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寄生虫线虫中的核酸转染和转基因。

Nucleic acid transfection and transgenesis in parasitic nematodes.

机构信息

Department of Pathobiology, School of Veterinary Medicine, University of Pennsylvania, 3800 Spruce Street, Philadelphia, PA 19104, USA.

出版信息

Parasitology. 2012 Apr;139(5):574-88. doi: 10.1017/S0031182011001387. Epub 2011 Aug 31.

Abstract

Transgenesis is an essential tool for assessing gene function in any organism, and it is especially crucial for parasitic nematodes given the dwindling armamentarium of effective anthelmintics and the consequent need to validate essential molecular targets for new drugs and vaccines. Two of the major routes of gene delivery evaluated to date in parasitic nematodes, bombardment with DNA-coated microparticles and intragonadal microinjection of DNA constructs, draw upon experience with the free-living nematode Caenorhabditis elegans. Bombardment has been used to transiently transfect Ascaris suum, Brugia malayi and Litomosoides sigmodontis with both RNA and DNA. Microinjection has been used to achieve heritable transgenesis in Strongyloides stercoralis, S. ratti and Parastrongyloides trichosuri and for additional transient expression studies in B. malayi. A third route of gene delivery revisits a classic method involving DNA transfer facilitated by calcium-mediated permeabilization of recipient cells in developing B. malayi larvae and results in transgene inheritance through host and vector passage. Assembly of microinjected transgenes into multi-copy episomal arrays likely results in their transcriptional silencing in some parasitic nematodes. Methods such as transposon-mediated transgenesis that favour low-copy number chromosomal integration may remedy this impediment to establishing stable transgenic lines. In the future, stable transgenesis in parasitic nematodes could enable loss-of-function approaches by insertional mutagenesis, in situ expression of inhibitory double-stranded RNA or boosting RNAi susceptibility through heterologous expression of dsRNA processing and transport proteins.

摘要

转基因技术是评估任何生物体中基因功能的重要工具,对于寄生线虫来说尤其重要,因为有效的驱虫药物越来越少,因此需要验证新药物和疫苗的必要分子靶标。迄今为止,在寄生线虫中评估的两种主要基因传递途径,即用 DNA 包被的微粒子轰击和 DNA 构建体的性腺内微注射,都借鉴了自由生活线虫秀丽隐杆线虫的经验。轰击已被用于瞬时转染猪蛔虫、马来丝虫和西格莫线虫的 RNA 和 DNA。微注射已被用于使粪类圆线虫、大鼠粪类圆线虫和 Parastrongyloides trichosuri 获得可遗传的转基因,并在马来丝虫中进行额外的瞬时表达研究。第三种基因传递途径重新审视了一种经典方法,该方法涉及通过钙介导的接受细胞通透性促进 DNA 转移,从而导致转基因通过宿主和载体传递进行遗传。微注射转基因的组装成多拷贝的附加体阵列可能导致它们在一些寄生线虫中转录沉默。转座子介导的转基因技术等方法有利于低拷贝数染色体整合,可能会克服建立稳定的转基因系的这一障碍。将来,寄生线虫的稳定转基因技术可以通过插入诱变、双链 RNA 的原位表达或通过异源表达 dsRNA 加工和运输蛋白来提高 RNAi 敏感性,从而实现功能丧失方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a201/3319118/97b3c97f4a63/nihms365486f1.jpg

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