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Rep 解旋酶的自动抑制亚基调控

Regulation of Rep helicase unwinding by an auto-inhibitory subdomain.

机构信息

Department of Molecular and Integrative Physiology, University of Illinois at Urbana-Champaign, Urbana, IL 61801, USA.

Department of Physics, Center for the Physics of Living Cells, University of Illinois at Urbana-Champaign, Urbana, IL 61801, USA.

出版信息

Nucleic Acids Res. 2019 Mar 18;47(5):2523-2532. doi: 10.1093/nar/gkz023.

Abstract

Helicases are biomolecular motors that unwind nucleic acids, and their regulation is essential for proper maintenance of genomic integrity. Escherichia coli Rep helicase, whose primary role is to help restart stalled replication, serves as a model for Superfamily I helicases. The activity of Rep-like helicases is regulated by two factors: their oligomeric state, and the conformation of the flexible subdomain 2B. However, the mechanism of control is not well understood. To understand the factors that regulate the active state of Rep, here we investigate the behavior of a 2B-deficient variant (RepΔ2B) in relation to wild-type Rep (wtRep). Using a single-molecule optical tweezers assay, we explore the effects of oligomeric state, DNA geometry, and duplex stability on wtRep and RepΔ2B unwinding activity. We find that monomeric RepΔ2B unwinds more processively and at a higher speed than the activated, dimeric form of wtRep. The unwinding processivity of RepΔ2B and wtRep is primarily limited by 'strand-switching'-during which the helicases alternate between strands of the duplex-which does not require the 2B subdomain, contrary to a previous proposal. We provide a quantitative model of the factors that enhance unwinding processivity. Our work sheds light on the mechanisms of regulation of unwinding by Rep-like helicases.

摘要

解旋酶是一种能够解开核酸的生物分子马达,其调控对于维持基因组完整性至关重要。大肠杆菌 Rep 解旋酶的主要作用是帮助停滞的复制重新启动,它是 Superfamily I 解旋酶的模型。Rep 样解旋酶的活性受到两个因素的调节:它们的寡聚状态和柔性亚基 2B 的构象。然而,其调控机制尚不清楚。为了了解调控 Rep 活性状态的因素,我们研究了缺乏亚基 2B 的变体(RepΔ2B)与野生型 Rep(wtRep)的行为关系。我们使用单分子光学镊子实验,探究了寡聚状态、DNA 几何形状和双链稳定性对 wtRep 和 RepΔ2B 解旋活性的影响。我们发现,单体 RepΔ2B 的解旋比激活的二聚体 wtRep 更具连续性和更快的速度。RepΔ2B 和 wtRep 的解旋连续性主要受到“链转换”的限制——在这个过程中,解旋酶在双链的链之间交替进行,这不需要 2B 亚基,这与之前的一个提议相反。我们提供了一个增强解旋连续性的因素的定量模型。我们的工作阐明了 Rep 样解旋酶的解旋调控机制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/abf2/6412110/f58268d50ffe/gkz023fig1.jpg

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