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2
Display of cell surface sites for fibronectin assembly is modulated by cell adherence to (1)F3 and C-terminal modules of fibronectin.纤连蛋白组装的细胞表面位点的展示受细胞对纤连蛋白的(1)F3和C末端模块的粘附调节。
PLoS One. 2009;4(1):e4113. doi: 10.1371/journal.pone.0004113. Epub 2009 Jan 1.
3
Fibrillin assembly requires fibronectin.原纤维蛋白组装需要纤连蛋白。
Mol Biol Cell. 2009 Feb;20(3):846-58. doi: 10.1091/mbc.e08-08-0830. Epub 2008 Nov 26.
4
Isoaspartate-glycine-arginine: a new tumor vasculature-targeting motif.异天冬氨酸-甘氨酸-精氨酸:一种新的肿瘤血管靶向基序。
Cancer Res. 2008 Sep 1;68(17):7073-82. doi: 10.1158/0008-5472.CAN-08-1272.
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Crystal structures of fibronectin-binding sites from Staphylococcus aureus FnBPA in complex with fibronectin domains.金黄色葡萄球菌FnBPA的纤连蛋白结合位点与纤连蛋白结构域复合物的晶体结构。
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Fibrillin-1 microfibril deposition is dependent on fibronectin assembly.原纤蛋白-1微原纤维沉积依赖于纤连蛋白组装。
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7
The role of integrin binding sites in fibronectin matrix assembly in vivo.整合素结合位点在体内纤连蛋白基质组装中的作用。
Curr Opin Cell Biol. 2008 Oct;20(5):502-7. doi: 10.1016/j.ceb.2008.06.001. Epub 2008 Jul 21.
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The neovasculature homing motif NGR: more than meets the eye.新生血管归巢基序NGR:不止于所见。
Blood. 2008 Oct 1;112(7):2628-35. doi: 10.1182/blood-2008-04-150862. Epub 2008 Jun 23.
9
Structural basis for the interaction of isoDGR with the RGD-binding site of alphavbeta3 integrin.异天冬酰胺-甘氨酸-精氨酸(isoDGR)与αvβ3整合素的RGD结合位点相互作用的结构基础。
J Biol Chem. 2008 Jul 11;283(28):19757-68. doi: 10.1074/jbc.M710273200. Epub 2008 May 13.
10
Extracellular matrix: from atomic resolution to ultrastructure.细胞外基质:从原子分辨率到超微结构
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异源二聚体 G 蛋白偶联受体序列不介导纤连蛋白 N 端结构域与贴壁型纤连蛋白缺失成纤维细胞的结合。

iso-DGR sequences do not mediate binding of fibronectin N-terminal modules to adherent fibronectin-null fibroblasts.

机构信息

Department of Biomolecular Chemistry and Medicine, University of Wisconsin, Madison, Wisconsin 53706, USA.

出版信息

J Biol Chem. 2010 Mar 19;285(12):8563-71. doi: 10.1074/jbc.M109.062646. Epub 2010 Jan 22.

DOI:10.1074/jbc.M109.062646
PMID:20097751
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2838278/
Abstract

Fibronectin (FN) without an RGD sequence (FN-RGE), and thus lacking the principal binding site for alpha5beta1 integrin, is deposited into the extracellular matrix of mouse embryos. Spontaneous conversion of (263)NGR and/or (501)NGR to iso-DGR possibly explains this enigma, i.e. ligation of iso-DGR by alphavbeta3 integrin may allow cells to assemble FN. Partial modification of (263)NGR to DGR or iso-DGR was detected in purified plasma FN by mass spectrometry. To test functions of the conversion, one or both NGR sequences were mutated to QGR in recombinant N-terminal 70-kDa construct of FN (70K), full-length FN, or FN-RGE. The mutations did not affect the binding of soluble 70K to already adherent fibroblasts or the ability of soluble 70K to compete with non-mutant FN or FN-RGE for binding to FN assembly sites. Non-mutant FN and FN-N263Q/N501Q with both NGRs mutated to QGRs were assembled equally well by adherent fibroblasts. FN-RGE and FN-RGE-N263Q/N501Q were also assembled equally well. Although substrate-bound 70K mediated cell adhesion in the presence of 1 mm Mn(2+) by a mechanism that was inhibited by cyclic RGD peptide, the peptide did not inhibit 70K binding to cell surface. Mutations of the NGR sequences had no effect on Mn(2+)-enhanced cell adhesion to adsorbed 70K but caused a decrease in cell adhesion to reduced and alkylated 70K. These results demonstrate that iso-DGR sequences spontaneously converted from NGR are cryptic and do not mediate the interaction of the 70K region of FN with the cell surface during FN assembly.

摘要

纤连蛋白(FN)不含 RGD 序列(FN-RGE),因此缺乏与α5β1 整合素的主要结合位点,被沉积到小鼠胚胎的细胞外基质中。(263)NGR 和/或(501)NGR 自发转化为 iso-DGR 可能解释了这个谜,即αvβ3 整合素结合 iso-DGR 可能允许细胞组装 FN。通过质谱法在纯化的血浆 FN 中检测到(263)NGR 向 DGR 或 iso-DGR 的部分修饰。为了测试转化的功能,在重组 FN(70K)的 N 端 70kDa 结构域(70K)、全长 FN 或 FN-RGE 的 NGR 序列中一个或两个都突变为 QGR。突变不影响可溶性 70K 与已附着的成纤维细胞的结合,也不影响可溶性 70K 与非突变 FN 或 FN-RGE 竞争结合 FN 组装位点的能力。非突变 FN 和 FN-N263Q/N501Q 中两个 NGR 都突变为 QGRs,均由附着的成纤维细胞组装。FN-RGE 和 FN-RGE-N263Q/N501Q 也同样组装。尽管在 1mm Mn(2+)存在下,基质结合的 70K 通过一种被环状 RGD 肽抑制的机制介导细胞黏附,但该肽不抑制 70K 与细胞表面的结合。NGR 序列的突变对 Mn(2+)增强的吸附 70K 上的细胞黏附没有影响,但导致降低和烷基化的 70K 上的细胞黏附减少。这些结果表明,从 NGR 自发转化而来的 iso-DGR 序列是隐蔽的,在 FN 组装过程中不会介导 FN 的 70K 区域与细胞表面的相互作用。