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氧传感器蛋白 HemAT-Bs 传感域到信号域通讯途径中特定部位的蛋白质动力学:时间分辨紫外共振拉曼研究。

Site-specific protein dynamics in communication pathway from sensor to signaling domain of oxygen sensor protein, HemAT-Bs: Time-resolved Ultraviolet Resonance Raman Study.

机构信息

Lehrstuhl für Biophysik, Ruhr-Universität Bochum, 44780 Bochum, Germany.

出版信息

J Biol Chem. 2012 Jun 8;287(24):19973-84. doi: 10.1074/jbc.M112.357855. Epub 2012 Apr 23.

DOI:10.1074/jbc.M112.357855
PMID:22528495
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3370181/
Abstract

HemAT-Bs is a heme-based signal transducer protein responsible for aerotaxis. Time-resolved ultraviolet resonance Raman (UVRR) studies of wild-type and Y70F mutant of the full-length HemAT-Bs and the truncated sensor domain were performed to determine the site-specific protein dynamics following carbon monoxide (CO) photodissociation. The UVRR spectra indicated two phases of intensity changes for Trp, Tyr, and Phe bands of both full-length and sensor domain proteins. The W16 and W3 Raman bands of Trp, the F8a band of Phe, and the Y8a band of Tyr increased in intensity at hundreds of nanoseconds after CO photodissociation, and this was followed by recovery in ∼50 μs. These changes were assigned to Trp-132 (G-helix), Tyr-70 (B-helix), and Phe-69 (B-helix) and/or Phe-137 (G-helix), suggesting that the change in the heme structure drives the displacement of B- and G-helices. The UVRR difference spectra of the sensor domain displayed a positive peak for amide I in hundreds of nanoseconds after photolysis, which was followed by recovery in ∼50 μs. This difference band was absent in the spectra of the full-length protein, suggesting that the isolated sensor domain undergoes conformational changes of the protein backbone upon CO photolysis and that the changes are restrained by the signaling domain. The time-resolved difference spectrum at 200 μs exhibited a pattern similar to that of the static (reduced - CO) difference spectrum, although the peak intensities were much weaker. Thus, the rearrangements of the protein moiety toward the equilibrium ligand-free structure occur in a time range of hundreds of microseconds.

摘要

HemAT-Bs 是一种基于血红素的信号转导蛋白,负责趋化作用。对全长 HemAT-Bs 和 Y70F 突变体以及截断的传感器结构域的野生型和 Y70F 突变体进行了时间分辨的紫外共振拉曼(UVRR)研究,以确定 CO 光解后特定于蛋白质的蛋白质动力学。UVRR 光谱表明,全长和传感器结构域蛋白的色氨酸、酪氨酸和苯丙氨酸带的强度变化有两个阶段。CO 光解数百纳秒后,色氨酸的 W16 和 W3 Raman 带、苯丙氨酸的 F8a 带和酪氨酸的 Y8a 带的强度增加,随后在 50μs 内恢复。这些变化被分配给色氨酸 132(G-螺旋)、酪氨酸 70(B-螺旋)和苯丙氨酸 69(B-螺旋)和/或苯丙氨酸 137(G-螺旋),表明血红素结构的变化驱动 B-和 G-螺旋的位移。传感器结构域的 UVRR 差谱在光解后数百纳秒显示酰胺 I 的正峰,随后在 50μs 内恢复。在全长蛋白的光谱中不存在该差异带,表明分离的传感器结构域在 CO 光解时经历蛋白质骨架的构象变化,并且变化受到信号结构域的限制。200μs 时的时间分辨差谱显示出与静态(还原-CO)差谱相似的模式,尽管峰强度弱得多。因此,蛋白质部分向平衡无配体结构的重排发生在数百微秒的时间范围内。

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本文引用的文献

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