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基于细菌人工染色体的突变分析对卡波氏肉瘤相关疱疹病毒小衣壳蛋白的功能特征进行研究。

Functional characterization of Kaposi's sarcoma-associated herpesvirus small capsid protein by bacterial artificial chromosome-based mutagenesis.

机构信息

Department of Microbiology, University of Pennsylvania School of Dental Medicine, 240 S. 40th Street, Philadelphia, PA 19104, USA.

出版信息

Virology. 2010 Nov 25;407(2):306-18. doi: 10.1016/j.virol.2010.08.017. Epub 2010 Sep 20.

Abstract

A systematic investigation of interactions amongst KSHV capsid proteins was undertaken in this study to comprehend lesser known KSHV capsid assembly mechanisms. Interestingly the interaction patterns of the KSHV small capsid protein, ORF65 suggested its plausible role in viral capsid assembly pathways. Towards further understanding this, ORF65-null recombinant mutants (BAC-∆65 and BAC-stop65) employing a bacterial artificial chromosome (BAC) system were generated. No significant difference was found in both overall viral gene expression and lytic DNA replication between stable monolayers of 293T-BAC36 (wild-type) and 293T-BAC-ORF65-null upon induction with 12-O-tetradecanoylphorbol-13-acetate, though the latter released 30-fold fewer virions to the medium than 293T-BAC36 cells. Sedimentation profiles of capsid proteins of ORF65-null recombinant mutants were non-reflective of their organization into the KSHV capsids and were also undetectable in cytoplasmic extracts compared to noticeable levels in nuclear extracts. These observations collectively suggested the pivotal role of ORF65 in the KSHV capsid assembly processes.

摘要

本研究系统地研究了 KSHV 衣壳蛋白之间的相互作用,以了解鲜为人知的 KSHV 衣壳组装机制。有趣的是,KSHV 小衣壳蛋白 ORF65 的相互作用模式表明其在病毒衣壳组装途径中可能发挥作用。为了进一步了解这一点,使用细菌人工染色体 (BAC) 系统生成了 ORF65 缺失重组突变体 (BAC-∆65 和 BAC-stop65)。在诱导物 12-O-十四烷酰佛波醇-13-乙酸酯的作用下,稳定单层的 293T-BAC36(野生型)和 293T-BAC-ORF65 缺失之间,总的病毒基因表达和裂解 DNA 复制没有明显差异,尽管后者释放到培养基中的病毒颗粒比 293T-BAC36 细胞少 30 倍。ORF65 缺失重组突变体的衣壳蛋白的沉淀谱不能反映它们在 KSHV 衣壳中的组织,与核提取物中明显的水平相比,在细胞质提取物中也无法检测到。这些观察结果共同表明 ORF65 在 KSHV 衣壳组装过程中起着关键作用。

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