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HNK-1碳水化合物介导的细胞与层粘连蛋白-1的黏附不同于肝素介导和硫苷脂介导的细胞黏附。

HNK-1 carbohydrate-mediated cell adhesion to laminin-1 is different from heparin-mediated and sulfatide-mediated cell adhesion.

作者信息

Hall H, Deutzmann R, Timpl R, Vaughan L, Schmitz B, Schachner M

机构信息

Department of Neurobiology, Swiss Federal Institute of Technology, Hönggerberg.

出版信息

Eur J Biochem. 1997 May 15;246(1):233-42. doi: 10.1111/j.1432-1033.1997.t01-1-00233.x.

DOI:10.1111/j.1432-1033.1997.t01-1-00233.x
PMID:9210489
Abstract

The sulfated HNK-1 carbohydrate present on glycolipids and on several neural recognition molecules has been shown to mediate the adhesion of murine small cerebellar neurons and astrocytes to the extracellular matrix molecule laminin-1. In this study, we characterized the binding of the HNK-1 carbohydrate to laminin-1 extracted from the Engelbreth-Holm-Swarm (EHS) sarcoma and distinguished it unequivocally from binding sites for other sulfated carbohydrates. Electron microscopic analysis of rotary shadowed complexes of laminin-1 and a HNK-1 neoglycoprotein revealed a major binding site on the G domain that comprises the C-terminal globule of the laminin alpha1 chain. The HNK-1 carbohydrate also interacted with placental laminin isoforms containing an alpha chain variant. It bound to the proteolytic laminin-1 fragment E8 comprising the domains G1-G3, but not to fragment E3 that carries the major heparin-binding site on domains G4-G5. No binding was observed to the short arm containing fragments E1XNd or P1. Binding studies with native or denatured laminin E8 fragments and proteolytic or recombinant fragments of the G domain localized the HNK-1 carbohydrate binding site to domain G2. The binding could be clearly distinguished from binding sites for other sulfated carbohydrates such as heparin and sulfatides. Further, the binding could not be abolished by reduction and alkylation or by urea treatment of laminin-1 and was independent of the native conformation of laminin-1 and of Ca2+. The G2 domain is also involved in the adhesion of HNK-1 carbohydrate expressing early postnatal cerebellar neurons and is different from heparin- and sulfatide-mediated cell adhesion to laminin-1. HNK-1 carbohydrate-mediated cell adhesion appears, however, to be dependent on the native conformation of laminin-1 indicating a more complex cellular recognition process.

摘要

已证明存在于糖脂和几种神经识别分子上的硫酸化HNK-1碳水化合物可介导小鼠小脑小神经元和星形胶质细胞与细胞外基质分子层粘连蛋白-1的粘附。在本研究中,我们对HNK-1碳水化合物与从恩格尔布雷特-霍尔姆-斯旺(EHS)肉瘤中提取的层粘连蛋白-1的结合进行了表征,并明确将其与其他硫酸化碳水化合物的结合位点区分开来。对层粘连蛋白-1和HNK-1新糖蛋白的旋转阴影复合物进行电子显微镜分析,发现在G结构域上有一个主要结合位点,该结构域包含层粘连蛋白α1链的C末端小球。HNK-1碳水化合物还与含有α链变体的胎盘层粘连蛋白异构体相互作用。它与包含G1-G3结构域的蛋白水解层粘连蛋白-1片段E8结合,但不与在G4-G5结构域上携带主要肝素结合位点的片段E3结合。未观察到与包含片段E1XNd或P1的短臂结合。对天然或变性的层粘连蛋白E8片段以及G结构域的蛋白水解或重组片段的结合研究将HNK-1碳水化合物结合位点定位到G2结构域。该结合可与其他硫酸化碳水化合物如肝素和硫苷脂的结合位点明显区分开来。此外,层粘连蛋白-1经还原和烷基化处理或经尿素处理后,结合并未被消除,且与层粘连蛋白-1的天然构象和Ca2+无关。G2结构域也参与表达HNK-1碳水化合物的出生后早期小脑神经元的粘附,并且与肝素和硫苷脂介导的细胞与层粘连蛋白-1的粘附不同。然而,HNK-1碳水化合物介导的细胞粘附似乎依赖于层粘连蛋白-1的天然构象,这表明细胞识别过程更为复杂。

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