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质子进入细菌视紫红质质子传导通道胞质部分的机制。

Mechanism of proton entry into the cytoplasmic section of the proton-conducting channel of bacteriorhodopsin.

作者信息

Checover S, Nachliel E, Dencher N A, Gutman M

机构信息

Department of Biochemistry, Tel Aviv University, Israel.

出版信息

Biochemistry. 1997 Nov 11;36(45):13919-28. doi: 10.1021/bi9717542.

DOI:10.1021/bi9717542
PMID:9374871
Abstract

Bacteriorhodopsin is the light-driven proton-pumping protein of Halobacterium salinarum that extracts protons from the well-buffered cytoplasmic space within the time limits set by the photocycle turnover. The specific mechanism of the proton uptake by the cytoplasmic surface of the protein was investigated in this study by the laser-induced proton pulse technique. The purple membrane preparations were labeled by fluorescein at two residues (36 or 38) of the cytoplasmic surface of the protein, sites that are close to the orifice of the proton-conducting channel. The membranes were pulsed by protons discharged from photoexcited pyranine [Nachliel, E., Gutman, M., Kiryati, S., and Dencher, N.A. (1996) Proc. Nat Acad. Sci. U.S.A. 93, 10747-10752). The reaction of the discharged protons with the pyranine anion and the fluorescein was measured with sub-microsecond resolution. The experimental signals were reconstructed through numeric integration of differential rate equations which quantitated the rates of all proton transfer reactions between all reactants present in the system. The interaction of protons with the orifice of the cytoplasmic channel is enhanced by the exposed carboxylates of the protein. A cluster of three carboxylates acts as a strong proton attractor site while one carboxylate, identified as D36, acts as a mediator that delivers the proton to the channel. The combination of these reactions render the surface of the protein with properties of a proton-collecting antenna. The size of the collecting area is less than that of the protein's surface.

摘要

细菌视紫红质是盐生盐杆菌中受光驱动的质子泵蛋白,它在光循环周转设定的时间限制内从缓冲良好的细胞质空间中提取质子。本研究通过激光诱导质子脉冲技术研究了该蛋白质细胞质表面摄取质子的具体机制。紫色膜制剂在蛋白质细胞质表面的两个残基(36或38)处用荧光素标记,这两个位点靠近质子传导通道的孔口。用从光激发的吡喃荧光素释放的质子对膜进行脉冲处理[Nachliel, E., Gutman, M., Kiryati, S., and Dencher, N.A. (1996) Proc. Nat Acad. Sci. U.S.A. 93, 10747 - 10752]。以亚微秒分辨率测量释放的质子与吡喃荧光素阴离子和荧光素的反应。通过对微分速率方程进行数值积分来重建实验信号,这些方程量化了系统中所有反应物之间所有质子转移反应的速率。蛋白质暴露的羧酸盐增强了质子与细胞质通道孔口的相互作用。三个羧酸盐组成的簇作为一个强质子吸引位点,而一个被鉴定为D36的羧酸盐作为将质子传递到通道的介质。这些反应的组合使蛋白质表面具有质子收集天线的特性。收集区域的大小小于蛋白质表面的大小。

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