Proteolysis of IGFBPs by cathepsin D in vitro and in cathepsin D-deficient mice

Progress in growth factor research Pub Date : 1995-01-01 DOI:10.1016/0955-2235(95)00005-4

Thomas Braulke , Max Claussen , Paul Saftig , Martin Wendland , Klaus Neifer , Bernhard Schmidt , Jürgen Zapf , Kurt bon Figura , Christoph Peters

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引用次数: 29

Abstract

Affinity-purified lysosomal protease cathepsin D cleaved recombinant human IGFBP-1 to -5 in fragments of defined sizes, while IGFBP-6 was not degraded. To assess the role of cathepsin D for proteolytic processing of IGFBP in vivo, serum from cathepsin D-deficient mice and conditioned media from cathepsin D-deficient fibroblasts and organ explants were analyzed. No differences for the pattern and level of IGFBPs were detected. When conditioned media from fibroblasts were incubated at acid pH, proteolysis of IGFBP-1 and -4 was observed only in media derived from cathepsin D-expressing cells. Additional experiments showed that the proteolysis of IGFBP-4 is mediated by cathepsin D and not by a protease activated by cathepsin D. The IGFBP-4 degrading activities in media from organ explants from cathepsin D-deficient mice were found to be sensitive to inhibitors of aspartyl and cysteine proteases. The data indicate that different classes of acid pH-dependent proteases can contribute to the regulation of IGFBP-4 abundance.

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组织蛋白酶D在体外和组织蛋白酶D缺陷小鼠体内对igfbp的蛋白水解

亲和纯化的溶酶体蛋白酶组织蛋白酶D将重组人IGFBP-1切割成确定大小的片段，而IGFBP-6不被降解。为了评估组织蛋白酶D在体内IGFBP蛋白水解过程中的作用，我们分析了组织蛋白酶D缺陷小鼠的血清和组织蛋白酶D缺陷成纤维细胞和器官外植体的条件培养基。未发现igfbp的模式和水平有差异。当来自成纤维细胞的条件培养基在酸性pH下孵育时，仅在来自表达组织蛋白酶d的细胞的培养基中观察到IGFBP-1和-4的蛋白水解。进一步的实验表明，IGFBP-4的蛋白水解是由组织蛋白酶D介导的，而不是由组织蛋白酶D激活的蛋白酶介导的。从组织蛋白酶D缺乏的小鼠器官外植体中提取的培养基中发现，IGFBP-4的降解活性对天冬氨酸和半胱氨酸蛋白酶抑制剂敏感。这些数据表明，不同类型的酸性ph依赖性蛋白酶可以参与IGFBP-4丰度的调节。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Progress in growth factor research

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