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Molecular genetic transfection of the coccidian parasite Sarcocystis neurona.

机译:球虫寄生虫囊藻神经元的分子遗传转染。

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摘要

Sarcocystis neurona is an apicomplexan parasite that is the major cause of equine protozoal myeloencephalitis (EPM). The biology of this pathogen remains poorly understood in part due to unavailability of molecular genetic tools. Hence, with an objective to develop DNA transfection capabilities for S. neurona, the 5' flanking region of the SnSAG1 gene was isolated from a genomic library and used to construct expression plasmids. In transient assays, the reporter molecules beta-galactosidase (beta-gal) and yellow fluorescent protein (YFP) could be detected in electroporated S. neurona, thereby confirming the feasibility of transgene expression in this organism. Stable transformation of S. neurona was achieved using a mutant dihydrofolate reductase thymidylate synthase (DHFR-TS) gene of Toxoplasma gondii that confers resistance to pyrimethamine. This selection system was used to create transgenic S. neurona that stably express beta-gal and YFP. As shown in this study, these transgenic clones can be useful for analyzing growth rate of parasites in vitro and for assessing drug sensitivities. More importantly, the DNA transfection methods described herein should greatly facilitate studies examining intracellular parasitism by this important coccidian pathogen.
机译:肉胞藻是一种寄生虫,是马原生动物脊髓性脑炎(EPM)的主要原因。由于分子遗传工具的缺乏,对该病原体的生物学知之甚少。因此,以开发针对神经链球菌的DNA转染能力为目的,从基因组文库中分离出SnSAG1基因的5'侧翼区并用于构建表达质粒。在瞬时测定中,可在电穿孔的神经链霉菌中检测到报告分子β-半乳糖苷酶(β-gal)和黄色荧光蛋白(YFP),从而证实了在该生物中表达转基因的可行性。使用赋予弓形虫抗药性的弓形虫突变型二氢叶酸还原酶胸苷酸合酶(DHFR-TS)基因实现了稳定的神经链球菌转化。该选择系统用于产生稳定表达β-gal和YFP的转基因链球菌。如本研究所示,这些转基因克隆可用于体外分析寄生虫的生长速率和评估药物敏感性。更重要的是,本文所述的DNA转染方法应大大促进研究这种重要的球虫病原体检查细胞内寄生虫的研究。

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