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酿酒酵母减数分裂特异性蛋白激酶Ime2的纯化及某些特性

Purification and some properties of Saccharomyces cerevisiae meiosis-specific protein kinase Ime2.

作者信息

Hui Catherine M, Campistrous Ana, Stuart David T

机构信息

Department of Biochemistry, University of Alberta, 561 Medical Sciences Building, Edmonton, Alta., Canada T6G 2H7.

出版信息

Protein Expr Purif. 2002 Dec;26(3):416-24. doi: 10.1016/s1046-5928(02)00548-x.

Abstract

Ime2 is the founding member of a family of protein kinases that are required for effective progression through meiotic development. Ime2 is essential for the induction of meiosis-specific genes and for the activation of meiotic DNA replication in the budding yeast Saccharomyces cerevisiae. Aside from the fact that Ime2 is a protein kinase and shares several amino acid motifs with cyclin dependent kinases, virtually nothing is known about its enzymatic properties or substrates. Biochemical characterization of Ime2 has been hindered by its low abundance and short half-life. We have created baculovirus expression vectors to produce recombinant Ime2 in insect cells. In this report, we describe the overproduction of Ime2 and its purification using affinity chromatography. Using this procedure, we have been able to purify up to 2mg Ime2 from 1L of infected insect cells. The Ime2 isolated by this method displays properties similar to those of the native enzyme that has been immunoprecipitated from yeast. The high level expression of Ime2 in this system and its ease of purification will be beneficial for more extensive biochemical analysis of Ime2 and related meiosis-specific kinases.

摘要

Ime2是一类蛋白激酶家族的创始成员,该家族对于减数分裂发育的有效进程是必需的。Ime2对于酿酒酵母中减数分裂特异性基因的诱导以及减数分裂DNA复制的激活至关重要。除了Ime2是一种蛋白激酶且与细胞周期蛋白依赖性激酶共享几个氨基酸基序这一事实外,关于其酶促特性或底物几乎一无所知。Ime2的生化特性研究因它的低丰度和短半衰期而受阻。我们构建了杆状病毒表达载体,以便在昆虫细胞中产生重组Ime2。在本报告中,我们描述了Ime2的过量表达及其通过亲和层析进行的纯化。使用该方法,我们能够从1升受感染的昆虫细胞中纯化出多达2毫克的Ime2。通过这种方法分离的Ime2表现出与从酵母中免疫沉淀出的天然酶相似的特性。Ime2在该系统中的高水平表达及其易于纯化将有利于对Ime2和相关减数分裂特异性激酶进行更广泛的生化分析。

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