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Construction of a bicistronic vector for the co-expression of two genes

机译:共表达两个基因的双顺反子载体的构建

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摘要

The nematode Caenorhabditis elegans is an important model animal for biological research. Currently, transgenic C. elegans strains are mainly generated by injecting DNA encoding a gene of interest, in combination with a reporter gene, into the gonad. With this approach, the interpretation of negative results, such as the failure to observe reporter expression, is frequently required. Single, selectable vectors are urgently required. Internal ribosome entry site (IRES) elements are known to bind the eukaryotic ribosomal translation initiation complex and independently promote translation initiation. Bioinformatic analysis predicted an IRES motif upstream of the start codon of the C. elegans Hsp-3 gene. While this sequence has a Y-shaped double-hairpin secondary structure characteristic of IRES elements, it was unclear if it could function as an IRES. In the present study, this predicted Hsp-3 IRES was incorporated into a bicistronic vector driven by the myo-3 promoter, which allowed co-expression of RFP and GFP genes in the muscle tissue of C. elegans and thereby demonstrated that this IRE,S element is functional. This vector provides a novel, powerful tool for C. elegans research.
机译:线虫秀丽隐杆线虫是生物学研究的重要模型动物。目前,转基因秀丽隐杆线虫菌株主要是通过将编码目的基因的DNA与报道基因一起注入性腺中而产生的。通过这种方法,经常需要对阴性结果进行解释,例如未能观察到报道基因表达。迫切需要单个可选择的载体。已知内部核糖体进入位点(IRES)元件结合真核生物核糖体翻译起始复合物并独立地促进翻译起始。生物信息学分析预测秀丽隐杆线虫Hsp-3基因的起始密码子上游的IRES主题。虽然该序列具有IRES元件的Y形双发夹二级结构特征,但是尚不清楚它是否可以充当IRES。在本研究中,将这种预测的Hsp-3 IRES整合到由myo-3启动子驱动的双顺反子载体中,该启动子允许在秀丽隐杆线虫的肌肉组织中共表达RFP和GFP基因,从而证明该IRE, S元素起作用。该载体为秀丽隐杆线虫的研究提供了一种新颖而强大的工具。

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