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The Hinge of the Human Papillomavirus Type 11 E2 Protein Contains Major Determinants for Nuclear Localization and Nuclear Matrix Association

机译:人乳头瘤病毒11型E2蛋白的铰链包含核定位和核基质关联的主要决定因素。

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摘要

The E2 protein of papillomaviruses is a site-specific DNA binding nuclear protein. It functions as the primary replication origin recognition protein and assists in the assembly of the preinitiation complex. It also helps regulate transcription from the native viral promoter. The E2 protein consists of an amino-terminal (N) trans-acting domain, a central hinge (H) domain, and a carboxyl-terminal (C) protein dimerization and DNA binding domain. The hinge is highly divergent among papillomaviruses, and little is known about its functions. We fused the enhanced green fluorescent protein (GFP) with the full-length human papillomavirus type 11 (HPV-11) E2 protein and showed that the resultant fusion, called gfpE2, maintained transcription and replication functions of the wild-type protein and formed similar subnuclear foci. Using a series of GFP fusion proteins, we showed that the hinge conferred strong nuclear localization, whereas the N or C domain was present in both cytoplasm and nucleus. Biochemical fractionation demonstrated that the N domain and hinge, but not the C domain, independently associated with the nuclear matrix. Mutational analyses showed that a cluster of basic amino acid residues, which is conserved among many mucosotropic papillomaviruses, was required for efficient nuclear localization and nuclear matrix association. This mutation no longer repressed the HPV-11 upstream regulatory region-controlled reporter expression. However, a very small fraction of this mutant colocalized with E1 in the nucleus, perhaps by a piggyback mechanism, and was able to support transient replication. We propose that the hinge is critical for the diverse regulatory functions of the HPV-11 E2 protein during mRNA transcription and viral DNA replication.
机译:乳头瘤病毒的E2蛋白是结合位点的DNA核蛋白。它起主要的复制起点识别蛋白的作用,并有助于预启动复合体的组装。它还有助于调节天然病毒启动子的转录。 E2蛋白由一个氨基末端(N)反式作用域,一个中央铰链(H)域和一个羧基末端(C)蛋白二聚化和DNA结合域组成。乳头瘤病毒之间的铰链高度不同,对其功能了解甚少。我们将增强的绿色荧光蛋白(GFP)与全长人乳头瘤病毒11型(HPV-11)E2蛋白融合,并显示所得的融合体gfpE2保持了野生型蛋白的转录和复制功能,并形成了相似的结构亚核灶。使用一系列的GFP融合蛋白,我们表明铰链赋予了强大的核定位,而在细胞质和细胞核中都存在N或C结构域。生化分级分离表明,N结构域和铰链而不是C结构域与核基质独立相关。突变分析表明,有效的核定位和核基质缔合需要许多嗜溶性乳头状瘤病毒之间保守的碱性氨基酸残基簇。该突变不再抑制HPV-11上游调节区控制的报告基因表达。但是,这种突变体的一小部分可能与E1共同位于细胞核中,可能是通过搭载机制实现的,并且能够支持瞬时复制。我们建议铰链对于在mRNA转录和病毒DNA复制过程中HPV-11 E2蛋白的多种调节功能至关重要。

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