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原始原生动物病原体蓝氏贾第鞭毛虫的稳定DNA转染

Stable DNA transfection of the primitive protozoan pathogen Giardia lamblia.

作者信息

Sun C H, Chou C F, Tai J H

机构信息

Graduate Institute of Life Sciences, National Defense Medical Center, Taipei, Taiwan, ROC.

出版信息

Mol Biochem Parasitol. 1998 Apr 1;92(1):123-32. doi: 10.1016/s0166-6851(97)00239-9.

Abstract

We have developed a stable DNA transfection vector pRANneo for genetic manipulation of the primitive protozoan Giardia lamblia. pRANneo was constructed by replacing the protein coding region of a Giardia ran gene with a bacterial neomycin phosphotransferase gene (neo). This plasmid was electroporated into G. lamblia, and the transfectants were selected by G418. pRANneo replicated episomally to approximately 80 copies per G. lamblia trophozoite as demonstrated by dot hybridizations, Southern hybridizations and transformations of the DpnI-treated plasmids into Escherichia coli. pRANneo/GDHluc was then constructed by incorporation of a luciferase expression system into pRANneo to persistently express firefly luciferase in G. lamblia under G418 selection. The NEO and luciferase proteins were detected in the transfected G. lamblia cells by Western blottings. The level of luciferase activity and the plasmid copy number correlated with the concentration of G418. Removal of G418 from the transfectant culture resulted in gradual loss of the plasmid and luciferase activity. The stable DNA transfection system should provide a valuable tool for genetic studies of G. lamblia.

摘要

我们开发了一种稳定的DNA转染载体pRANneo,用于对原生动物蓝氏贾第鞭毛虫进行基因操作。pRANneo是通过用细菌新霉素磷酸转移酶基因(neo)取代贾第鞭毛虫ran基因的蛋白质编码区构建而成的。将该质粒电穿孔导入蓝氏贾第鞭毛虫,并用G418筛选转染子。通过斑点杂交、Southern杂交以及将经DpnI处理的质粒转化到大肠杆菌中证明,pRANneo以附加体形式复制,每个蓝氏贾第鞭毛虫滋养体约有80个拷贝。然后通过将荧光素酶表达系统引入pRANneo构建了pRANneo/GDHluc,以便在G418选择下在蓝氏贾第鞭毛虫中持续表达萤火虫荧光素酶。通过蛋白质免疫印迹法在转染的蓝氏贾第鞭毛虫细胞中检测到了NEO和荧光素酶蛋白。荧光素酶活性水平和质粒拷贝数与G418浓度相关。从转染子培养物中去除G418会导致质粒和荧光素酶活性逐渐丧失。这种稳定的DNA转染系统应为蓝氏贾第鞭毛虫的遗传学研究提供一种有价值的工具。

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