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用于斑马鱼永久基因表达图谱绘制的优化Gal4遗传学方法。

Optimized Gal4 genetics for permanent gene expression mapping in zebrafish.

作者信息

Distel Martin, Wullimann Mario F, Köster Reinhard W

机构信息

Helmholtz Zentrum München, Institute of Developmental Genetics, Ingolstädter Landstrasse 1, 85764 Neuherberg, Germany.

出版信息

Proc Natl Acad Sci U S A. 2009 Aug 11;106(32):13365-70. doi: 10.1073/pnas.0903060106. Epub 2009 Jul 23.

Abstract

Combinatorial genetics for conditional transgene activation allows studying gene function with temporal and tissue specific control like the Gal4-UAS system, which has enabled sophisticated genetic studies in Drosophila. Recently this system was adapted for zebrafish and promising applications have been introduced. Here, we report a systematic optimization of zebrafish Gal4-UAS genetics by establishing an optimized Gal4-activator (KalTA4). We provide quantitative data for KalTA4-mediated transgene activation in dependence of UAS copy numbers to allow for studying dosage effects of transgene expression. Employing a Tol2 transposon-mediated KalTA4 enhancer trap screen biased for central nervous system expression, we present a collection of self-reporting red fluorescent KalTA4 activator strains. These strains reliably transactivate UAS-dependent transgenes and can be rendered homozygous. Furthermore, we have characterized the transactivation kinetics of tissue-specific KalTA4 activation, which led to the development of a self-maintaining effector strain "Kaloop." This strain relates transient KalTA4 expression during embryogenesis via a KalTA4-mediated autoregulatory mechanism to live adult structures. We demonstrate its use by showing that the secondary octaval nucleus in the adult hindbrain is likely derived from egr2b-expressing cells in rhombomere 5 during stages of early embryogenesis. These data demonstrate prolonged and maintained expression by Kalooping, a technique that can be used for permanent spatiotemporal genetic fate mapping and targeted transgene expression in zebrafish.

摘要

用于条件性转基因激活的组合遗传学能够像Gal4-UAS系统那样,通过时间和组织特异性控制来研究基因功能,该系统已在果蝇中实现了复杂的遗传学研究。最近,这个系统被应用于斑马鱼,并引入了一些有前景的应用。在这里,我们通过建立一个优化的Gal4激活因子(KalTA4),报告了斑马鱼Gal4-UAS遗传学的系统优化。我们提供了KalTA4介导的转基因激活依赖于UAS拷贝数的定量数据,以研究转基因表达的剂量效应。利用Tol2转座子介导的偏向中枢神经系统表达的KalTA4增强子捕获筛选,我们展示了一系列自我报告的红色荧光KalTA4激活因子菌株。这些菌株能可靠地反式激活依赖于UAS的转基因,并且可以纯合化。此外,我们还对组织特异性KalTA4激活的反式激活动力学进行了表征,这导致了一种自我维持效应菌株“Kaloop”的开发。该菌株通过KalTA4介导的自动调节机制,将胚胎发育过程中短暂的KalTA4表达与成年活体结构联系起来。我们通过展示成年后脑的次级八分体核可能在胚胎发育早期阶段源自菱脑节5中表达egr2b的细胞,来证明其用途。这些数据证明了通过Kalooping实现的延长和持续表达,这是一种可用于斑马鱼永久时空遗传命运图谱绘制和靶向转基因表达的技术。

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