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首页> 外文期刊>Genetics: A Periodical Record of Investigations Bearing on Heredity and Variation >Analysis of sequences regulating larval expression of the Adh gene of Drosophila melanogaster.
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Analysis of sequences regulating larval expression of the Adh gene of Drosophila melanogaster.

机译:分析调节果蝇Adh基因幼虫表达的序列。

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The effects of a series of eight, 50 base pair internal deletions in the 5' region upstream of the proximal transcription start site of the Adh gene of Drosophila melanogaster were examined in a quantitative assay. Mixtures of two plasmids, one bearing a deleted gene, the other with an intact reference gene, were injected into alcohol dehydrogenase-negative embryos. Third instar larvae of the injected generation were assayed for relative alcohol dehydrogenase enzyme activity. Quantitative analysis of the eight deletions indicated that two regions were required for any detectable enzyme activity and one region was required for appropriate tissue specificity. The remaining five deletions significantly decreased, but did not eliminate activity. When the deleted genes were placed on a plasmid with an intact reference gene, activities of all but one deletion were restored to levels equivalent to that of the intact reference gene (regardless of orientation). This restoration of activity did not occur when the regulatory region of the intact gene was replaced with the Hsp70 heat shock promoter nor when the 50-base pair deletion encompassed the region that includes the TATA sequence. The fact that seven of the eight deleted genes express activity in the presence of a reference gene on the same plasmid suggests that the deleted gene is controlled by regulatory elements in the reference gene. Further, these regulatory elements exhibit no preference for their own, more proximate, promoter.
机译:在定量测定中检查了果蝇Adh基因的近端转录起始位点上游的5'区域上游的一系列八个,50个碱基对的内部缺失的影响。将两种质粒的混合物注射到乙醇脱氢酶阴性的胚胎中,一种质粒带有缺失的基因,另一种带有完整的参考基因。分析了所注射代的第三龄幼虫的相对醇脱氢酶活性。八个缺失的定量分析表明,任何可检测的酶活性都需要两个区域,而适当的组织特异性则需要一个区域。其余五个删除明显减少,但没有消除活性。当将缺失的基因置于具有完整参考基因的质粒上时,除一个缺失外,所有缺失基因的活性都恢复到与完整参考基因相同的水平(与方向无关)。当完整基因的调控区被Hsp70热休克启动子取代时,或者当50个碱基对的缺失涵盖了包含TATA序列的区域时,都没有发生这种活性恢复。八个缺失基因中的七个在相同质粒上存在参照基因的情况下表达活性的事实表明,该缺失基因受参照基因中的调控元件控制。此外,这些调节元件对它们自己的,更接近的启动子没有偏好。

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