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Adoption of the Q transcriptional regulatory system for zebrafish transgenesis

机译:Q转录调控系统对斑马鱼转基因的采用

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The Gal4-UAS regulatory system of yeast is widely used to modulate gene expression in Drosophila; however, there are limitations to its usefulness in transgenic zebrafish, owing to progressive methylation and silencing of the CpG-rich multicopy upstream activation sequence. Although a modified, less repetitive UAS construct may overcome this problem, it is highly desirable to have additional transcriptional regulatory systems that can be applied independently or in combination with the Gal4/UAS system for intersectional gene expression. The Q transcriptional regulatory system of Neurospora crassa functions similarly to Gal4/UAS. QF is a transcriptional activator that binds to the QUAS upstream regulatory sequence to drive reporter gene expression. Unlike Gal4, the QF binding site does not contain essential CpG dinucleotide sequences that are subject to DNA methylation. The QS protein is a repressor of QF mediated transcriptional activation akin to Gal80. The functionality of the Q system has been demonstrated in Drosophila and Caenorhabditis elegans and we now report its successful application to a vertebrate model, the zebrafish, Danio rerio. Several tissue-specific promoters were used to drive QF expression in stable transgenic lines, as assessed by activation of a QUAS:GFP transgene. The QS repressor was found to dramatically reduce QF activity in injected zebrafish embryos; however, a similar repression has not yet been achieved in transgenic animals expressing QS under the control of ubiquitous promoters. A dual reporter construct containing both QUAS and UAS, each upstream of different fluorescent proteins was also generated and tested in transient assays, demonstrating that the two systems can work in parallel within the same cell. The adoption of the Q system should greatly increase the versatility and power of transgenic approaches for regulating gene expression in zebrafish.
机译:酵母的Gal4-UAS调节系统被广泛用于调节果蝇中的基因表达。但是,由于富含CpG的多拷贝上游激活序列的逐步甲基化和沉默,其在转基因斑马鱼中的用途受到限制。尽管经过修改的,重复性较低的UAS构建体可以解决此问题,但非常需要具有其他转录调控系统,这些系统可以独立应用或与Gal4 / UAS系统结合使用以进行交叉基因表达。芥菜神经孢的Q转录调节系统的功能类似于Gal4 / UAS。 QF是一种转录激活因子,可与QUAS上游调节序列结合以驱动报告基因的表达。与Gal4不同,QF结合位点不包含必需的CpG二核苷酸序列,该序列必须经历DNA甲基化。 QS蛋白是QF介导的类似于Gal80的转录激活的阻遏物。 Q系统的功能已在果蝇和秀丽隐杆线虫中得到证实,现在我们报道了其在脊椎动物模型斑马鱼Danio rerio中的成功应用。如通过QUAS:GFP转基因的激活所评估的,几种组织特异性启动子用于在稳定的转基因系中驱动QF表达。发现QS阻遏物可显着降低注射的斑马鱼胚胎中的QF活性。然而,在遍在启动子控制下表达QS的转基因动物中尚未实现类似的抑制。还生成了同时包含每个荧光蛋白上游的QUAS和UAS的双报告子构建体,并在瞬时分析中对其进行了测试,表明这两个系统可以在同一细胞内并行工作。 Q系统的采用应大大提高转基因方法在斑马鱼中调控基因表达的多功能性和功能。

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