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Development of a toolkit for piggyBac-mediated integrative transfection of the human filarial parasite Brugia malayi

机译:开发PiggyBac介导的人丝寄生虫Brugia Malayi的整合转染的工具包

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摘要

BACKGROUND:The human filarial parasites cause diseases that are among the most important causes of morbidity in the developing world. The elimination programs targeting these infections rely on a limited number of drugs, making the identification of new chemotherapeutic agents a high priority. The study of these parasites has lagged due to the lack of reverse genetic methods. METHODOLOGY/PRINCIPAL FINDINGS:We report a novel co-culture method that results in developmentally competent infective larvae of one of the human filarial parasites (Brugia malayi) and describe a method to efficiently transfect the larval stages of this parasite. We describe the production of constructs that result in integrative transfection using the piggyBac transposon system, and a selectable marker that can be used to identify transgenic parasites. We describe the production and use of dual reporter plasmids containing both a secreted luciferase selectable marker and fluorescent protein reporters that will be useful to study temporal and spatial patterns of gene expression. CONCLUSIONS/SIGNIFICANCE:The methods and constructs reported here will permit the efficient production of integrated transgenic filarial parasite lines, allowing reverse genetic technologies to be applied to all life cycle stages of the parasite.
机译:背景:人丝寄生虫引起疾病,这是发展中国家中发病率最重要的原因之一。靶向这些感染的消除程序依赖于有限数量的药物,使得鉴定新的化学治疗剂是高优先级的。由于缺乏逆向遗传方法,对这些寄生虫的研究已经滞后。方法/主要结果:我们报告了一种新的共同培养方法,导致了一种人丝虫寄生虫(Brugia Malayi)的发育态性感染性幼虫,并描述了一种有效转染寄生虫幼虫阶段的方法。我们描述了使用Piggybac转座系统产生整合转染的构建体的制备,以及可用于鉴定转基因寄生虫的可选标记。我们描述了含有分泌的荧光素酶选择标记和荧光蛋白质报告称的双重记者质粒的生产和使用,这将是研究基因表达的时间和空间模式。结论/意义:这里报道的方法和构建将允许有效地生产综合的转基因丝寄生虫,允许逆向遗传技术应用于寄生虫的所有生命周期阶段。

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