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R52Q突变体的晶体结构表明R52在光活性黄色蛋白的发色团pKa调节中发挥作用。

The crystal structure of the R52Q mutant demonstrates a role for R52 in chromophore pKa regulation in photoactive yellow protein.

作者信息

Shimizu Nobutaka, Kamikubo Hironari, Yamazaki Yoichi, Imamoto Yasushi, Kataoka Mikio

机构信息

Structural Biology Group, Research and Utilization Division, Japan Synchrotron Radiation Research Institute, Hyogo, Japan.

出版信息

Biochemistry. 2006 Mar 21;45(11):3542-7. doi: 10.1021/bi051430a.

Abstract

Mutating arginine 52 to glutamine (R52Q) in photoactive yellow protein (PYP) increases the pK(a) of the chromophore by 1 pH unit. The structure of the R52Q PYP mutant was determined by X-ray crystallography and was compared to the structure of wild-type PYP to assess the role of R52 in pK(a) regulation. The essential differences between R52Q and the wild type were confined to the loop region containing the 52nd residue. While the hydrogen bonds involving the chromophore were unchanged by the mutation, removing the guanidino group generated a cavity near the chromophore; this cavity is occupied by two water molecules. In the wild type, R52 forms hydrogen bonds with T50 and Y98; these hydrogen bonds are lost in R52Q. Q52 is linked to Y98 by hydrogen bonding through the two water molecules. R52 acts as a lid on the chromophore binding pocket and controls the accessibility of the exterior solvent and the pK(a) of the chromophore. R52 is found to flip out during the formation of PYP(M). The result of this movement is quite similar to the altered structure of R52Q. Thus, we propose that conformational changes at R52 are partly responsible for pK(a) regulation during the photocycle.

摘要

将光活性黄色蛋白(PYP)中的精氨酸52突变为谷氨酰胺(R52Q)可使发色团的pK(a)增加1个pH单位。通过X射线晶体学确定了R52Q PYP突变体的结构,并将其与野生型PYP的结构进行比较,以评估R52在pK(a)调节中的作用。R52Q与野生型之间的本质差异局限于包含第52位残基的环区域。虽然涉及发色团的氢键未因突变而改变,但去除胍基在发色团附近产生了一个空腔;这个空腔被两个水分子占据。在野生型中,R52与T50和Y98形成氢键;这些氢键在R52Q中丢失。Q52通过两个水分子通过氢键与Y98相连。R52充当发色团结合口袋的盖子,控制外部溶剂的可及性和发色团的pK(a)。发现R52在PYP(M)形成过程中翻转出来。这种运动的结果与R52Q的结构改变非常相似。因此,我们提出R52处的构象变化部分负责光循环期间的pK(a)调节。

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