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异源二聚体ABC转运蛋白EfrCD中不对称核苷酸结合位点的拆分任务

Split tasks of asymmetric nucleotide-binding sites in the heterodimeric ABC exporter EfrCD.

作者信息

Hürlimann Lea M, Hohl Michael, Seeger Markus A

机构信息

Institute of Medical Microbiology, University of Zurich, Switzerland.

出版信息

FEBS J. 2017 Jun;284(11):1672-1687. doi: 10.1111/febs.14065. Epub 2017 Apr 18.

DOI:10.1111/febs.14065
PMID:28417533
Abstract

Many heterodimeric ATP-binding cassette (ABC) exporters evolved asymmetric ATP-binding sites containing a degenerate site incapable of ATP hydrolysis due to noncanonical substitutions in conserved sequence motifs. Recent studies revealed that nucleotide binding to the degenerate site stabilizes contacts between the nucleotide-binding domains (NBDs) of the inward-facing transporter and regulates ATP hydrolysis at the consensus site via allosteric coupling mediated by the D-loops. However, it is unclear whether nucleotide binding to the degenerate site is strictly required for substrate transport. In this study, we examined the functional consequences of a systematic set of mutations introduced at the degenerate and consensus site of the multidrug efflux pump EfrCD of Enterococcus faecalis. Mutating motifs which differ among the two ATP-binding sites (Walker B, switch loop, and ABC signature) or which are involved in interdomain communication (D-loop and Q-loop) led to asymmetric results in the functional assays and were better tolerated at the degenerate site. This highlights the importance of the degenerate site to allosterically regulate the events at the consensus site. Mutating invariant motifs involved in ATP binding and NBD closure (A-loop and Walker A) resulted in equally reduced transport activities, regardless at which ATP-binding site they were introduced. In contrast to previously investigated heterodimeric ABC exporters, mutation of the degenerate site Walker A lysine completely inactivated ATPase activity and substrate transport, indicating that ATP binding to the degenerate site is essential for EfrCD. This study provides novel insights into the split tasks of asymmetric ATP-binding sites of heterodimeric ABC exporters.

摘要

许多异源二聚体ATP结合盒(ABC)转运蛋白进化出不对称的ATP结合位点,其中包含一个由于保守序列基序中的非典型取代而无法进行ATP水解的简并位点。最近的研究表明,核苷酸与简并位点的结合稳定了内向转运蛋白的核苷酸结合结构域(NBD)之间的接触,并通过D环介导的变构偶联调节共有位点处的ATP水解。然而,尚不清楚核苷酸与简并位点的结合对于底物转运是否是严格必需的。在本研究中,我们研究了在粪肠球菌多药外排泵EfrCD的简并位点和共有位点引入的一系列系统性突变的功能后果。突变两个ATP结合位点之间不同的基序(沃克B、开关环和ABC特征)或参与结构域间通讯的基序(D环和Q环)在功能测定中导致不对称结果,并且在简并位点更易耐受。这突出了简并位点对变构调节共有位点事件的重要性。突变参与ATP结合和NBD闭合的不变基序(A环和沃克A)导致转运活性同样降低,无论它们是在哪个ATP结合位点引入的。与先前研究的异源二聚体ABC转运蛋白相反,简并位点沃克A赖氨酸的突变完全使ATP酶活性和底物转运失活,表明ATP与简并位点的结合对EfrCD至关重要。本研究为异源二聚体ABC转运蛋白不对称ATP结合位点的分工提供了新的见解。

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