Geurts Aron M, Wilber Andrew, Carlson Corey M, Lobitz Paul D, Clark Karl J, Hackett Perry B, McIvor R Scott, Largaespada David A
Department of Genetics, Cell Biology, and Development, The Arnold and Mabel Beckman Center for Transposon Research, University of Minnesota, Minneapolis, MN 55455, USA.
BMC Biotechnol. 2006 Jun 26;6:30. doi: 10.1186/1472-6750-6-30.
Insertional mutagenesis techniques with transposable elements have been popular among geneticists studying model organisms from E. coli to Drosophila and, more recently, the mouse. One such element is the Sleeping Beauty (SB) transposon that has been shown in several studies to be an effective insertional mutagen in the mouse germline. SB transposon vector studies have employed different functional elements and reporter molecules to disrupt and report the expression of endogenous mouse genes. We sought to generate a transposon system that would be capable of reporting the expression pattern of a mouse gene while allowing for conditional expression of a gene of interest in a tissue- or temporal-specific pattern.
Here we report the systematic development and testing of a transposon-based gene-trap system incorporating the doxycycline-repressible Tet-Off (tTA) system that is capable of activating the expression of genes under control of a Tet response element (TRE) promoter. We demonstrate that the gene trap system is fully functional in vitro by introducing the "gene-trap tTA" vector into human cells by transposition and identifying clones that activate expression of a TRE-luciferase transgene in a doxycycline-dependent manner. In transgenic mice, we mobilize gene-trap tTA vectors, discover parameters that can affect germline mobilization rates, and identify candidate gene insertions to demonstrate the in vivo functionality of the vector system. We further demonstrate that the gene-trap can act as a reporter of endogenous gene expression and it can be coupled with bioluminescent imaging to identify genes with tissue-specific expression patterns.
Akin to the GAL4/UAS system used in the fly, we have made progress developing a tool for mutating and revealing the expression of mouse genes by generating the tTA transactivator in the presence of a secondary TRE-regulated reporter molecule. A vector like the gene-trap tTA could provide a means for both annotating mouse genes and creating a resource of mice that express a regulable transcription factor in temporally- and tissue-specific patterns for conditional gene expression studies. These mice would be a valuable resource to the mouse genetics community for purpose of dissecting mammalian gene function.
利用转座元件的插入诱变技术在研究从大肠杆菌到果蝇以及最近的小鼠等模式生物的遗传学家中很受欢迎。其中一种元件是睡美人(SB)转座子,多项研究表明它是小鼠种系中一种有效的插入诱变剂。SB转座子载体研究采用了不同的功能元件和报告分子来破坏和报告内源性小鼠基因的表达。我们试图构建一种转座子系统,该系统能够报告小鼠基因的表达模式,同时允许以组织或时间特异性模式有条件地表达感兴趣的基因。
在此,我们报告了一种基于转座子的基因捕获系统的系统开发和测试,该系统整合了强力霉素可抑制的Tet-Off(tTA)系统,能够激活四环素反应元件(TRE)启动子控制下的基因表达。我们通过转座将“基因捕获tTA”载体导入人细胞,并鉴定出以强力霉素依赖方式激活TRE-荧光素酶转基因表达的克隆,从而证明该基因捕获系统在体外完全功能正常。在转基因小鼠中,我们动员基因捕获tTA载体,发现可影响种系动员率的参数,并鉴定候选基因插入位点,以证明载体系统的体内功能。我们进一步证明,基因捕获可以作为内源性基因表达的报告子,并且可以与生物发光成像相结合,以鉴定具有组织特异性表达模式的基因。
类似于果蝇中使用的GAL4/UAS系统,我们在开发一种工具方面取得了进展,该工具通过在二级TRE调控的报告分子存在下产生tTA反式激活因子来突变和揭示小鼠基因的表达。像基因捕获tTA这样的载体可以为注释小鼠基因以及创建一个小鼠资源库提供一种手段,该资源库以时间和组织特异性模式表达可调节的转录因子,用于条件性基因表达研究。这些小鼠将是小鼠遗传学领域剖析哺乳动物基因功能的宝贵资源。
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