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酵母作为用于胰岛素降解酶功能研究的易处理遗传系统。

Yeast as a tractable genetic system for functional studies of the insulin-degrading enzyme.

作者信息

Kim Seonil, Lapham Andrea N, Freedman Christopher G K, Reed Tiffany L, Schmidt Walter K

机构信息

Department of Cellular Biology, University of Georgia, Athens, Georgia 30602, USA.

出版信息

J Biol Chem. 2005 Jul 29;280(30):27481-90. doi: 10.1074/jbc.M414192200. Epub 2005 Jun 8.

DOI:10.1074/jbc.M414192200
PMID:15944156
Abstract

We have developed yeast as an expression and genetic system for functional studies of the insulin-degrading enzyme (IDE), which cleaves and inactivates certain small peptide molecules, including insulin and the neurotoxic A beta peptide. We show that heterologously expressed rat IDE is enzymatically active, as judged by the ability of IDE-containing yeast extracts to cleave insulin in vitro. We also show that IDE can promote the in vivo production of the yeast a-factor mating pheromone, a function normally attributed to the yeast enzymes Axl1p and Ste23p. However, IDE cannot substitute for the function of Axl1p in promoting haploid axial budding and repressing haploid invasive growth, activities that require an uncharacterized activity of Axl1p. Particulate fractions enriched for Axl1p or Ste23p are incapable of cleaving insulin, suggesting that the functional conservation of these enzymes may not be bidirectionally conserved. We have made practical use of our genetic system to confirm that residues composing the extended zinc metalloprotease motif of M16A family enzymes are required for the enzymatic activity of IDE, Ste23p, and Axl1p. We have determined that IDE and Axl1p both require an intact C terminus for optimal activity. We expect that the tractable genetic system that we have developed will be useful for investigating the enzymatic and structure/function properties of IDE and possibly for the identification of novel IDE alleles having altered substrate specificity.

摘要

我们已将酵母开发为一种用于胰岛素降解酶(IDE)功能研究的表达和遗传系统,该酶可切割并使某些小肽分子失活,包括胰岛素和神经毒性Aβ肽。我们发现,通过含IDE的酵母提取物在体外切割胰岛素的能力判断,异源表达的大鼠IDE具有酶活性。我们还发现,IDE可促进酵母a因子交配信息素的体内产生,这一功能通常归因于酵母酶Axl1p和Ste23p。然而,在促进单倍体轴向出芽和抑制单倍体侵袭性生长方面,IDE无法替代Axl1p的功能,而这些活动需要Axl1p的一种未知活性。富含Axl1p或Ste23p的颗粒级分无法切割胰岛素,这表明这些酶的功能保守性可能并非双向保守。我们已实际应用我们的遗传系统来确认,构成M16A家族酶扩展锌金属蛋白酶基序的残基是IDE、Ste23p和Axl1p酶活性所必需的。我们已确定,IDE和Axl1p都需要完整的C末端以实现最佳活性。我们预计,我们开发的易于处理的遗传系统将有助于研究IDE的酶学和结构/功能特性,并可能有助于鉴定具有改变的底物特异性的新型IDE等位基因。

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