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Deposition of plasma fibronectin in tissues.血浆纤连蛋白在组织中的沉积。
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3
Primary structure of human plasma fibronectin--characterization of the 6,000 dalton C-terminal fragment containing the interchain disulfide bridges.人血浆纤连蛋白的一级结构——含链间二硫键的6000道尔顿C末端片段的特性分析
Biochem Biophys Res Commun. 1984 May 16;120(3):1015-21. doi: 10.1016/s0006-291x(84)80208-9.
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Cytoskeleton of rat aortic smooth muscle cells. Normal conditions and experimental intimal thickening.大鼠主动脉平滑肌细胞的细胞骨架。正常情况与实验性内膜增厚
Lab Invest. 1984 Jun;50(6):645-52.
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Intimal injury in vivo activates vascular smooth muscle cell migration and explant outgrowth in vitro.体内的内膜损伤会激活血管平滑肌细胞迁移,并在体外促进外植体生长。
Arteriosclerosis. 1984 May-Jun;4(3):183-8. doi: 10.1161/01.atv.4.3.183.
6
Actin expression in smooth muscle cells of rat aortic intimal thickening, human atheromatous plaque, and cultured rat aortic media.大鼠主动脉内膜增厚、人动脉粥样硬化斑块及培养的大鼠主动脉中膜平滑肌细胞中的肌动蛋白表达。
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Human fibronectin: cell specific alternative mRNA splicing generates polypeptide chains differing in the number of internal repeats.人纤连蛋白:细胞特异性可变mRNA剪接产生内部重复序列数量不同的多肽链。
Nucleic Acids Res. 1984 Jul 25;12(14):5853-68. doi: 10.1093/nar/12.14.5853.
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Cell surface interactions with extracellular materials.细胞表面与细胞外物质的相互作用。
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Plasma fibronectin is synthesized and secreted by hepatocytes.血浆纤连蛋白由肝细胞合成并分泌。
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Physiology of fibronectin.纤连蛋白的生理学
Annu Rev Med. 1984;35:561-75. doi: 10.1146/annurev.me.35.020184.003021.

血管平滑肌细胞中纤连蛋白额外结构域A序列的表达取决于细胞表型。

Expression of extra domain A fibronectin sequence in vascular smooth muscle cells is phenotype dependent.

作者信息

Glukhova M A, Frid M G, Shekhonin B V, Vasilevskaya T D, Grunwald J, Saginati M, Koteliansky V E

机构信息

Institute of Experimental Cardiology, Academy of Medical Sciences, Moscow, Union of Soviet Socialist Republics.

出版信息

J Cell Biol. 1989 Jul;109(1):357-66. doi: 10.1083/jcb.109.1.357.

DOI:10.1083/jcb.109.1.357
PMID:2663879
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2115465/
Abstract

Different fibronectin (FN) variants arise from the single gene transcript alternatively spliced in a tissue-specific manner (Hynes, R. O. 1985. Annu. Rev. Cell Biol. 1:67-90; Owens, R. J., A. R. Kornblihtt, and F. E. Baralle. 1986. Oxf. Surv. Eurcaryotic Genes. 3:141-160). We used mAb IST-9, specific for extra domain A (ED-A) FN sequence, and cDNA probe to ED-A exon to determine whether ED-A is present in FN synthesized by vascular smooth muscle cells (SMCs) and, if so, whether expression of ED-A is SMC phenotype dependent. ED-A-containing FN (A-FN) was not revealed in tunica media of human arteries and normal rat aorta by immunofluorescence and immunoblotting techniques. A cDNA probe to ED-A exon did not hybridize with RNA isolated from human aortic media. A positive reaction with IST-9 was observed in (a) diffuse intimal thickening and atherosclerotic plaque from human arteries; (b) experimentally induced intimal thickening in rat aorta; and (c) cultured vascular SMCs. A-FN mRNA was present in the RNA preparation from human aortic intima as judged by hybridization with cDNA probe to ED-A. On the other hand, an mAb interacting with an epitope common for all FN variants revealed FN in both intima and media of human arteries and in the normal rat aorta. A cDNA probe to a sequence shared by all FN variants hybridized with RNA from both intima and media of human aorta, though the level of expression was higher in intima. The data suggest that ED-A exon is omitted during splicing of the FN mRNA precursor in medial SMCs while the expression of A-FN is characteristic of "modulated" SMCs--those of intimal thickenings, of atherosclerotic lesions, and growing in culture.

摘要

不同的纤连蛋白(FN)变体源自单个基因转录本,该转录本以组织特异性方式进行可变剪接(海因斯,R.O. 1985.《细胞生物学年度评论》1:67 - 90;欧文斯,R.J.,A.R. 科恩布利特,和F.E. 巴拉莱。1986.《牛津真核基因综述》3:141 - 160)。我们使用针对额外结构域A(ED - A)FN序列的单克隆抗体IST - 9和ED - A外显子的cDNA探针,来确定ED - A是否存在于血管平滑肌细胞(SMC)合成的FN中,如果存在,ED - A的表达是否依赖于SMC表型。通过免疫荧光和免疫印迹技术,在人动脉的中膜以及正常大鼠主动脉中未检测到含ED - A的FN(A - FN)。ED - A外显子的cDNA探针未与人主动脉中膜分离的RNA杂交。在以下情况中观察到与IST - 9的阳性反应:(a)人动脉的弥漫性内膜增厚和动脉粥样硬化斑块;(b)大鼠主动脉实验性诱导的内膜增厚;(c)培养的血管SMC。通过与ED - A的cDNA探针杂交判断,人主动脉内膜的RNA制剂中存在A - FN mRNA。另一方面,一种与所有FN变体共有的表位相互作用的单克隆抗体在人动脉的内膜和中膜以及正常大鼠主动脉中均检测到FN。针对所有FN变体共有的序列的cDNA探针与人主动脉内膜和中膜的RNA杂交,尽管内膜中的表达水平更高。数据表明,在内侧SMC中,FN mRNA前体剪接过程中省略了ED - A外显子,而A - FN的表达是“调节型”SMC的特征——内膜增厚、动脉粥样硬化病变以及培养中生长的SMC的特征。