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面向内的 MetNI 甲硫氨酸 ABC 转运蛋白构象:对反抑制机制的影响。

Inward facing conformations of the MetNI methionine ABC transporter: Implications for the mechanism of transinhibition.

机构信息

Division of Chemistry and Chemical Engineering 114-96, California Institute of Technology, Pasadena, CA 91125, USA.

出版信息

Protein Sci. 2012 Jan;21(1):84-96. doi: 10.1002/pro.765. Epub 2011 Dec 5.

DOI:10.1002/pro.765
PMID:22095702
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3323783/
Abstract

Two new crystal structures of the Escherichia coli high affinity methionine uptake ATP Binding Cassette (ABC) transporter MetNI, purified in the detergents cyclohexyl-pentyl-β-D-maltoside (CY5) and n-decyl-β-D-maltopyranoside (DM), have been solved in inward facing conformations to resolutions of 2.9 and 4.0 Å, respectively. Compared to the previously reported 3.7 Å resolution structure of MetNI purified in n-dodecyl-β-D-maltopyranoside (DDM), the higher resolution of the CY5 data enabled significant improvements to the structural model in several regions, including corrections to the sequence registry, and identification of ADP in the nucleotide binding site. CY5 crystals soaked with selenomethionine established details of the methionine binding site in the C2 regulatory domain of the ABC subunit, including the displacement of the side chain of MetN residue methionine 301 by the exogenous ligand. When compared to the CY5 or DDM structures, the DM structure exhibits a significant repositioning of the dimeric C2 domains, including an unexpected register shift in the intermolecular β-sheet hydrogen bonding between monomers, and a narrowing of the nucleotide binding space. The immediate proximity of the exogenous methionine binding site to the conformationally variable dimeric interface provides an indication of how methionine binding to the regulatory domains might mediate the phenomenon of transinhibition.

摘要

两个新的大肠杆菌高亲和力蛋氨酸摄取 ATP 结合盒(ABC)转运蛋白 MetNI 的晶体结构,分别在去污剂环己基戊基-β-D-麦芽糖苷(CY5)和正癸基-β-D-麦芽糖苷(DM)中以内向构象的形式进行了纯化,分辨率分别为 2.9 和 4.0 Å。与之前在正十二烷基-β-D-麦芽糖苷(DDM)中纯化的 3.7 Å 分辨率的 MetNI 结构相比,CY5 数据的更高分辨率使结构模型在几个区域得到了显著改善,包括序列登记处的校正和核苷酸结合位点中 ADP 的鉴定。用硒代蛋氨酸浸泡的 CY5 晶体确定了 ABC 亚基 C2 调节域中蛋氨酸结合位点的详细信息,包括外源配体取代 MetN 残基蛋氨酸 301 的侧链。与 CY5 或 DDM 结构相比,DM 结构表现出二聚体 C2 结构域的显著重新定位,包括单体间分子间β-折叠氢键的意想不到的注册移位,以及核苷酸结合空间的变窄。外源性蛋氨酸结合位点与构象可变二聚体界面的紧邻接近表明,蛋氨酸与调节域的结合如何介导反抑制现象。

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