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A versatile bacterial expression vector designed for single-step cloning of multiple DNA fragments using homologous recombination

机译:一种通用的细菌表达载体,设计用于通过同源重组一步克隆多个DNA片段

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摘要

Production of recombinant proteins is the starting point for biochemical and biophysical analyses and requires methodology to efficiently proceed from gene sequence to purified protein. While optimized strategies for the efficient cloning of single-gene fragments for bacterial expression is available, efficient multiple DNA fragment cloning still presents a challenge. To facilitate this step, we have developed an efficient cloning strategy based on yeast homologous recombination cloning (YHRC) into the new pETbased bacterial expression vector pSUMO-YHRC. The vector supports cloning for untagged expression as well as fusions to His_6-SUMO or His_6 tags. We demonstrate that YHRC from single PCR products of 6 independent genes into the vector results in virtually no background. Importantly, in a quantitative assay for functional expression we find that single-step YHRC of 7 DNA fragments can be performed with very high cloning efficiencies. The method and reagents described in this paper significantly simplifies the construction of expression plasmids from multiple DNA fragments, including complex gene fusions, chimeric genes and polycistronic constructs.
机译:重组蛋白的生产是生物化学和生物物理分析的起点,并且需要有效地从基因序列发展到纯化蛋白的方法。尽管有用于细菌表达的单基因片段有效克隆的优化策略,但有效的多DNA片段克隆仍然是一个挑战。为了促进此步骤,我们已经基于酵母同源重组克隆(YHRC)开发了一种有效的克隆策略,将其克隆到新的基于pET的细菌表达载体pSUMO-YHRC中。该载体支持无标记表达的克隆以及与His_6-SUMO或His_6标签的融合。我们证明YHRC从6个独立基因的单个PCR产物进入载体的结果几乎没有背景。重要的是,在功能性表达的定量分析中,我们发现可以以很高的克隆效率进行7个DNA片段的单步YHRC。本文中描述的方法和试剂可从多个DNA片段(包括复杂的基因融合体,嵌合基因和多顺反子构建体)中大大简化表达质粒的构建。

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