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单纯疱疹病毒1型VP16的DNA结合衍生物(缺乏羧基末端酸性激活结构域)的转录激活作用。

Transcriptional activation by DNA-binding derivatives of HSV-1 VP16 that lack the carboxyl-terminal acidic activation domain.

作者信息

Popova B, Bilan P, Xiao P, Faught M, Capone J P

机构信息

Department of Biochemistry, McMaster University, Hamilton, Ontario, Canada.

出版信息

Virology. 1995 May 10;209(1):19-28. doi: 10.1006/viro.1995.1227.

Abstract

The herpes simplex virus transactivator VP16 directs the assembly of a multicomponent protein-DNA complex with cellular components Oct-1 and VCAF-1, contributing a potent carboxyl-terminal acidic activation domain that is essential for activation of gene expression in mammalian cells. We show here that VP16, devoid of this acidic activation domain, functions as a strong transcriptional activator in the yeast Saccharomyces cerevisiae when appended onto a heterologous GAL4 DNA binding domain, as determined by measuring activation of a resident GAL1:lacZ reporter gene. Deletion analysis indicated that sequences contained within the amino-terminal 369 amino acids of VP16 were necessary for transactivation by truncated VP16. Activation by truncated VP16 in yeast was comparable to that observed with a hybrid protein consisting of the GAL4 DNA binding domain linked to the VP16 acidic activation domain. Similar GAL4-VP16 hybrid proteins were only marginally active in mammalian cells. Sequence requirements for transactivation by truncated VP16 can be demarcated from domains of VP16 that are required for interaction with VCAF-1 and for protein-DNA complex formation with Oct-1. Our findings indicate that VP16 contains additional sequences upstream of the acidic activation domain that may play a direct role in transactivation.

摘要

单纯疱疹病毒反式激活因子VP16指导与细胞成分Oct-1和VCAF-1组装成多组分蛋白质-DNA复合物,其贡献了一个有效的羧基末端酸性激活结构域,这对于哺乳动物细胞中基因表达的激活至关重要。我们在此表明,当连接到异源GAL4 DNA结合结构域上时,缺乏该酸性激活结构域的VP16在酿酒酵母中作为一种强大的转录激活因子发挥作用,这是通过测量常驻GAL1:lacZ报告基因的激活来确定的。缺失分析表明,VP16氨基末端369个氨基酸内包含的序列对于截短的VP16的反式激活是必需的。截短的VP16在酵母中的激活与由连接到VP16酸性激活结构域的GAL4 DNA结合结构域组成的杂交蛋白所观察到的激活相当。类似的GAL4-VP16杂交蛋白在哺乳动物细胞中仅具有微弱的活性。截短的VP16反式激活的序列要求可以与VP16中与VCAF-1相互作用以及与Oct-1形成蛋白质-DNA复合物所需的结构域区分开来。我们的研究结果表明,VP16在酸性激活结构域上游包含额外的序列,这些序列可能在反式激活中起直接作用。

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