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Random multi-recombinant PCR for the construction of combinatorial protein libraries

机译:随机多重组PCR构建组合蛋白文库

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摘要

Development of a new methodology to create protein libraries, which enable the exploration of global protein space, is an exciting challenge. In this study we have developed random multi-recombinant PCR (RM-PCR), which permits the shuffling of several DNA fragments without homologous sequences. In order to evaluate this methodology, we applied it to create two different combinatorial DNA libraries. For the construction of a ‘random shuffling library’, RM-PCR was used to shuffle six DNA fragments each encoding 25 amino acids; this affords many different fragment sequences whose every position has an equal probability to encode any of the six blocks. For the construction of the ‘alternative splicing library’, RM-PCR was used to perform different alternative splicings at the DNA level, which also yields different block sequences. DNA sequencing of the RM-PCR products in both libraries revealed that most of the sequences were quite different, and had a long open reading frame without a frame shift or stop codon. Furthermore, no distinct bias among blocks was observed. Here we describe how to use RM-PCR for the construction of combinatorial DNA libraries, which encode protein libraries that would be suitable for selection experiments in the global protein space.
机译:开发一种新的方法来创建蛋白质文库,这可以探索全球蛋白质空间,这是一个令人兴奋的挑战。在这项研究中,我们开发了随机多重组PCR(RM-PCR),该PCR允许几个DNA片段的改组而无需同源序列。为了评估此方法,我们将其应用于创建两个不同的组合DNA库。为了构建“随机改组文库”,RM-PCR用于改组6个DNA片段,每个片段编码25个氨基酸。这提供了许多不同的片段序列,它们的每个位置都有相等的概率来编码六个块中的任何一个。对于“替代剪接文库”的构建,RM-PCR被用于在DNA水平上执行不同的替代剪接,这也产生了不同的嵌段序列。两个文库中RM-PCR产物的DNA测序表明,大多数序列完全不同,并且具有较长的开放阅读框,没有移码或终止密码子。此外,在块之间没有观察到明显的偏差。在这里,我们描述了如何使用RM-PCR来构建组合DNA文库,该文库编码的蛋白质文库适合在全球蛋白质空间中进行选择实验。

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