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首页> 外文期刊>General and comparative endocrinology >Transfection of isolated rainbow trout, Oncorhynchus mykiss, granulosa cells through chemical transfection and electroporation at 12 degrees C
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Transfection of isolated rainbow trout, Oncorhynchus mykiss, granulosa cells through chemical transfection and electroporation at 12 degrees C

机译:在12摄氏度下通过化学转染和电穿孔转染分离的虹鳟鱼,mycorhynchus mykiss,颗粒细胞

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摘要

Over-expression or inhibition of gene expression can be efficiently used to analyse the functions and/or regulation of target genes. Modulation of gene expression can be achieved through transfection of exogenous nucleic acids into target cells. Such techniques require the development of specific protocols to transfect cell cultures with nucleic acids. The aim of this study was to develop a method of transfection suitable for rainbow trout granulosa cells in primary culture. After the isolation of rainbow trout granulosa cells, chemical transfection of cells with a fluorescent morpholino oligonucleotide (MO) was tested using FuGENE HD at 12 degrees C. Electroporation was also employed to transfect these cells with either a plasmid or MO. Transfection was more efficient using electroporation (with the following settings: 1200 V/40 ms/1 p) than chemical transfection, but electroporation by itself was deleterious, resulting in a decrease of the steroidogenic capacity of the cells, measured via estradiol production from its androgenic substrate. The disturbance of cell biology induced by the transfection method per se should be taken into account in data interpretation when investigating the effects of under- or over-expression of candidate genes. (C) 2015 Elsevier Inc. All rights reserved.
机译:基因表达的过表达或抑制可有效地用于分析靶基因的功能和/或调节。基因表达的调节可通过将外源核酸转染到靶细胞中来实现。这样的技术需要开发特定的方案以用核酸转染细胞培养物。这项研究的目的是开发一种适合原代培养中虹鳟颗粒细胞的转染方法。分离虹鳟颗粒细胞后,在12摄氏度下使用FuGENE HD测试了用荧光吗啉代寡核苷酸(MO)进行的细胞化学转染。还使用电穿孔法用质粒或MO转染这些细胞。使用电穿孔(具有以下设置:1200 V / 40 ms / 1 p)进行转染比化学转染更有效,但电穿孔本身是有害的,导致细胞的类固醇生成能力降低(通过从其产生的雌二醇产量来衡量)雄激素底物。在调查候选基因表达不足或过高的影响时,在数据解释中应考虑到由转染方法本身引起的细胞生物学紊乱。 (C)2015 Elsevier Inc.保留所有权利。

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