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首页> 美国卫生研究院文献>other >Dissecting structures and functions of SecA-only protein-conducting channels: ATPase pore structure ion channel activity protein translocation and interaction with SecYEG/SecDF•YajC
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Dissecting structures and functions of SecA-only protein-conducting channels: ATPase pore structure ion channel activity protein translocation and interaction with SecYEG/SecDF•YajC

机译:剖析仅SecA蛋白传导通道的结构和功能:ATPase孔结构离子通道活性蛋白易位以及与SecYEG / SecDF•YajC的相互作用

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SecA is an essential protein in the major bacterial Sec-dependent translocation pathways. E. coli SecA has 901 aminoacyl residues which form multi-functional domains that interact with various ligands to impart function. In this study, we constructed and purified tethered C-terminal deletion fragments of SecA to determine the requirements for N-terminal domains interacting with lipids to provide ATPase activity, pore structure, ion channel activity, protein translocation and interactions with SecYEG-SecDF•YajC. We found that the N-terminal fragment SecAN493 (SecA1-493) has low, intrinsic ATPase activity. Larger fragments have greater activity, becoming highest around N619-N632. Lipids greatly stimulated the ATPase activities of the fragments N608-N798, reaching maximal activities around N619. Three helices in amino-acyl residues SecA619-831, which includes the “Helical Scaffold” Domain (SecA619-668) are critical for pore formation, ion channel activity, and for function with SecYEG-SecDF•YajC. In the presence of liposomes, N-terminal domain fragments of SecA form pore-ring structures at fragment-size N640, ion channel activity around N798, and protein translocation capability around N831. SecA domain fragments ranging in size between N643-N669 are critical for functional interactions with SecYEG-SecDF•YajC. In the presence of liposomes, inactive C-terminal fragments complement smaller non-functional N-terminal fragments to form SecA-only pore structures with ion channel activity and protein translocation ability. Thus, SecA domain fragment interactions with liposomes defined critical structures and functional aspects of SecA-only channels. These data provide the mechanistic basis for SecA to form primitive, low-efficiency, SecA-only protein-conducting channels, as well as the minimal parameters for SecA to interact functionally with SecYEG-SecDF•YajC to form high-efficiency channels.
机译:SecA是主要细菌依赖Sec的易位途径中的必需蛋白。大肠杆菌SecA具有901个氨酰基残基,这些残基形成与多个配体相互作用以赋予功能的多功能域。在本研究中,我们构建并纯化了SecA的系链C末端缺失片段,以确定N末端域与脂质相互作用以提供ATPase活性,孔结构,离子通道活性,蛋白质易位以及与SecYEG-SecDF•YajC相互作用的要求。 。我们发现N末端片段SecAN493(SecA1-493)具有较低的固有ATPase活性。较大的片段具有更大的活性,在N619-N632附近变为最高。脂质极大地刺激了片段N608-N798的ATPase活性,在N619附近达到最大活性。氨基酰基残基SecA619-831中的三个螺旋(包括“螺旋支架”结构域(SecA619-668))对于孔的形成,离子通道活性以及SecYEG-SecDF•YajC的功能至关重要。在脂质体存在下,SecA的N末端结构域片段会在片段大小N640,N798附近的离子通道活性和N831附近的蛋白质易位能力上形成孔环结构。 SecA域片段的大小在N643-N669之间,对于与SecYEG-SecDF•YajC的功能相互作用至关重要。在脂质体的存在下,无活性的C末端片段与较小的非功能性N末端片段互补,形成仅具有离子通道活性和蛋白质易位能力的SecA孔结构。因此,SecA域片段与脂质体的相互作用定义了仅SecA通道的关键结构和功能方面。这些数据为SecA形成原始的,低效率的,仅SecA的蛋白传导通道提供了机械基础,以及SecA与SecYEG-SecDF•YajC在功能上相互作用以形成高效通道的最小参数。

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