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A versatile strategy for rapid conditional genome engineering using loxP sites in a small synthetic intron in Plasmodium falciparum

机译:在恶性疟原虫的小型合成内含子中使用loxp位点进行快速条件基因组工程的通用策略

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摘要

Conditional genome engineering in the human malaria pathogen Plasmodium falciparum remains highly challenging. Here we describe a strategy for facile and rapid functional analysis of genes using an approach based on the Cre/lox system and tailored for organisms with short and few introns. Our method allows the conditional, site-specific removal of genomic sequences of essential and non-essential genes by placing loxP sites into a short synthetic intron to produce a module (loxPint) can be placed anywhere in open reading frames without compromising protein expression. When duplicated, the loxPint module serves as an intragenic recombineering point that can be used for the fusion of gene elements to reporters or the conditional introduction of point mutations. We demonstrate the robustness and versatility of the system by targeting the P. falciparum merozoite surface protein 1 gene (msp1), which has previously proven refractory to genetic interrogation, and the parasite exported kinase FIKK10.1.
机译:人类疟疾病原体恶性疟原虫中的条件基因组工程仍然具有很高的挑战性。在这里,我们描述了一种基于Cre / lox系统,针对内含子少而又少的生物量身定制的方法,可以对基因进行便捷,快速的功能分析。我们的方法允许通过将loxP位点放到短的合成内含子中以产生模块(loxPint),有条件地,位点特异性地去除必需和非必需基因的基因组序列,该模块可以放置在开放阅读框中的任何位置而不会影响蛋白质表达。当复制时,loxPint模块用作基因内重组点,可用于将基因元件融合到报告基因或有条件地引入点突变。我们通过针对恶性疟原虫裂殖子表面蛋白1基因(msp1)证明了该系统的鲁棒性和多功能性,该基因先前已被证明对遗传询问无抵抗力,并且寄生虫输出激酶FIKK10.1。

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