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由内源性无规则转位结构域的竞争招募托宾蛋白的运动学基础。

Kinetic basis for the competitive recruitment of TolB by the intrinsically disordered translocation domain of colicin E9.

机构信息

Department of Biology (Area 10), University of York, Wentworth Way, Heslington, York YO10 5DD, UK.

出版信息

J Mol Biol. 2012 May 18;418(5):269-80. doi: 10.1016/j.jmb.2012.01.039. Epub 2012 Jan 30.

DOI:10.1016/j.jmb.2012.01.039
PMID:22310049
Abstract

TolB and Pal are members of the Tol-Pal system that spans the cell envelope of Gram-negative bacteria and contributes to the stability and integrity of the bacterial outer membrane (OM). Lipoylated Pal is tethered to the OM and binds the β-propeller domain of periplasmic TolB, which, as recent evidence suggests, disengages TolB from its interaction with other components of the Tol system in the inner membrane. Antibacterial nuclease colicins such as colicin E9 (ColE9) also bind the β-propeller domain of TolB in order to catalyze their translocation across the bacterial OM. In contrast to Pal, however, colicin binding to TolB promotes its interaction with other components of the Tol system. Here, through a series of pre-steady-state kinetic experiments utilizing fluorescence resonance energy transfer pairs within the individual protein-protein complexes, we establish the kinetic basis for such 'competitive recruitment' by the TolB-binding epitope (TBE) of ColE9. Surprisingly, the 16-residue disordered ColE9 TBE associates more rapidly with TolB than Pal, a folded 13-kDa protein. Moreover, we demonstrate that calcium ions, which bind within the confines of the TolB β-propeller domain tunnel and are known to increase the affinity of the TolB-ColE9 complex, do not exert their influence through long-range electrostatic effects, as had been predicted, but through short-range effects that slow the dissociation rate of ColE9 TBE from its complex with TolB. Our study demonstrates that an intrinsically disordered protein undergoing binding-induced folding can compete effectively with a globular protein for a common target by associating more rapidly than the globular protein.

摘要

托布和帕尔是跨越革兰氏阴性细菌细胞包膜的托布-帕尔系统的成员,有助于稳定和完整细菌外膜(OM)。脂酰化的帕尔被固定在 OM 上,并与周质中的 β- 桨叶结构域的 TolB 结合,最近的证据表明,这使 TolB 与其在内膜中的 Tol 系统的其他成分的相互作用脱离。抗菌核酸酶 colicins 如 colicin E9(ColE9)也结合 TolB 的 β- 桨叶结构域,以催化它们穿过细菌 OM 的易位。然而,与帕尔不同的是,colicin 与 TolB 的结合促进了其与 Tol 系统的其他成分的相互作用。在这里,通过利用单个蛋白质-蛋白质复合物内的荧光共振能量转移对进行的一系列准稳态动力学实验,我们确定了 ColE9 的 TolB 结合表位(TBE)进行这种“竞争招募”的动力学基础。令人惊讶的是,16 个残基无序的 ColE9 TBE 比折叠的 13kDa 蛋白帕尔更快地与 TolB 结合。此外,我们证明了钙离子在 TolB β- 桨叶结构域隧道内结合,已知其增加 TolB-ColE9 复合物的亲和力,但不是通过如前所述的远程静电效应,而是通过减慢 ColE9 TBE 与其与 TolB 复合物解离速率的短程效应来发挥作用。我们的研究表明,经历结合诱导折叠的固有无序蛋白质可以通过比球形蛋白质更快地结合来有效地与共同靶标竞争,从而有效地与球形蛋白质竞争。

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