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迈向真核生物结构复杂组学

Towards eukaryotic structural complexomics.

作者信息

Bieniossek Christoph, Berger Imre

机构信息

Institute for Molecular Biology and Biophysics, ETH Hönggerberg, 8093, Zurich, Switzerland.

出版信息

J Struct Funct Genomics. 2009 Mar;10(1):37-46. doi: 10.1007/s10969-008-9047-6. Epub 2008 Nov 14.

Abstract

Many eukaryotic proteins exist in large multisubunit assemblies and often show compromised folding or activity when their interaction partners are not present. Protein complexes in eukaryotes can contain ten or more subunits with individual polypeptides ranging in size up to several hundred kilodalton, severely restricting the application of conventional cloning strategies and imposing constraints on the choice of the expression host. Modern structural molecular biology often depends on introducing diversity into the specimens under investigation, including mutation, truncation and placement of purification aids. Current recombinant expression methods often require a disproportionate labor investment prior to multiprotein expression, and subsequent to expression and analysis do not provide for rapid revision of the experiment. We have developed reagents and protocols for rapid and flexible multiprotein complex expressions suitable for structural biology, focusing on multigene baculoviral vectors and their recombination mediated assembly. A top priority in protein science is automation. Our strategy can be readily adapted in a robotics setup, for baculovirus/insect cell expression of protein complexes, but likewise also for mammalian or prokaryotic hosts.

摘要

许多真核生物蛋白质以大型多亚基组装体的形式存在,并且当它们的相互作用伙伴不存在时,常常表现出折叠或活性受损。真核生物中的蛋白质复合物可以包含十个或更多个亚基,单个多肽的大小可达数百千道尔顿,这严重限制了传统克隆策略的应用,并对表达宿主的选择施加了限制。现代结构分子生物学通常依赖于在被研究的样本中引入多样性,包括突变、截短和纯化辅助物的放置。目前的重组表达方法在多蛋白表达之前通常需要投入不成比例的劳动力,并且在表达和分析之后不能快速修改实验。我们已经开发了适用于结构生物学的快速灵活的多蛋白复合物表达的试剂和方案,重点是多基因杆状病毒载体及其重组介导的组装。蛋白质科学的一个首要任务是自动化。我们的策略可以很容易地应用于机器人装置中,用于杆状病毒/昆虫细胞表达蛋白质复合物,但同样也适用于哺乳动物或原核宿主。

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