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本文引用的文献

1
Beyond Cell-Cell Adhesion: Sensational Cadherins for Hearing and Balance.超越细胞间黏附:令人瞩目的黏附蛋白与听觉和平衡。
Cold Spring Harb Perspect Biol. 2018 Sep 4;10(9):a029280. doi: 10.1101/cshperspect.a029280.
2
An elastic element in the protocadherin-15 tip link of the inner ear.内耳原钙黏蛋白 15 顶端连接的弹性元件。
Nat Commun. 2016 Nov 18;7:13458. doi: 10.1038/ncomms13458.
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Processing of X-ray diffraction data collected in oscillation mode.振荡模式下收集的X射线衍射数据的处理。
Methods Enzymol. 1997;276:307-26. doi: 10.1016/S0076-6879(97)76066-X.
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Direct mechanical stimulation of tip links in hair cells through DNA tethers.通过DNA系链对毛细胞中的纤毛连接进行直接机械刺激。
Elife. 2016 Jun 22;5:e16041. doi: 10.7554/eLife.16041.
5
The CD2 isoform of protocadherin-15 is an essential component of the tip-link complex in mature auditory hair cells.原钙黏蛋白-15的CD2亚型是成熟听觉毛细胞中顶连接复合体的重要组成部分。
EMBO Mol Med. 2014 Jul;6(7):984-92. doi: 10.15252/emmm.201403976.
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CHARMM36 all-atom additive protein force field: validation based on comparison to NMR data.CHARMM36 全原子加和蛋白力场:基于 NMR 数据比较的验证。
J Comput Chem. 2013 Sep 30;34(25):2135-45. doi: 10.1002/jcc.23354. Epub 2013 Jul 6.
7
Molecular remodeling of tip links underlies mechanosensory regeneration in auditory hair cells.尖端链接的分子重塑是听觉毛细胞机械感觉再生的基础。
PLoS Biol. 2013;11(6):e1001583. doi: 10.1371/journal.pbio.1001583. Epub 2013 Jun 11.
8
Noddy, a mouse harboring a missense mutation in protocadherin-15, reveals the impact of disrupting a critical interaction site between tip-link cadherins in inner ear hair cells.Noddy 是一只携带有原钙黏蛋白 15 错义突变的老鼠,揭示了破坏内耳毛细胞尖端连接黏附蛋白之间关键相互作用位点的影响。
J Neurosci. 2013 Mar 6;33(10):4395-404. doi: 10.1523/JNEUROSCI.4514-12.2013.
9
Structure of a force-conveying cadherin bond essential for inner-ear mechanotransduction.力传导钙黏着蛋白键的结构对于内耳机械转导至关重要。
Nature. 2012 Dec 6;492(7427):128-32. doi: 10.1038/nature11590. Epub 2012 Nov 7.
10
Thinking outside the cell: how cadherins drive adhesion.跳出细胞看问题:钙黏蛋白如何驱动黏附。
Trends Cell Biol. 2012 Jun;22(6):299-310. doi: 10.1016/j.tcb.2012.03.004. Epub 2012 May 1.

通过原钙黏蛋白-15的可变剪接变体调节内耳纤毛尖端连接亲和力

Tuning Inner-Ear Tip-Link Affinity Through Alternatively Spliced Variants of Protocadherin-15.

作者信息

Narui Yoshie, Sotomayor Marcos

机构信息

Department of Chemistry and Biochemistry , The Ohio State University , Columbus , Ohio 43210 , United States.

出版信息

Biochemistry. 2018 Mar 20;57(11):1702-1710. doi: 10.1021/acs.biochem.7b01075. Epub 2018 Mar 6.

DOI:10.1021/acs.biochem.7b01075
PMID:29443515
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5892193/
Abstract

Human hearing relies upon the tip-to-tip interaction of two nonclassical cadherins, protocadherin-15 (PCDH15) and cadherin-23 (CDH23). Together, these proteins form a filament called the tip link that connects neighboring stereocilia of mechanosensitive hair cells. As sound waves enter the cochlea, the stereocilia deflect and tension is applied to the tip link, opening nearby transduction channels. Disruption of the tip link by loud sound or calcium chelators eliminates transduction currents and illustrates that tip-link integrity is critical for mechanosensing. Tip-link remodeling after disruption is a dynamic process, which can lead to the formation of atypical complexes that incorporate alternatively spliced variants of PCDH15. These variants are categorized into six groups (N1-N6) based upon differences in the first two extracellular cadherin (EC) repeats. Here, we characterized the two N-terminal EC repeats of all PCDH15 variants (pcdh15(N1) to pcdh15(N6)) and combined these variants to test complex formation. We solved the crystal structure of a new complex composed of CDH23 EC1-2 (cdh23) and pcdh15(N2) at 2.3 Å resolution and compared it to the canonical cdh23-pcdh15(N1) complex. While there were subtle structural differences, the binding affinity between cdh23 and pcdh15(N2) is ∼6 times weaker than cdh23 and pcdh15(N1) as determined by surface plasmon resonance analysis. Steered molecular dynamics simulations predict that the unbinding force of the cdh23-pcdh15(N2) complex can be lower than the canonical tip link. Our results demonstrate that alternative heterophilic tip-link structures form stable protein-protein interactions in vitro and suggest that homophilic PCDH15-PCDH15 tip links form through the interaction of additional EC repeats.

摘要

人类听觉依赖于两种非经典钙黏蛋白原钙黏蛋白-15(PCDH15)和钙黏蛋白-23(CDH23)的尖端对尖端相互作用。这些蛋白质共同形成一种称为尖端连接的细丝,连接机械敏感毛细胞的相邻静纤毛。当声波进入耳蜗时,静纤毛发生偏转,张力作用于尖端连接,打开附近的转导通道。大声或钙螯合剂破坏尖端连接会消除转导电流,表明尖端连接的完整性对于机械传感至关重要。破坏后的尖端连接重塑是一个动态过程,可导致形成包含PCDH15可变剪接变体的非典型复合物。这些变体根据前两个细胞外钙黏蛋白(EC)重复序列的差异分为六组(N1-N6)。在这里,我们对所有PCDH15变体(pcdh15(N1)至pcdh15(N6))的两个N端EC重复序列进行了表征,并将这些变体组合起来测试复合物的形成。我们以2.3埃的分辨率解析了由CDH23 EC1-2(cdh23)和pcdh15(N2)组成的新复合物的晶体结构,并将其与经典的cdh23-pcdh15(N1)复合物进行了比较。虽然存在细微的结构差异,但通过表面等离子体共振分析确定,cdh23与pcdh15(N2)之间的结合亲和力比cdh23与pcdh15(N1)弱约6倍。引导分子动力学模拟预测,cdh23-pcdh15(N2)复合物的解离力可能低于经典的尖端连接。我们的结果表明,替代的异嗜性尖端连接结构在体外形成稳定的蛋白质-蛋白质相互作用,并表明同嗜性PCDH15-PCDH15尖端连接通过额外EC重复序列的相互作用形成。