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生长分化因子8前肽抑制结构域的表征与鉴定

Characterization and identification of the inhibitory domain of GDF-8 propeptide.

作者信息

Jiang Man-Shiow, Liang Li-fang, Wang Shusheng, Ratovitski Tamara, Holmstrom James, Barker Christopher, Stotish Ronald

机构信息

MetaMorphix, Inc., Savage, MD 20763, USA.

出版信息

Biochem Biophys Res Commun. 2004 Mar 12;315(3):525-31. doi: 10.1016/j.bbrc.2004.01.085.

DOI:10.1016/j.bbrc.2004.01.085
PMID:14975732
Abstract

GDF-8 is a negative regulator of skeletal muscle mass. The mechanisms which regulate the biological activity of GDF-8 have not yet been elucidated. Analogous to the TGF-beta system, GDF-8 propeptide binds to and inhibits the activity of GDF-8. In these studies, we define the critical domain of the GDF-8 propeptide necessary for inhibitory activity. Two molecules of GDF-8 propeptide monomer inhibit the biological activity of one molecule of GDF-8 homodimer. Although the propeptide contains N-linked glycosylation when synthesized in mammalian cells, this glycosylation is not necessary for the inhibition of GDF-8. Taking advantage of the bacterial expression system, we express and purify GDF-8 propeptide which retains full inhibitory activity. To define the functional regions of the propeptide, we express a series of truncated GST-propeptide fusion proteins and examined their inhibitory activity. We observe that fusion proteins containing the C-terminal region (amino acid residues 99-266) are very stable, but do not exhibit inhibitory activity; while fusion proteins containing the N-terminal region (amino acid residues 42-115) are labile but contain essential inhibitory activity. The data suggest that the C-terminal region may play a role in the stability of the GDF-8 propeptide and that the inhibitory domain is located in the region between amino acids 42 and 115.

摘要

生长分化因子8(GDF - 8)是骨骼肌质量的负调节因子。调节GDF - 8生物活性的机制尚未阐明。与转化生长因子β(TGF - β)系统类似,GDF - 8前肽可结合并抑制GDF - 8的活性。在这些研究中,我们确定了GDF - 8前肽抑制活性所必需的关键结构域。两分子GDF - 8前肽单体可抑制一分子GDF - 8同二聚体的生物活性。尽管前肽在哺乳动物细胞中合成时含有N - 连接糖基化,但这种糖基化对于抑制GDF - 8并非必需。利用细菌表达系统,我们表达并纯化了具有完全抑制活性的GDF - 8前肽。为了确定前肽的功能区域,我们表达了一系列截短的谷胱甘肽S - 转移酶(GST)-前肽融合蛋白,并检测了它们的抑制活性。我们观察到,包含C末端区域(氨基酸残基99 - 266)的融合蛋白非常稳定,但不表现出抑制活性;而包含N末端区域(氨基酸残基42 - 115)的融合蛋白不稳定,但具有基本的抑制活性。数据表明,C末端区域可能在GDF - 8前肽的稳定性中起作用,并且抑制结构域位于氨基酸42和115之间的区域。

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