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对牛乳头瘤病毒1型E2反式激活因子功能至关重要的氨基酸。

Amino acids critical for the functions of the bovine papillomavirus type 1 E2 transactivator.

作者信息

Brokaw J L, Blanco M, McBride A A

机构信息

Laboratory of Viral Diseases, National Institutes of Allergy and Infectious Diseases, Bethesda, Maryland 20892-0455, USA.

出版信息

J Virol. 1996 Jan;70(1):23-9. doi: 10.1128/JVI.70.1.23-29.1996.

Abstract

The N-terminal domain of the bovine papillomavirus type 1 E2 protein is important for viral DNA replication, for transcriptional transactivation, and for interaction with the E1 protein. To determine which residues of this 200-amino-acid domain are important for these activities, single conservative amino acid substitutions have been generated in 17 residues that are invariant among all papillomavirus E2 proteins. The resulting mutated E2 proteins were tested for the ability to support viral DNA replication, activate transcription, and cooperatively bind to the origin of replication with the E1 protein. We identified five mutated proteins that were completely defective for transcriptional activation and either were defective or could support viral DNA replication at only low levels. However, several of these proteins could still interact efficiently with the E1 protein. In addition, we identified several mutated proteins that were unable to efficiently cooperatively bind to the origin with the E1 protein. Although a number of the mutated proteins demonstrated wild-type activity in all of the functions tested, only 3 out of 17 mutated viral genomes were able to induce foci in a C127 focus formation assay when the mutations were generated in the background of the entire bovine papillomavirus type 1 genome. This finding suggests that the E2 protein may have additional activities that are important for the viral life cycle.

摘要

牛乳头瘤病毒1型E2蛋白的N端结构域对于病毒DNA复制、转录反式激活以及与E1蛋白的相互作用都很重要。为了确定这个200个氨基酸的结构域中哪些残基对这些活性至关重要,我们在所有乳头瘤病毒E2蛋白中保守不变的17个残基上进行了单个保守氨基酸替换。对产生的突变E2蛋白进行了测试,以检测它们支持病毒DNA复制、激活转录以及与E1蛋白协同结合复制起点的能力。我们鉴定出5种突变蛋白,它们在转录激活方面完全缺陷,并且在病毒DNA复制方面要么有缺陷,要么只能在低水平上支持复制。然而,其中几种蛋白仍能与E1蛋白高效相互作用。此外,我们还鉴定出几种无法与E1蛋白高效协同结合复制起点的突变蛋白。尽管许多突变蛋白在所有测试功能中都表现出野生型活性,但当在整个牛乳头瘤病毒1型基因组背景下产生突变时,17个突变病毒基因组中只有3个能够在C127集落形成试验中诱导集落形成。这一发现表明,E2蛋白可能具有对病毒生命周期很重要的其他活性。

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