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ABC 蛋白 DrrA 的极端 C 末端包含参与 DrrAB 复合物功能和组装的独特基序。

The extreme C terminus of the ABC protein DrrA contains unique motifs involved in function and assembly of the DrrAB complex.

机构信息

Department of Biology, Georgia State University, Atlanta, Georgia 30303, USA.

出版信息

J Biol Chem. 2010 Dec 3;285(49):38324-36. doi: 10.1074/jbc.M110.131540. Epub 2010 Sep 27.

Abstract

Two novel regulatory motifs, LDEVFL and C-terminal regulatory Glu (E)-rich motif (CREEM), are identified in the extreme C terminus of the ABC protein DrrA, which is involved in direct interaction with the N-terminal cytoplasmic tail of the membrane protein DrrB and in homodimerization of DrrA. Disulfide cross-linking analysis showed that the CREEM and the region immediately upstream of CREEM participate directly in forming an interaction interface with the N terminus of DrrB. A series of mutations created in the LDEVFL and CREEM motifs drastically affected overall function of the DrrAB transporter. Mutations in the LDEVFL motif also significantly impaired interaction between the C terminus of DrrA and the N terminus of DrrB as well as the ability of DrrA and DrrB to co-purify, therefore suggesting that the LDEVFL motif regulates CREEM-mediated interaction between DrrA and DrrB and plays a key role in biogenesis of the DrrAB complex. Modeling analysis indicated that the LDEVFL motif is critical for conformational integrity of the C-terminal domain of DrrA and confirmed that the C terminus of DrrA forms an independent domain. This is the first report which describes the presence of an assembly domain in an ABC protein and uncovers a novel mechanism whereby the ABC component facilitates the assembly of the membrane component. Homology sequence comparisons showed the presence of the LDEVFL and CREEM motifs in close prokaryotic and eukaryotic homologs of DrrA, suggesting that these motifs may play a similar role in other homologous drug and lipid export systems.

摘要

两个新的调控基序,LDEVFL 和 C 末端调控谷氨酸(E)丰富基序(CREEM),在 ABC 蛋白 DrrA 的极端 C 末端被鉴定出来,该蛋白参与与膜蛋白 DrrB 的 N 端胞质尾直接相互作用,并介导 DrrA 二聚化。二硫键交联分析表明,CREEM 和 CREEM 上游区域直接参与与 DrrB N 端形成相互作用界面。在 LDEVFL 和 CREEM 基序中创建的一系列突变极大地影响了 DrrAB 转运体的整体功能。在 LDEVFL 基序中的突变也显著削弱了 DrrA C 末端与 DrrB N 端之间的相互作用,以及 DrrA 和 DrrB 共同纯化的能力,因此表明 LDEVFL 基序调节 CREEM 介导的 DrrA 和 DrrB 之间的相互作用,并在 DrrAB 复合物的生物发生中发挥关键作用。建模分析表明,LDEVFL 基序对于 DrrA C 末端结构域的构象完整性至关重要,并证实 DrrA 的 C 末端形成独立的结构域。这是首次描述 ABC 蛋白中存在组装结构域的报道,并揭示了 ABC 组件促进膜组件组装的新机制。同源序列比较表明,在 DrrA 的密切原核和真核同源物中存在 LDEVFL 和 CREEM 基序,表明这些基序可能在其他同源药物和脂质出口系统中发挥类似作用。

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