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鞭毛蛋白激活 Toll 样受体 5 的识别基序的扩展和细化。

Extension and refinement of the recognition motif for Toll-like receptor 5 activation by flagellin.

机构信息

Department of Synthetic Biology and Immunology, National Institute of Chemistry, Ljubljana, Slovenia.

Centre of Excellence EN-FIST, Ljubljana, Slovenia.

出版信息

J Leukoc Biol. 2018 Oct;104(4):767-776. doi: 10.1002/JLB.3VMA0118-035R. Epub 2018 Jun 19.

DOI:10.1002/JLB.3VMA0118-035R
PMID:29920759
Abstract

TLRs sense conserved and essential molecular components of microbes that invade multicellular organisms. The wide range of TLR agonists, differing in size and shape, is recognized either through a single or a pair of binding sites on the ectodomains of TLRs. TLR5 recognizes bacterial flagellin through two distinct binding sites on the ectodomain, the first facilitating primary binding of flagellin and the second guiding receptor dimerization necessary for signaling. The regions of flagellin recognized by TLR5 encompass key functional regions within the D1 domain of flagellin, which is also required for the assembly of functional flagella. In addition to previously identified binding sites at the N-terminal and central segment of the TLR5 ectodomain, we extended the TLR5'-D1 interaction interface on TLR5 and showed a species-specific recognition relevance of this extended region. In addition, we showed that the loop and following β-hairpin region of flagellin, previously proposed to participate in the TLR5-flagellin dimerization interface, is not accountable for these species-specific differences. We further identified residues that contribute to the interaction between two TLR5 ectodomains in an active signaling complex. Our work demonstrates that flagellin is recognized by TLR5 through a more extensive interaction surface than previously characterized.

摘要

TLRs 能够感知入侵多细胞生物的微生物中保守且必需的分子成分。TLRs 的配体范围广泛,大小和形状各异,通过 TLRs 胞外域上的一个或一对结合位点来识别。TLR5 通过胞外域上的两个不同结合位点识别细菌鞭毛蛋白,第一个结合位点促进鞭毛蛋白的初始结合,第二个结合位点引导受体二聚化,这对于信号转导是必需的。TLR5 识别的鞭毛蛋白区域包含鞭毛蛋白 D1 结构域内的关键功能区域,这也是功能性鞭毛组装所必需的。除了先前在 TLR5 胞外域的 N 端和中央片段中鉴定出的结合位点外,我们扩展了 TLR5 的 TLR5'-D1 相互作用界面,并显示了该扩展区域的种属特异性识别相关性。此外,我们还表明,先前提出参与 TLR5-鞭毛蛋白二聚化界面的鞭毛蛋白的环和随后的β发夹区域,不能解释这些种属特异性差异。我们进一步确定了在活性信号复合物中有助于两个 TLR5 胞外域相互作用的残基。我们的工作表明,鞭毛蛋白通过比先前表征的更广泛的相互作用表面被 TLR5 识别。

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