首页> 美国卫生研究院文献>Journal of Virology >Herpes simplex virus alpha protein ICP27 possesses separable positive and negative regulatory activities.
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Herpes simplex virus alpha protein ICP27 possesses separable positive and negative regulatory activities.

机译:单纯疱疹病毒α蛋白ICP27具有可分离的阳性和阴性调节活性。

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摘要

The HSV-1 alpha (immediate-early) protein ICP27 expressed in transfected cells can activate the expression of certain HSV-1 promoters as well as inhibit the transactivated expression of others. We constructed a set of plasmids encoding mutant ICP27 molecules truncated at their carboxyl termini and used transfection assays to determine the functional properties of the mutant proteins. A polypeptide containing the amino-terminal 263 amino acid residues of ICP27 retained partial ability to activate gene expression but was unable to inhibit transactivation. Mutant proteins possessing 406 or 504 amino acids of ICP27 were unable to activate gene expression but retained full ability to inhibit transactivation. These results define two separable regulatory activities of ICP27, one positive and one negative, which can modulate gene expression in transfected cells. Immunoblot and immunofluorescence experiments were used to study the immunological reactivities and intracellular localizations of the mutant proteins. All proteins possessing the amino-terminal 263 amino acids of ICP27 reacted with an ICP27-specific monoclonal antibody and were localized to the cell nucleus. The mutant proteins, however, exhibited a number of phenotypes with regard to intranuclear localization. A mutant possessing 504 residues of ICP27 was similar to the wild-type protein in apparently localizing to all regions of the nucleus. A mutant containing 406 residues of ICP27, on the other hand, was mostly excluded from the nucleolar regions, while a 263-residue mutant was localized predominantly in the nucleoli. Thus, some aspect of ICP27 structure or function can dramatically affect its intranuclear distribution.
机译:在转染的细胞中表达的HSV-1α(早期)蛋白ICP27可以激活某些HSV-1启动子的表达,并抑制其他HSV-1启动子的表达。我们构建了一套质粒,编码在其羧基末端被截断的突变ICP27分子,并使用转染测定来确定突变蛋白的功能特性。包含ICP27氨基末端263个氨基酸残基的多肽保留了部分激活基因表达的能力,但无法抑制反式激活。具有ICP27的406或504个氨基酸的突变蛋白无法激活基因表达,但保留了完全抑制反式激活的能力。这些结果定义了ICP27的两种可分离的调节活性,一种为阳性,一种为阴性,可以调节转染细胞中的基因表达。免疫印迹和免疫荧光实验用于研究突变蛋白的免疫反应性和细胞内定位。具有ICP27氨基末端263个氨基酸的所有蛋白质均与ICP27特异性单克隆抗体反应,并位于细胞核中。然而,突变蛋白在核内定位方面表现出许多表型。具有ICP27的504个残基的突变体与野生型蛋白相似,显然位于细胞核的所有区域。另一方面,含有ICP27的406个残基的突变体大部分被排除在核仁区域,而263个残基的突变体主要位于核仁中。因此,ICP27结构或功能的某些方面会极大地影响其核内分布。

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