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快速筛选 BAC 用于斑马鱼的 tol2 介导转基因。

Rapid BAC selection for tol2-mediated transgenesis in zebrafish.

机构信息

Hubrecht Institute - KNAW and Utrecht Medical Center, Uppsalalaan 8, 3584 CT, Utrecht, The Netherlands.

出版信息

Development. 2011 Oct;138(19):4327-32. doi: 10.1242/dev.068080. Epub 2011 Aug 24.

DOI:10.1242/dev.068080
PMID:21865323
Abstract

The generation of zebrafish transgenic lines that express specific fluorophores in a cell- or tissue-specific manner is an important technique that takes full advantage of the optical clarity of the embryo. Identifying promoter fragments that faithfully recapitulate endogenous expression patterns and levels is often difficult and using large genomic DNA fragments, such as bacterial artificial chromosomes (BACs), makes the process of transgenesis less reliable. Here we provide a detailed protocol that allows for BAC selection and subsequent rapid modification through recombineering in Escherichia coli, resulting in BACs that can be injected into zebrafish embryos and, aided by tol2-mediated transgenesis, reliably yield stable transgenic lines. A number of BACs can be prepared in parallel, and injection of the BACs containing CFP/YFP/RFP or Gal4 cassettes allows for immediate testing of whether a particular BAC will yield the desired result. Furthermore, since injected embryos often show widespread expression, recombineered BACs provide an alternative to two-color in situ hybridizations: BACs injected into embryos of a different transgenic reporter line thus enable in vivo colocalization studies. Using this protocol, we have generated 66 stable lines for 23 different genes, with an average transgenesis rate above 10%. Importantly, we provide evidence that BAC size shows no apparent correlation to the transgenesis rate achieved and that there are no severe position effects.

摘要

生成以细胞或组织特异性方式表达特定荧光蛋白的斑马鱼转基因系是充分利用胚胎光学透明度的重要技术。鉴定能真实再现内源性表达模式和水平的启动子片段通常很困难,而且使用细菌人工染色体 (BAC) 等大基因组 DNA 片段会使转基因过程的可靠性降低。在这里,我们提供了一个详细的方案,允许通过大肠杆菌中的重组酶工程进行 BAC 选择和随后的快速修饰,从而产生可注射到斑马鱼胚胎中的 BAC,并借助 tol2 介导的转基因技术,可靠地产生稳定的转基因系。可以并行制备多个 BAC,并且注射包含 CFP/YFP/RFP 或 Gal4 盒的 BAC 可以立即测试特定 BAC 是否会产生所需的结果。此外,由于注射的胚胎通常表现出广泛的表达,因此重组 BAC 提供了替代双色原位杂交的方法:注射到不同转基因报告系胚胎中的 BAC 可用于体内共定位研究。使用此方案,我们已经为 23 个不同基因生成了 66 个稳定的系,平均转基因率超过 10%。重要的是,我们提供的证据表明 BAC 大小与实现的转基因率之间没有明显的相关性,并且没有严重的位置效应。

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