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Interchain and intrachain disulphide bonds in human platelet glycoprotein IIb. Localization of the epitopes for several monoclonal antibodies.

机译:人血小板糖蛋白IIb中的链间和链内二硫键。几种单克隆抗体的表位定位。

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摘要

The single interchain disulphide bond in platelet glycoprotein IIb (GPIIb) is accessible to extracellular reductants, and selective cleavage does not liberate GPIIb alpha from platelet plasma membrane, confirming that non-covalent interactions contribute to maintaining attachment of this subunit to the membrane. Eosin-maleimide labelling of isolated GPIIb after selective cleavage of this interchain disulphide bond, followed by full reduction and alkylation, CNBr cleavage, and analysis of the cleavage products allowed us to establish that this interchain disulphide bridge is formed between GPIIb beta (GPIIb beta-subunit) Cys-9 and GPIIb alpha Cys-826, and this conclusion was confirmed by independent routes. The other two cysteines of GPIIb beta (Cys-14 and Cys-19) form the single intrachain disulphide bond in this subunit. Last, the intrachain disulphides in GPIIb alpha (GPIIb alpha-subunit) are distributed in four main peptide domains which are not disulphide-bonded among themselves. The linear epitope for monoclonal antibody M1 is localized between Pro-4 and Met-24 (or Met-31) of GPIIb beta. The linear epitope for M3 is situated between Cys-826 and the C-terminus of GPIIb alpha. The M4 epitope is also linear and localized somewhere between residues 115 and 285 of GPIIb alpha. Finally, the epitopes for M5 and M6 are somewhere between Cys-608 and Met-704, within a 35 kDa membrane-bound chymotryptic product of digestion of GPIIb in whole platelets. The N-terminal amino acid sequences determined for eight different cleavage products of GPIIb alpha and GPIIb beta agree with the corresponding amino acid sequences predicted by cDNA sequence for human-erythroleukaemic-cell GPIIb [Poncz, Eisman, Heindenreich, Silver, Vilaire, Surrey, Schwartz & Bennett (1987) J. Biol. Chem. 262, 8476-8482].
机译:血小板糖蛋白IIb(GPIIb)中的单个链间二硫键易于细胞外还原剂进入,选择性切割不会从血小板质膜上释放GPIIbα,从而证实非共价相互作用有助于维持该亚基与膜的附着。选择性裂解该链间二硫键,然后进行完全还原和烷基化,CNBr裂解,并对裂解产物进行分析后,分离出的GPIIb进行了曙红-马来酰亚胺标记,这使我们能够确定在GPIIb beta(GPIIb beta-亚基)Cys-9和GPIIbαCys-826,这一结论得到了独立途径的证实。 GPIIb beta的其他两个半胱氨酸(Cys-14和Cys-19)在该亚基中形成单个链内二硫键。最后,GPIIb alpha中的链内二硫键(GPIIb alpha亚基)分布在四个主要的肽结构域之间,它们之间没有二硫键。单克隆抗体M1的线性表位位于GPIIb beta的Pro-4和Met-24(或Met-31)之间。 M3的线性表位位于Cys-826和GPIIbα的C端之间。 M4表位也是线性的并且位于GPIIbα的残基115和285之间的某处。最后,M5和M6的表位在Cys-608和Met-704之间,在整个血小板中消化GPIIb的35 kDa膜结合胰凝乳蛋白酶产物中。为GPIIb alpha和GPIIb beta的八个不同裂解产物确定的N端氨基酸序列与人红血球细胞GPIIb的cDNA序列预测的相应氨基酸序列一致[Poncz,Eisman,Heindenreich,Silver,Vilaire,Surrey, Schwartz&Bennett(1987)J.Biol。化学262,8476-8482]。

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