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在依赖ATP结合盒转运蛋白的途径中,大肠杆菌脂多糖O9a抗原组装过程中聚合、链终止和输出的协调。

Coordination of polymerization, chain termination, and export in assembly of the Escherichia coli lipopolysaccharide O9a antigen in an ATP-binding cassette transporter-dependent pathway.

作者信息

Clarke Bradley R, Greenfield Laura K, Bouwman Catrien, Whitfield Chris

机构信息

Department of Molecular and Cellular Biology, University of Guelph, Guelph, Ontario N1G 2W1, Canada.

出版信息

J Biol Chem. 2009 Oct 30;284(44):30662-72. doi: 10.1074/jbc.M109.052878. Epub 2009 Sep 4.

Abstract

The Escherichia coli O9a O-polysaccharide (O-PS) is a prototype for O-PS synthesis and export by the ATP-binding cassette transporter-dependent pathway. Comparable systems are widespread in Gram-negative bacteria. The polymannose O9a O-PS is assembled on a polyisoprenoid lipid intermediate by mannosyltransferases located at the cytoplasmic membrane, and the final polysaccharide chain length is determined by the chain terminating dual kinase/methyltransferase, WbdD. The WbdD protein is tethered to the membrane via a C-terminal region containing amphipathic helices located between residues 601 and 669. Here, we establish that the C-terminal domain of WbdD plays an additional pivotal role in assembly of the O-PS by forming a complex with the chain-extending mannosyltransferase, WbdA. Membrane preparations from a DeltawbdD mutant had severely diminished mannosyltransferase activity in vitro, and no significant amounts of the WbdA protein are targeted to the membrane fraction. Expression of a polypeptide comprising the WbdD C-terminal region was sufficient to restore both proper localization of WbdA and mannosyltransferase activity. In contrast to WbdA, the other required mannosyltransferases (WbdBC) are targeted to the membrane independent of WbdD. A bacterial two-hybrid system confirmed the interaction of WbdD and WbdA and identified two regions in the C terminus of WbdD that contributed to the interaction. Therefore, in the O9a assembly export system, the WbdD protein orchestrates the critical localization and coordination of activities involved in O-PS chain extension and termination at the cytoplasmic membrane.

摘要

大肠杆菌O9a O-多糖(O-PS)是通过ATP结合盒转运蛋白依赖性途径进行O-PS合成和输出的一个原型。类似的系统在革兰氏阴性菌中广泛存在。多聚甘露糖型O9a O-PS由位于细胞质膜的甘露糖基转移酶组装在聚异戊二烯脂质中间体上,最终多糖链的长度由链终止双激酶/甲基转移酶WbdD决定。WbdD蛋白通过包含位于601至669位残基之间的两亲性螺旋的C末端区域与膜相连。在此,我们证实WbdD的C末端结构域通过与链延伸甘露糖基转移酶WbdA形成复合物,在O-PS的组装中发挥了额外的关键作用。来自ΔwbdD突变体的膜制剂在体外的甘露糖基转移酶活性严重降低,并且没有大量的WbdA蛋白靶向到膜组分。包含WbdD C末端区域的多肽的表达足以恢复WbdA的正确定位和甘露糖基转移酶活性。与WbdA不同,其他必需的甘露糖基转移酶(WbdBC)靶向到膜与WbdD无关。细菌双杂交系统证实了WbdD和WbdA之间的相互作用,并确定了WbdD C末端的两个区域有助于这种相互作用。因此,在O9a组装输出系统中,WbdD蛋白协调了细胞质膜上O-PS链延伸和终止所涉及的关键定位和活性协调。

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