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开发一种基于Gateway的新型载体系统,用于在大肠杆菌中进行高效、多平行蛋白表达。

Development of a novel Gateway-based vector system for efficient, multiparallel protein expression in Escherichia coli.

作者信息

Freuler Felix, Stettler Thomas, Meyerhofer Marco, Leder Lukas, Mayr Lorenz M

机构信息

Novartis Institutes for BioMedical Research (NIBR), Center for Proteomic Chemistry (CPC), Forum 1, Novartis Campus, CH-4056 Basel, Switzerland.

出版信息

Protein Expr Purif. 2008 Jun;59(2):232-41. doi: 10.1016/j.pep.2008.02.003. Epub 2008 Feb 21.

Abstract

We describe a cloning and expression system which is based on the Escherichia coli T7 expression system and Gateway recombination technology. We have produced numerous destination vectors with selected fusion tags and an additional set of entry vectors containing the gene of interest and optional labeling tags. This powerful system enables us to transfer a cDNA to several expression vectors in parallel and combine them with various labeling tags. To remove the attached amino terminal tags along with the unwanted attB1 site, we inserted PreScission protease cleavage sites. In contrast to the commercially available destination vectors, our plasmids provide kanamycin resistance, which can be an advantage when expressing toxic proteins in E. coli. Some small-scale protein expression experiments are shown to demonstrate the usefulness of these novel Gateway vectors. In summary, this system has some benefits over the widely used and commercially available Gateway standard system, and it enables many different combinations for expression constructs from a single gene of interest.

摘要

我们描述了一种基于大肠杆菌T7表达系统和Gateway重组技术的克隆与表达系统。我们已经构建了许多带有选定融合标签的目的载体,以及另一组包含感兴趣基因和可选标记标签的入门载体。这个强大的系统使我们能够将一个cDNA并行转移到多个表达载体中,并将它们与各种标记标签相结合。为了去除附着的氨基末端标签以及不需要的attB1位点,我们插入了PreScission蛋白酶切割位点。与市售的目的载体不同,我们的质粒提供卡那霉素抗性,这在大肠杆菌中表达毒性蛋白时可能是一个优势。展示了一些小规模蛋白质表达实验,以证明这些新型Gateway载体的实用性。总之,该系统比广泛使用的市售Gateway标准系统具有一些优势,并且它能够从单个感兴趣基因实现表达构建体的许多不同组合。

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