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泡沫病毒蛋白酶-逆转录酶酶活性的结构要求。

Structural requirements for enzymatic activities of foamy virus protease-reverse transcriptase.

机构信息

Universität Bayreuth, Lehrstuhl Biopolymere, Universitätsstr. 30, D-95447, Bayreuth, Germany.

出版信息

Proteins. 2014 Mar;82(3):375-85. doi: 10.1002/prot.24394. Epub 2013 Oct 17.

DOI:10.1002/prot.24394
PMID:23966123
Abstract

Reverse transcriptases (RTs) are pivotal in the life cycle of retroviruses and convert the genomic viral RNA into double-stranded DNA. The RT polymerase domain is subdivided into fingers, palm, thumb, and the connection subdomain, which links the polymerase to the C-terminal RNase H domain. In contrast to orthoretroviruses, mature RT of foamy viruses harbors the protease (PR) domain at its N-terminus (PR-RT). Therefore and due to low homology to other RTs, it is difficult to define the boundaries and functions of the (sub)domains. We introduced N- and C-terminal deletions into simian foamy virus PR-RT to investigate the impact of the truncations on the catalytic activities. Both, the RNase H domain and the connection subdomain contribute substantially to polymerase integrity and stability as well as to polymerase activity and substrate binding. The 42 amino acids long region C-terminal of the PR is important for polymerase stability and activity. PR activation via binding of PR-RT to viral RNA requires the presence of the full length PR-RT including the RNase H domain. In vitro, the cleavage efficiencies of FV PR for the Gag and Pol cleavage site are comparable, even though in virus particles only the Pol site is cleaved to completion suggesting that additional factors control PR activity and that virus maturation needs to be strictly regulated.

摘要

逆转录酶(RTs)在逆转录病毒的生命周期中起着关键作用,它将基因组病毒 RNA 转化为双链 DNA。RT 聚合酶结构域分为手指、手掌、拇指和连接亚结构域,连接亚结构域将聚合酶与 C 端的核糖核酸酶 H 结构域连接起来。与正逆转录病毒不同,成熟的泡沫病毒 RT 在其 N 端具有蛋白酶(PR)结构域(PR-RT)。因此,由于与其他 RT 的同源性低,很难定义(亚)结构域的边界和功能。我们在猴泡沫病毒 PR-RT 中引入 N 端和 C 端缺失,以研究这些截断对催化活性的影响。核糖核酸酶 H 结构域和连接亚结构域都对聚合酶完整性和稳定性以及聚合酶活性和底物结合有很大的贡献。PR 42 个氨基酸长的 C 端区域对聚合酶稳定性和活性很重要。PR-RT 与病毒 RNA 结合导致 PR 激活,这需要全长的 PR-RT,包括核糖核酸酶 H 结构域。在体外,FV PR 对 Gag 和 Pol 切割位点的切割效率相当,尽管在病毒颗粒中只有 Pol 位点被完全切割,这表明额外的因素控制 PR 活性,并且病毒成熟需要严格调控。

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