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A Systematic Enhancer Screen Using Lentivector Transgenesis Identifies Conserved and Non-Conserved Functional Elements at the Olig1 and Olig2 Locus

机译:使用Lentivector转基因的系统增强子屏幕可识别Olig1和Olig2基因座的保守和非保守功能元件

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摘要

Finding sequences that control expression of genes is central to understanding genome function. Previous studies have used evolutionary conservation as an indicator of regulatory potential. Here, we present a method for the unbiased in vivo screen of putative enhancers in large DNA regions, using the mouse as a model. We cloned a library of 142 overlapping fragments from a 200 kb-long murine BAC in a lentiviral vector expressing LacZ from a minimal promoter, and used the resulting vectors to infect fertilized murine oocytes. LacZ staining of E11 embryos obtained by first using the vectors in pools and then testing individual candidates led to the identification of 3 enhancers, only one of which shows significant evolutionary conservation. In situ hybridization and 3C/4C experiments suggest that this enhancer, which is active in the neural tube and posterior diencephalon, influences the expression of the Olig1 and/or Olig2 genes. This work provides a new approach for the large-scale in vivo screening of transcriptional regulatory sequences, and further demonstrates that evolutionary conservation alone seems too limiting a criterion for the identification of enhancers.
机译:寻找控制基因表达的序列对于理解基因组功能至关重要。先前的研究已将进化保守性用作调节潜力的指标。在这里,我们提出了一种使用鼠标作为模型的无偏见的大分子DNA区域推定增强子的体内筛选方法。我们从一个最小启动子表达LacZ的慢病毒载体中,从200 kb长的鼠类BAC中克隆了142个重叠片段的文库,并使用所得载体感染受精的鼠卵母细胞。首先通过在库中使用载体,然后测试单个候选物,对E11胚胎进行LacZ染色,从而鉴定出3种增强子,其中只有一种显示出显着的进化保守性。原位杂交和3C / 4C实验表明,这种增强子在神经管和后脑后部中活跃,影响Olig1和/或Olig2基因的表达。这项工作为大规模体内筛选转录调控序列提供了一种新方法,并进一步证明仅进化保守似乎太限制了鉴定增强子的标准。

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