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通过计算机模拟方法揭示了双糖链蛋白聚糖、核心蛋白聚糖、纤维调节蛋白和光蛋白聚糖对基质金属蛋白酶-14的差异靶向作用。

Differential MMP-14 targeting by biglycan, decorin, fibromodulin, and lumican unraveled by in silico approach.

作者信息

Rivet Romain, Rao Rajas Mallenahalli, Nizet Pierre, Belloy Nicolas, Huber Louise, Dauchez Manuel, Ramont Laurent, Baud Stéphanie, Brézillon Stéphane

机构信息

CNRS UMR 7369, Matrice Extracellulaire et Dynamique Cellulaire (MEDyC), Université de Reims Champagne Ardenne, Reims, France.

P3M, Multi-Scale-Molecular Modeling Platform, Université de Reims Champagne Ardenne, Reims, France.

出版信息

Am J Physiol Cell Physiol. 2023 Feb 1;324(2):C353-C365. doi: 10.1152/ajpcell.00429.2022. Epub 2022 Dec 19.

DOI:10.1152/ajpcell.00429.2022
PMID:36534501
Abstract

Small leucine-rich proteoglycans (SLRPs) are major regulators of extracellular matrix assembly and cell signaling. Lumican, a member of the SLRPs family, and its derived peptides were shown to possess antitumor activity by interacting directly with the catalytic domain of MMP-14 leading to the inhibition of its activity. The aim of the present report was to characterize by in silico three-dimensional (3D) modeling the structure and the dynamics of four SLRPs including their core protein and their specific polysaccharide chains to assess their capacity to bind to MMP-14 and to regulate its activity. Molecular docking experiments were performed to identify the specific amino acids of MMP-14 interacting with each of the four SLRPs. The inhibition of each SLRP (100 nM) on MMP-14 activity was measured and the constants of inhibition () were evaluated. The impact of the number of glycan chains, structures, and dynamics of lumican on the interaction with MMP-14 was assessed by molecular dynamics simulations. Molecular docking analysis showed that all SLRPs bind to MMP-14 through their concave face, but in different regions of the catalytic domain of MMP-14. Each SLRPs inhibited significantly the MMP-14 activity. Finally, molecular dynamics showed the role of glycan chains in interaction with MMP-14 and shielding effect of SLRPs. Altogether, the results demonstrated that each SLRP exhibited inhibition of MMP-14 activity. However, the differential targeting of MMP-14 by the SLRPs was shown to be related not only to the core protein conformation but also to the glycan chain structures and dynamics.

摘要

富含亮氨酸的小分子蛋白聚糖(SLRPs)是细胞外基质组装和细胞信号传导的主要调节因子。Lumican是SLRPs家族的成员之一,其衍生肽通过直接与MMP - 14的催化结构域相互作用而具有抗肿瘤活性,从而导致其活性受到抑制。本报告的目的是通过计算机三维(3D)建模来表征四种SLRPs的结构和动力学,包括其核心蛋白及其特定的多糖链,以评估它们与MMP - 14结合并调节其活性的能力。进行分子对接实验以确定与四种SLRPs中的每一种相互作用的MMP - 14的特定氨基酸。测量了每种SLRP(100 nM)对MMP - 14活性的抑制作用,并评估了抑制常数()。通过分子动力学模拟评估了Lumican的聚糖链数量、结构和动力学对与MMP - 14相互作用的影响。分子对接分析表明,所有SLRPs都通过其凹面与MMP - 14结合,但在MMP - 14催化结构域的不同区域。每种SLRPs都显著抑制了MMP - 14的活性。最后,分子动力学显示了聚糖链在与MMP - 14相互作用中的作用以及SLRPs的屏蔽效应。总之,结果表明每种SLRP都表现出对MMP - 14活性的抑制作用。然而,SLRPs对MMP - 14的差异靶向不仅与核心蛋白构象有关,还与聚糖链结构和动力学有关。

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