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类囊体膜中的质子通道CF0。只有一小部分缺乏CF1的CF0具有高单位电导率(169飞西门子)且处于活性状态。

The proton channel, CF0, in thylakoid membranes. Only a low proportion of CF1-lacking CF0 is active with a high unit conductance (169 fS).

作者信息

Lill H, Engelbrecht S, Schönknecht G, Junge W

出版信息

Eur J Biochem. 1986 Nov 3;160(3):627-34. doi: 10.1111/j.1432-1033.1986.tb10084.x.

Abstract

We investigated the conductance of pea thylakoid membranes and their capacity for photophosphorylation as function of the extraction of chloroplast coupling factor CF1. The degree of extraction was varied via the incubation time in EDTA-containing hypo-osmolar medium and was measured by rocket electroimmunodiffusion. The conductance of thylakoid membranes was measured by flash kinetic spectrophotometry. The time course of extraction followed the time course of thylakoid swelling. Contrary to expectation increasing loss of CF1 did not primarily increase the velocity of proton efflux from each vesicle. Instead proton-tight vesicles were converted to leaky ones, which lost phosphorylating activity. Two subpopulations occurred, although both types of vesicles, leaky and proton-tight ones, were CF1-depleted to a similar degree. This implied that only a small fraction of CF1-lacking CF0 was functional as a proton channel. Tight vesicles had no functional channels while leaky ones had at least one. We determined the proportion of tight vesicles in three independent ways: via the residual phosphorylation activity, via measurements of proton efflux and via measurements of the electric relaxation across the membrane. The results obtained were identical. A statistical evaluation of the data led us to the following conclusions. EDTA treatment produced vesicles containing approximately 10(5) chlorophyll molecules, equivalent to a total of approximately 100 CF0CF1 per vesicle. Even at the highest degree of extraction (75% of total CF1 extracted) only 2.5 out of 75 exposed CF0 per vesicle were proton-conducting. The unit conductance of one open CF0 channel was 169 +/- 18 fS at pH 7.5 and room temperature. At an electrical driving force of 100 mV this was equivalent to the passage of approximately 10(5) protons/s. The most important consequence of this relatively high unit conductance was that a single open CF0 channel was capable of dissipating the protonmotive force of one vesicle, thereby deactivating the whole remaining catalytic capacity of this vesicle.

摘要

我们研究了豌豆类囊体膜的电导率及其光磷酸化能力与叶绿体偶联因子CF1提取量的关系。通过在含EDTA的低渗培养基中的孵育时间来改变提取程度,并通过火箭免疫电泳法进行测定。类囊体膜的电导率通过闪光动力学分光光度法进行测量。提取的时间进程与类囊体肿胀的时间进程一致。与预期相反,CF1损失的增加并没有主要提高每个囊泡中质子外流的速度。相反,质子紧密的囊泡转变为有泄漏的囊泡,失去了磷酸化活性。出现了两个亚群,尽管泄漏型和质子紧密型这两种类型的囊泡CF1都被消耗到了相似的程度。这意味着只有一小部分缺乏CF1的CF0作为质子通道起作用。紧密型囊泡没有功能性通道,而泄漏型囊泡至少有一个。我们通过三种独立的方法确定了紧密型囊泡的比例:通过残余磷酸化活性、通过质子外流测量以及通过膜上电弛豫测量。得到的结果是相同的。对数据的统计评估得出了以下结论。EDTA处理产生的囊泡含有约10⁵个叶绿素分子,相当于每个囊泡总共约100个CF0CF1。即使在最高提取程度(提取了总CF1的75%)时,每个囊泡中暴露的75个CF0中只有2.5个是质子传导性的。在pH 7.5和室温下,一个开放的CF0通道的单位电导率为169±18 fS。在100 mV的电驱动力下,这相当于每秒约10⁵个质子通过。这种相对较高的单位电导率最重要的结果是,单个开放的CF0通道能够耗散一个囊泡的质子动力,从而使该囊泡剩余的整个催化能力失活。

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