合的杂交HIV启动子上具有Gal4野生型活性的70%和50%。这项研究表明,当Tat靶向启动子且存在功能性增强子活性时,Tat对HIV-1启动子的反式激活在酵母中发生。Sp1功能以及Tat从RNA转移到启动子是HIV-1体内反式激活的两个主要因素,它们在酿酒酵母中存在缺陷,但可以被功能等同物替代。

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