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利用氢交换和室温磷光对蛋白质球状核心进行长时间尺度探测。

Long time-scale probing of the protein globular core using hydrogen-exchange and room temperature phosphorescence.

作者信息

Schlyer B D, Steel D G, Gafni A

机构信息

Institute of Gerontology, University of Michigan, Ann Arbor 48109, USA.

出版信息

Biochem Biophys Res Commun. 1996 Jun 25;223(3):670-4. doi: 10.1006/bbrc.1996.0953.

Abstract

Preliminary room temperature phosphorescence measurements of the highly buried Trp109 in E. coli alkaline phosphatase have been used to report on the kinetics of protein hydrogen-deuterium exchange. Upon dilution in D2O the phosphorescence lifetime increases (at 20 degrees C) in a biphasic manner with an immediate change (< 30 seconds) followed by a slow change occurring on an extremely long timescale (days). The immediate D2O-induced lifetime increase is similar to that observed upon dilution into glycerol, a known protein hydrating agent. On the other hand, the slow D2O-induced first order growth in Trp109 lifetime is due to exchange at highly protected protein groups. As the phosphorescence lifetime of Trp109 is dependent on local rigidity, this increase in lifetime reflects changes in alkaline phosphatase structure. This first use of room temperature phosphorescence to monitor proton exchange shows promise as a sensitive and selective probe of protein core dynamics.

摘要

利用对大肠杆菌碱性磷酸酶中深度埋藏的色氨酸109进行的初步室温磷光测量来报告蛋白质氢-氘交换动力学。在重水中稀释时,磷光寿命(在20摄氏度下)以双相方式增加,先是立即变化(<30秒),随后是在极长的时间尺度(数天)上发生的缓慢变化。重水诱导的立即寿命增加类似于稀释到甘油(一种已知的蛋白质水合试剂)中时观察到的情况。另一方面,重水诱导的色氨酸109寿命的缓慢一级增长是由于高度受保护的蛋白质基团处的交换。由于色氨酸109的磷光寿命取决于局部刚性,寿命的这种增加反映了碱性磷酸酶结构的变化。这种首次使用室温磷光监测质子交换的方法有望成为一种灵敏且具有选择性的蛋白质核心动力学探针。

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