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Failure of highly purified lysyl hydroxylase to hydroxylate lysyl residues in the non-helical regions of collagen

机译:高纯度赖氨酰羟化酶不能使胶原蛋白非螺旋区中的赖氨酰残基羟化

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pThe activity of highly purified lysyl hydroxylase towards lysyl residues within both the helical and the N-terminal non-helical telopeptide regions of chick type I collagen has been examined. The peptides alpha 1(I)-CB1 and alpha 2(I)-CB1, isolated from protocollagen following CNBr digestion and containing the N-terminal telopeptidyl lysyl residues, failed themselves to act as substrates. With protocollagen as substrate, analysis of products obtained following bacterial collagenase digestion of the reaction mixture showed that overall 37% hydroxylation of lysyl residues within the helical region of collagen had been obtained, which may be maximal. No hydroxylation, however, of the single lysyl residue in either alpha 1(I)-CB1 or alpha 2(I)-CB1, isolated following CNBr digestion of the reaction mixture, was observed, despite the known susceptibility of these residues to hydroxylation. These findings provide strong circumstantial evidence for the suggestion that a lysyl hydroxylase specific for the telopeptidyl residues and distinct from that active towards lysyl residues in the helical portion of the molecule may exist [Barnes, Constable, Morton & Royce (1974) Biochem. J. 139, 461-468]./p
机译:已经检查了高纯度的赖氨酰羟化酶对雏鸡I型胶原的螺旋和N末端非螺旋端肽区域内的赖氨酰残基的活性。从CNBr消化后从协议中分离并包含N末端端肽基赖氨酰残基的肽alpha 1(I)-CB1和alpha 2(I)-CB1本身无法充当底物。使用协议酶作为底物,对细菌胶原酶消化反应混合物后获得的产物进行分析表明,已获得胶原螺旋区域内赖氨酰残基的总体37%羟基化,这可能是最大的。然而,尽管CNBR消化了反应混合物后,α1(I)-CB1或α2(I)-CB1中的单个赖氨酰基残基均未发现羟基化,尽管这些残基对羟基化的敏感性很高。这些发现提供了强有力的环境证据,表明可能存在特异于端肽基残基且与分子的螺旋部分中的对赖氨酰基残基有活性的赖氨酰羟化酶[Barnes,Constable,Morton& Chem。,2003,6,5,5]。 Royce(1974)生物化学。 J. 139,461-468]。

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