Robson Alice, Booth Antonia E G, Gold Vicki A M, Clarke Anthony R, Collinson Ian
Department of Biochemistry, University of Bristol, University Walk, Bristol, BS8 1TD, UK.
J Mol Biol. 2007 Dec 7;374(4):965-76. doi: 10.1016/j.jmb.2007.09.086. Epub 2007 Oct 4.
In bacteria, the SecYEG protein translocation complex employs the cytosolic ATPase SecA to couple the energy of ATP binding and hydrolysis to the mechanical force required to push polypeptides through the membrane. The molecular basis of this energy transducing reaction is not well understood. A peptide-binding array has been employed to identify sites on SecYEG that interact with SecA. These results along with fluorescence spectroscopy have been exploited to characterise a long-distance conformational change that connects the nucleotide-binding fold of SecA to the transmembrane polypeptide channel in SecY. These movements are driven by binding of non-hydrolysable ATP analogues to a monomer of SecA in association with the SecYEG complex. We also determine that interaction with SecYEG simultaneously decreases the affinity of SecA for ATP and inhibitory magnesium, favouring a previously identified active state of the ATPase. Mutants of SecA capable of binding but not hydrolysing ATP do not elicit this conformationally active state, implicating residues of the Walker B motif in the early chain of events that couple ATP binding to the mobility of the channel.
在细菌中,SecYEG 蛋白质转运复合物利用胞质 ATP 酶 SecA,将 ATP 结合与水解的能量与推动多肽穿过膜所需的机械力耦合起来。这种能量转换反应的分子基础尚未完全理解。已使用肽结合阵列来鉴定 SecYEG 上与 SecA 相互作用的位点。这些结果与荧光光谱法一起被用于表征一种长距离构象变化,该变化将 SecA 的核苷酸结合结构域与 SecY 中的跨膜多肽通道相连。这些运动由不可水解的 ATP 类似物与 SecYEG 复合物结合时与 SecA 单体的结合所驱动。我们还确定,与 SecYEG 的相互作用同时降低了 SecA 对 ATP 和抑制性镁的亲和力,有利于先前确定的 ATP 酶的活性状态。能够结合但不能水解 ATP 的 SecA 突变体不会引发这种构象活性状态,这表明沃克 B 基序的残基参与了将 ATP 结合与通道流动性耦合的早期事件链。