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利用Bmp1/Tll1双纯合缺失小鼠和蛋白质组学来鉴定和验证骨形态发生蛋白1/类原肠胚样金属蛋白酶的体内底物。

Use of Bmp1/Tll1 doubly homozygous null mice and proteomics to identify and validate in vivo substrates of bone morphogenetic protein 1/tolloid-like metalloproteinases.

作者信息

Pappano William N, Steiglitz Barry M, Scott Ian C, Keene Douglas R, Greenspan Daniel S

机构信息

Department of Biomolecular Chemistry, University of Wisconsin, Madison, Wisconsin 53706, USA.

出版信息

Mol Cell Biol. 2003 Jul;23(13):4428-38. doi: 10.1128/MCB.23.13.4428-4438.2003.

DOI:10.1128/MCB.23.13.4428-4438.2003
PMID:12808086
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC164836/
Abstract

Bone morphogenetic protein 1 (BMP-1) and mammalian Tolloid (mTLD), two proteinases encoded by Bmp1, provide procollagen C-proteinase (pCP) activity that converts procollagens I to III into the major fibrous components of mammalian extracellular matrix (ECM). Yet, although Bmp1(-/-) mice have aberrant collagen fibrils, they have residual pCP activity, indicative of genetic redundancy. Mammals possess two additional proteinases structurally similar to BMP-1 and mTLD: the genetically distinct mammalian Tolloid-like 1 (mTLL-1) and mTLL-2. Mice lacking the mTLL-1 gene Tll1 are embryonic lethal but have pCP activity levels similar to those of the wild type, suggesting that mTLL-1 might not be an in vivo pCP. In vitro studies have shown BMP-1 and mTLL-1 capable of cleaving Chordin, an extracellular antagonist of BMP signaling, suggesting that these proteases might also serve to modulate BMP signaling and to coordinate the latter with ECM formation. However, in vivo evidence of roles for BMP-1 and mTLL-1 in BMP signaling in mammals is lacking. To remove functional redundancy obscuring the in vivo functions of BMP-1-related proteases in mammals, we here characterize Bmp1 Tll1 doubly null mouse embryos. Although these appear morphologically indistinguishable from Tll1(-/-) embryos, biochemical analysis of cells derived from doubly null embryos shows functional redundancy removed to an extent enabling us to demonstrate that (i) products of Bmp1 and Tll1 are responsible for in vivo cleavage of Chordin in mammals and (ii) mTLL-1 is an in vivo pCP that provides residual activity observed in Bmp1(-/-) embryos. Removal of functional redundancy also enabled use of Bmp1(-/-) Tll1(-/-) cells in a proteomics approach for identifying novel substrates of Bmp1 and Tll1 products.

摘要

骨形态发生蛋白1(BMP-1)和哺乳动物类 tolloid蛋白(mTLD)是由Bmp1编码的两种蛋白酶,它们具有前胶原C蛋白酶(pCP)活性,可将I至III型前胶原转化为哺乳动物细胞外基质(ECM)的主要纤维成分。然而,尽管Bmp1基因敲除小鼠具有异常的胶原纤维,但它们仍具有残余的pCP活性,这表明存在基因冗余。哺乳动物还拥有另外两种在结构上与BMP-1和mTLD相似的蛋白酶:基因上不同的哺乳动物类 tolloid样蛋白1(mTLL-1)和mTLL-2。缺乏mTLL-1基因Tll1的小鼠胚胎致死,但pCP活性水平与野生型相似,这表明mTLL-1可能不是体内的pCP。体外研究表明,BMP-1和mTLL-1能够切割Chordin,后者是BMP信号传导的细胞外拮抗剂,这表明这些蛋白酶也可能用于调节BMP信号传导,并使其与ECM形成相协调。然而,缺乏BMP-1和mTLL-1在哺乳动物BMP信号传导中作用的体内证据。为了消除掩盖BMP-1相关蛋白酶在哺乳动物体内功能的功能冗余,我们在此对Bmp1 Tll1双基因敲除小鼠胚胎进行了表征。尽管这些胚胎在形态上与Tll1基因敲除胚胎无法区分,但对双基因敲除胚胎来源的细胞进行生化分析表明,功能冗余已在一定程度上消除,这使我们能够证明:(i)Bmp1和Tll1的产物负责哺乳动物体内Chordin的切割;(ii)mTLL-1是一种体内pCP,它提供了在Bmp1基因敲除胚胎中观察到的残余活性。功能冗余的消除还使得能够在蛋白质组学方法中使用Bmp1基因敲除Tll1基因敲除细胞来鉴定Bmp1和Tll1产物的新底物。

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