Rogers S L, McCarthy J B, Palm S L, Furcht L T, Letourneau P C
J Neurosci. 1985 Feb;5(2):369-78. doi: 10.1523/JNEUROSCI.05-02-00369.1985.
Proteolytic fragments of fibronectin were used to identify regions of the molecule that support neurite extension and to investigate further the differential behavior of central and peripheral nervous system neurons in response to fibronectin (Rogers, S. L., P. C. Letourneau, S. L. Palm, J. B. McCarthy, and L. T. Furcht (1983) Dev. Biol. 98: 212-220). Fibronectin fragments with differing biological activities were produced by proteolytic digestion with trypsin and cathepsin D and sequential affinity chromatography on gelatin-agarose and heparin-Sepharose. The resulting fragments (described by Smith, D. E., D. F. Mosher, R. B. Johnson, and L. T. Furcht (1982) J. Biol. Chem. 257: 5831-5838; Smith, D. E., and L. T. Furcht (1982) J. Biol. Chem. 257: 6518-6523 included an NH2-terminal 27,000-dalton peptide that weakly binds heparin, a 46,000-dalton gelatin-binding fragment, a series of fragments (80,000 to 125,000 daltons) from the center of the molecule containing previously described cell-binding activity, two major peptides of Mr = 33,000 and 66,000 that bind heparin strongly and are thought to originate from the A and B chains, respectively, of plasma fibronectin, and a 31,000-dalton COOH-terminal peptide containing a free sulfhydryl from the A chain of the molecule. Tissue culture dishes were treated with these proteolytic preparations, and dissociated embryonic chick peripheral (PNS) and central nervous system (CNS) cells were cultured on each experimental substratum in serum-free medium. The fibronectin fragments were evaluated for ability to promote cell attachment, neurite initiation, and maintenance of neurite growth. The 27,000-, 46,000-, and 31,000-dalton preparations did not promote cell attachment or neurite extension. Both PNS and CNS neurons attached to and extended stable neurites upon the COOH-terminal heparin-binding preparation containing the 33,000- and 66,000-dalton peptides. A differential response of the neurons to the 80,000- to 125,000-dalton "cell-binding" peptides was observed: whereas PNS neurons maintained neuritic growth on this preparation for at least 48 hr, CNS neurons extended neurites during the first 24 hr of culture but, by 48 hr, withdrew these neurites and became increasingly clumped. On the basis of (1) the observed neuronal responses to the heparin binding and "cell binding" regions, and (2) the different ligand-binding properties of these regions, we propose that cell attachment and neurite extension can be mediated and/or modulated by two separate regions of fibronectin and that cellular response to the intact molecule may involve multivalent interactions.
纤连蛋白的蛋白水解片段被用于识别该分子中支持神经突延伸的区域,并进一步研究中枢和外周神经系统神经元对纤连蛋白的不同反应(罗杰斯,S.L.,P.C.勒图尔诺,S.L.帕尔姆,J.B.麦卡锡和L.T.弗奇特(1983年)《发育生物学》98卷:212 - 220页)。通过用胰蛋白酶和组织蛋白酶D进行蛋白水解消化,并先后在明胶 - 琼脂糖和肝素 - 琼脂糖上进行亲和层析,产生了具有不同生物活性的纤连蛋白片段。所得片段(由史密斯,D.E.,D.F.莫舍,R.B.约翰逊和L.T.弗奇特(1982年)《生物化学杂志》257卷:5831 - 5838页;史密斯,D.E.和L.T.弗奇特(1982年)《生物化学杂志》257卷:6518 - 6523页描述)包括一个与肝素弱结合的氨基末端27,000道尔顿肽、一个46,000道尔顿的明胶结合片段、一系列来自分子中心的片段(80,000至125,000道尔顿),含有先前描述的细胞结合活性、两个主要的分子量分别为33,000和66,000的肽,它们与肝素强烈结合,被认为分别源自血浆纤连蛋白的A链和B链,以及一个来自分子A链的含有游离巯基的31,000道尔顿羧基末端肽。用这些蛋白水解制剂处理组织培养皿,并将解离的胚胎鸡外周(PNS)和中枢神经系统(CNS)细胞在无血清培养基中的每个实验基质上培养。评估纤连蛋白片段促进细胞附着、神经突起始和神经突生长维持的能力。27,000、46,000和31,000道尔顿的制剂不促进细胞附着或神经突延伸。PNS和CNS神经元都附着在含有33,000和66,000道尔顿肽的羧基末端肝素结合制剂上并延伸出稳定的神经突。观察到神经元对80,000至125,000道尔顿“细胞结合”肽的不同反应:PNS神经元在该制剂上至少维持神经突生长48小时,而CNS神经元在培养的最初24小时内延伸神经突,但到48小时时,收回这些神经突并变得越来越聚集。基于(1)观察到的神经元对肝素结合和“细胞结合”区域的反应,以及(2)这些区域不同的配体结合特性,我们提出细胞附着和神经突延伸可以由纤连蛋白的两个不同区域介导和/或调节,并且细胞对完整分子的反应可能涉及多价相互作用。
