首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Cathepsin D-mediated processing of procollagen: lysosomal enzyme involvement in secretory processing of procollagen.
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Cathepsin D-mediated processing of procollagen: lysosomal enzyme involvement in secretory processing of procollagen.

机译:组织蛋白酶D介导的原胶原加工:溶酶体酶参与原胶原的分泌加工。

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摘要

The proteolytic removal of the extension COOH-terminal propeptide from procollagen has been examined in vitro. A crude enzyme activity was identified in a whole-chicken-embryo extract that acted at acid pH and appeared to be similar to one identified previously [Davidson, J. M., McEneany , L. S. G. & Bornstein , P. (1979) Eur. J. Biochem. 100, 551-558]. This activity was inhibitable by pepstatin but not by leupeptin, suggesting that it might be cathepsin D. Cathepsin D was purified 907-fold from chicken livers by affinity chromatography on pepstatin-aminohexyl-Sepharose 4B and was found to remove the COOH propeptides from procollagen. At pH 6.0, the site of cleavage appeared to shift from the COOH telopeptide to the COOH telopeptide/propeptide junction, based upon the difference in electrophoretic migration of the cleavage products, although determining the actual cleavage site will require end-group analysis. A model for the involvement of cathepsin D in the in vivo processing of procollagen is presented.
机译:体外检查了从原胶原蛋白水解去除延伸的COOH-末端前肽的过程。在全鸡胚提取物中鉴定出粗酶活性,该全鸡胚提取物在酸性pH下起作用,并且似乎与先前鉴定的酶活性相似[Davidson,J.M.,McEneany,L.S.G。&Bornstein,P。(1979)Eur.J.Med.Chem.Soc。,1992,5,1897]。 J.生物化学。 100,551-558]。胃蛋白酶抑制剂可抑制此活性,而亮肽酶则不能抑制该活性,表明它可能是组织蛋白酶D。通过在胃蛋白酶抑制素-氨基己基-琼脂糖4B上进行亲和层析,从鸡肝中纯化组织蛋白酶D 907倍,发现可从原胶原中去除COOH前肽。在pH 6.0时,基于裂解产物电泳迁移的差异,裂解位点似乎从COOH端肽转移到COOH端肽/前肽接头,尽管确定实际的裂解位点需要进行端基分析。提出了组织蛋白酶D参与胶原蛋白的体内加工的模型。

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