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Purification of human procollagen type III N-proteinase from placenta and preparation of antiserum.

机译:从胎盘中纯化人类III型前胶原N型蛋白酶并制备抗血清。

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摘要

Procollagen type III N-proteinase, of Mr about 70,000, was detected in human placental tissue and purified from this source more than 5800-fold. It was found to be a glycoprotein, which was bound to both concanavalin A-Ultrogel and heparin-Sepharose affinity columns. Binding to a type III pN-collagen-Sepharose affinity column was used as the final step in purification. The purified enzyme accepted only native type III procollagen or [14C]carboxymethylated type III pN-collagen as its substrate; type I, type II and type IV procollagen and heat-denatured type III pN-collagen were not cleaved by the enzyme. Antibodies against this purified enzyme protein raised in rabbits demonstrated a high inhibitory effect on the enzyme activity. Immunoblotting of the denatured protein and immunoelectrophoresis of the native enzyme showed only one major antigenic component, again with an Mr of about 70,000. The antibodies cross-reacted with the enzyme preparation from foetal-calf aorta smooth-muscle cells.
机译:在人类胎盘组织中检出了大约70,000先生的III型前胶原N蛋白酶,并从该来源纯化了5800倍以上。发现它是一种糖蛋白,与伴刀豆球蛋白A-Ultrogel和肝素-Sepharose亲和柱结合。与III型pN-胶原-Sepharose亲和柱的结合用作纯化的最后一步。纯化的酶仅接受天然III型胶原蛋白或[14C]羧甲基化III型pN胶原蛋白作为底物;该酶不会裂解I型,II型和IV型胶原蛋白,以及热变性的III型pN胶原蛋白。在兔体内产生的针对这种纯化酶蛋白的抗体表现出对酶活性的高度抑制作用。变性蛋白的免疫印迹和天然酶的免疫电泳显示仅一种主要抗原成分,同样具有约70,000的Mr。抗体与来自小腿小动脉主动脉平滑肌细胞的酶制剂发生交叉反应。

著录项

  • 作者

    Halila, R; Peltonen, L;

  • 作者单位
  • 年度 1986
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  • 原文格式 PDF
  • 正文语种 en
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