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首页> 外文期刊>Journal of Structural Biology >Transient transfection coupled to baculovirus infection for rapid protein expression screening in insect cells.
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Transient transfection coupled to baculovirus infection for rapid protein expression screening in insect cells.

机译:瞬时转染结合杆状病毒感染,可快速筛查昆虫细胞中的蛋白质表达。

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Baculovirus infected insect cells are widely used for heterologous protein expression. Despite the power of this system, the use of baculovirus techniques for protein expression screening is hampered by the time and resources needed to generate each recombinant baculovirus. Here, we show that a transfection/infection based expression system is suitable for screening of expression constructs in insect cells and represents a valid alternative to other traditional screening methodologies using recombinant baculovirus. The described method is based on gene delivery by transfection coupled to the induction of protein expression by non-recombinant baculovirus infection. Vectors that control expression by a combination of the baculovirus promoters ie1 and p10 and the enhancer element hr5 are among the ones suitable for this method. Infection with non-recombinant baculovirus drastically increases the basal activity of these elements, leading to protein over-expression. Multiple vectors can be simultaneously co-transfected/infected, making transfection/infection amenable for screening of multiple co-expressed proteins and protein complexes. Taken together, our results prove that the transfection/infection protocol is a valid and innovative approach for increasing speed and reducing costs of protein expression screening for structural and functional studies.
机译:杆状病毒感染的昆虫细胞被广泛用于异源蛋白表达。尽管此系统功能强大,但杆状病毒技术用于蛋白质表达筛选的过程仍然受制于生成每种重组杆状病毒所需的时间和资源。在这里,我们表明基于转染/感染的表达系统适用于筛选昆虫细胞中的表达构建体,并且代表了使用重组杆状病毒替代其他传统筛选方法的有效选择。所描述的方法基于通过转染进行的基因递送与通过非重组杆状病毒感染诱导的蛋白表达相结合。通过杆状病毒启动子 ie1 和 p10 和增强子元素 hr5 的组合来控制表达的载体是适用于该方法的载体。用非重组杆状病毒感染会大大增加这些元素的基础活性,从而导致蛋白质过表达。可以同时共转染/感染多个载体,使转染/感染适合筛选多种共表达的蛋白质和蛋白质复合物。综上所述,我们的结果证明,转染/感染方案是一种有效的创新方法,可提高速度并降低用于结构和功能研究的蛋白质表达筛选的成本。

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