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大肠杆菌中的能量转导:uncB基因座突变的生理和生化效应

Energy transduction in Escherichia coli: physiological and biochemical effects of mutation in the uncB locus.

作者信息

Hasan S M, Tsuchiya T, Rosen B P

出版信息

J Bacteriol. 1978 Jan;133(1):108-13. doi: 10.1128/jb.133.1.108-113.1978.

Abstract

The transduction of energy through biological membranes was investigated in Escherichia coli strains defective in the ATP synthetase complex. Everted vesicles prepared from strains containing an uncA or uncB mutation were compared with those of the parental strain for their ability to couple energy derived from the oxidation of substrates by the electron transport chain or from the hydrolysis of ATP by the Mg2+-adenosine triphosphatase, as measured by the energy-dependent quenching of quinacrine fluorescence or the active transport of 45Ca2+. Removal of the Mg2+-adenosine triphosphatase from membranes derived from the parental or an uncA strain caused a loss of energy-linked functions and a concomitant increase in the permeability of the membrane for protons. Proton impermeability was restored by treatment with N,N'-dicyclohexylcarbodiimide. When membranes of the uncB strain were treated in a similar manner, there was no loss of respiratory-driven functions, nor was there a change in proton permeability. These observations suggest that the uncB mutation specifically results in alteration of an intrinsic membrane protein channel necessary for the generation of utilzation of the electrochemical gradient of protons by that complex. Loss of the function of the proton channel is believed to prevent the transduction of energy through the ATP synthetase complex.

摘要

在ATP合成酶复合物存在缺陷的大肠杆菌菌株中,对通过生物膜的能量转导进行了研究。将含有uncA或uncB突变的菌株制备的外翻囊泡与亲本菌株的外翻囊泡进行比较,以研究它们通过电子传递链氧化底物或通过Mg2 + -腺苷三磷酸酶水解ATP所产生的能量进行偶联的能力,这通过喹吖因荧光的能量依赖性猝灭或45Ca2 +的主动转运来测量。从亲本菌株或uncA菌株来源的膜中去除Mg2 + -腺苷三磷酸酶会导致能量相关功能丧失,并伴随膜对质子的通透性增加。用N,N'-二环己基碳二亚胺处理可恢复质子不可渗透性。当以类似方式处理uncB菌株的膜时,呼吸驱动功能没有丧失,质子通透性也没有变化。这些观察结果表明,uncB突变特异性地导致一种内在膜蛋白通道的改变,该通道是该复合物产生或利用质子电化学梯度所必需的。质子通道功能的丧失被认为会阻止能量通过ATP合成酶复合物进行转导。

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