Francis G, Butler W T, Finch J E
Biochem J. 1978 Dec 1;175(3):921-30. doi: 10.1042/bj1750921.
The covalent structure of the first 111 residues from the N-terminus of peptide alpha1(II)-CB10 from bovine nasal-cartilage collagen is presented. This region comprises residues 552-661 of the alpha1(II) chain. The sequence was determined by automated Edman degradation of peptide alpha1(II)-CB10 and of peptides produced by cleavage with trypsin and hydroxylamine. Comparison of this region of the alpha1(II) chain with the homologous segment of the alpha1(I) chain indicated a homology level of 85%, slightly higher than that of 81% reported for the N-terminal region of the alpha1(II) chain (Butler, Miller & Finch (1976) Biochemistry15, 3000-3006). The occurrence of two residues of glycosylated hydroxylysine was established at positions 564 and 603, the first present exclusively as galactosylhydroxylysine and the latter as a mixture of galactosylhydroxylysine and glucosylgalactosylhydroxylysine. Also, two residues at positions 648 and 657 were tentatively identified as glycosylated hydroxylysines. The amino acid sequences adjacent to the hydroxylysine residues so far identified in the alpha1(II) chain were compared with the homologous regions of the alpha1(I) and alpha2 chains, but no obvious prerequisite for hydroxylation could be seen. From comparison with the homologous sequence of the alpha1(I) chain, it appears that the alpha1(II)-chain sequence presented here contains three more amino acids than that reported for the alpha1(I) chain. This triplet would be interposed between residues 63 and 64 of the reported sequence of peptide alpha1(I)-CB7 from calf skin collagen. Data on the purification of the subpeptides and their amino acid compositions have been deposited as Supplementary Publication SUP 50087 (7 pages) at the British Library Lending Division, Boston Spa, Wetherby, West Yorkshire LS23 7BQ, U.K., from whom copies can be obtained on the terms indicated in Biochem. J. (1978) 169, 5.
本文介绍了来自牛鼻软骨胶原蛋白的肽α1(II)-CB10 N端前111个残基的共价结构。该区域包含α1(II)链的552 - 661位残基。通过对肽α1(II)-CB10以及用胰蛋白酶和羟胺裂解产生的肽进行自动Edman降解来确定序列。将α1(II)链的该区域与α1(I)链的同源片段进行比较,同源性水平为85%,略高于报道的α1(II)链N端区域的81%(巴特勒、米勒和芬奇(1976年),《生物化学》15,3000 - 3006)。已确定在564位和603位存在两个糖基化羟赖氨酸残基,第一个仅以半乳糖基羟赖氨酸形式存在,后者为半乳糖基羟赖氨酸和葡萄糖基半乳糖基羟赖氨酸的混合物。此外,在648位和657位的两个残基初步鉴定为糖基化羟赖氨酸。将α1(II)链中迄今已鉴定的与羟赖氨酸残基相邻的氨基酸序列与α1(I)和α2链的同源区域进行比较,但未发现明显的羟化先决条件。通过与α1(I)链的同源序列比较,此处呈现的α1(II)链序列似乎比报道的α1(I)链序列多三个氨基酸。这个三联体将插入到来自小牛皮肤胶原蛋白的肽α1(I)-CB7报道序列的63位和64位残基之间。关于亚肽纯化及其氨基酸组成的数据已作为补充出版物SUP 50087(7页)存放在英国西约克郡韦瑟比波士顿温泉市英国国家图书馆出借部,邮编LS23 7BQ,可按《生物化学杂志》(1978年)169,5中所示条件从该处获取副本。