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利用Tol2转座子介导的转基因技术在斑马鱼中评估假定增强子的生物学相关性。

Evaluating the biological relevance of putative enhancers using Tol2 transposon-mediated transgenesis in zebrafish.

作者信息

Fisher Shannon, Grice Elizabeth A, Vinton Ryan M, Bessling Seneca L, Urasaki Akihiro, Kawakami Koichi, McCallion Andrew S

机构信息

McKusick-Nathans Institute of Genetic Medicine, Johns Hopkins University School of Medicine, Baltimore, MD 21205, USA.

出版信息

Nat Protoc. 2006;1(3):1297-305. doi: 10.1038/nprot.2006.230.

Abstract

Evaluating the biological relevance of the myriad putative regulatory noncoding sequences in vertebrate genomes represents a huge challenge. Functional analyses in vivo have typically relied on costly and labor-intensive transgenic strategies in mice. Transgenesis has also been applied in nonrodent vertebrates, such as zebrafish, but until recently these efforts have been hampered by significant mosaicism and poor rates of germline transmission. We have developed a transgenic strategy in zebrafish based on the Tol2 transposon, a mobile element that was recently identified in another teleost, Medaka. This method takes advantage of the increased efficiency of genome integration that is afforded by this intact DNA transposon, activity that is mediated by the corresponding transposase protein. The approach described in this protocol uses a universal vector system that permits rapid incorporation of DNA that is tagged with sequence targets for site-specific recombination. To evaluate the regulatory potential of a candidate sequence, the desired interval is PCR-amplified using sequence-specific primers that are flanked by the requisite target sites for cloning, and recombined into a universal expression plasmid (pGW_cfosEGFP). Purified recombinant DNAs are then injected into 1-2-cell zebrafish embryos and the resulting reporter expression patterns are analyzed at desired timepoints during development. This system is amenable to large-scale application, facilitating rapid functional analysis of noncoding sequences from both mammalian and teleost species.

摘要

评估脊椎动物基因组中大量假定的调控非编码序列的生物学相关性是一项巨大挑战。体内功能分析通常依赖于小鼠中成本高昂且 labor-intensive 的转基因策略。转基因技术也已应用于非啮齿类脊椎动物,如斑马鱼,但直到最近,这些努力一直受到显著的嵌合现象和种系传递率低的阻碍。我们基于 Tol2 转座子开发了一种斑马鱼转基因策略,Tol2 转座子是一种最近在另一种硬骨鱼——青鳉中发现的移动元件。该方法利用了这种完整 DNA 转座子所带来的基因组整合效率的提高,这种活性由相应的转座酶蛋白介导。本方案中描述的方法使用了一种通用载体系统,该系统允许快速整合带有用于位点特异性重组的序列靶点标签的 DNA。为了评估候选序列的调控潜力,使用两侧带有用于克隆的必需靶点的序列特异性引物对所需区间进行 PCR 扩增,并将其重组到通用表达质粒(pGW_cfosEGFP)中。然后将纯化的重组 DNA 注射到 1-2 细胞期的斑马鱼胚胎中,并在发育过程中的所需时间点分析产生的报告基因表达模式。该系统适用于大规模应用,有助于对来自哺乳动物和硬骨鱼物种的非编码序列进行快速功能分析。

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