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The pCri system: A vector collection for recombinant protein expression and purification

机译:pCri系统:用于重组蛋白表达和纯化的载体集合

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摘要

A major bottleneck in structural, biochemical and biophysical studies of proteins is the need for large amounts of pure homogenous material, which is generally obtained by recombinant overexpression. Here we introduce a vector collection, the pCri System, for cytoplasmic and periplasmic/extracellular expression of heterologous proteins that allows the simultaneous assessment of prokaryotic and eukaryotic host cells (Escherichia coli, Bacillus subtilis, and Pichia pastoris). By using a single polymerase chain reaction product, genes of interest can be directionally cloned in all vectors within four different rare restriction sites at the 5′end and multiple cloning sites at the 3′end. In this way, a number of different fusion tags but also signal peptides can be incorporated at the N-and C-terminus of proteins, facilitating their expression, solubility and subsequent detection and purification. Fusion tags can be efficiently removed by treatment with site-specific peptidases, such as tobacco etch virus proteinase, thrombin, or sentrin specific peptidase 1, which leave only a few extra residues at the N-terminus of the protein. The combination of different expression systems in concert with the cloning approach in vectors that can fuse various tags makes the pCri System a valuable tool for high throughput studies.
机译:蛋白质的结构,生化和生物物理研究的主要瓶颈是需要大量纯净的均质材料,通常通过重组过表达获得这些纯净的均质材料。在这里,我们介绍了用于异源蛋白的胞质和周质/胞外表达的载体pCri系统,该载体可以同时评估原核和真核宿主细胞(大肠杆菌,枯草芽孢杆菌和巴斯德毕赤酵母)。通过使用单个聚合酶链反应产物,可以将感兴趣的基因定向克隆到5'端四个不同的罕见限制性酶切位点和3'端多个克隆位点的所有载体中。以这种方式,可以在蛋白质的N-和C-末端掺入许多不同的融合标签以及信号肽,以促进它们的表达,溶解性以及随后的检测和纯化。融合标签可以通过用位点特异性肽酶(例如烟草蚀刻病毒蛋白酶,凝血酶或哨蛋白特异性肽酶1)进行处理而有效去除,这些酶在该蛋白的N末端仅留下一些额外的残基。不同表达系统的结合以及可融合各种标签的载体克隆方法使pCri系统成为进行高通量研究的有价值的工具。

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