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昆虫直接系统:从昆虫细胞中快速、高效地进行蛋白质表达和纯化。

InsectDirect System: rapid, high-level protein expression and purification from insect cells.

作者信息

Loomis Kathryn H, Yaeger Keith W, Batenjany Michael M, Mehler Mark M, Grabski Anthony C, Wong Shou C, Novy Robert E

机构信息

EMD Biosciences, Inc., 441 Charmany Dr., Madison, WI 53719, USA.

出版信息

J Struct Funct Genomics. 2005;6(2-3):189-94. doi: 10.1007/s10969-005-5241-y.

Abstract

A fundamental challenge in high-throughput (HT) expression screening is to rapidly identify the appropriate expression system for many targets in parallel. Known or unknown open reading frames (ORFs) are typically amplified by PCR and then cloned into a variety of vectors, producing recombinants used to direct target protein expression in Escherichia coli, insect cells, mammalian cells, or yeast. To facilitate rapid expression and purification in Spodoptera insect cells (Sf9), we developed transient expression vectors that include an enterokinase cleavage site immediately upstream of a ligation-independent cloning site (Ek/LIC). We also developed a high-efficiency insect cell transfection reagent, and automation-compatible fusion protein purification system for insect cells to facilitate expression screening and protein production. Positive clones identified from the small-scale screening were subjected to a larger scale production. Using this InsectDirect approach, we successfully expressed milligram quantities of different human proteins including heat shock proteins, phospholipases, and protein kinases.

摘要

高通量(HT)表达筛选中的一个基本挑战是要快速并行地为多个靶标确定合适的表达系统。已知或未知的开放阅读框(ORF)通常通过PCR进行扩增,然后克隆到各种载体中,产生用于在大肠杆菌、昆虫细胞、哺乳动物细胞或酵母中指导靶蛋白表达的重组体。为便于在草地贪夜蛾昆虫细胞(Sf9)中进行快速表达和纯化,我们开发了瞬时表达载体,其在不依赖连接的克隆位点(Ek/LIC)的紧邻上游包含一个肠激酶切割位点。我们还开发了一种高效的昆虫细胞转染试剂,以及用于昆虫细胞的与自动化兼容的融合蛋白纯化系统,以促进表达筛选和蛋白生产。从小规模筛选中鉴定出的阳性克隆进行更大规模的生产。使用这种InsectDirect方法,我们成功表达了毫克量的不同人类蛋白,包括热休克蛋白、磷脂酶和蛋白激酶。

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