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黑腹果蝇ninaE视蛋白基因启动子的分析

Analysis of the promoter of the ninaE opsin gene in Drosophila melanogaster.

作者信息

Mismer D, Rubin G M

出版信息

Genetics. 1987 Aug;116(4):565-78. doi: 10.1093/genetics/116.4.565.

Abstract

We have analyzed the cis-acting regulatory sequences of the ninaE gene. This gene encodes the major Drosophila melanogaster opsin, the protein component of the primary chromophore of photo-receptor cells R1-R6 of the adult eye. DNA fragments containing the start point of transcription of the ninaE gene were fused to either the Escherichia coli chloramphenicol acetyltransferase or lacZ (beta-galactosidase) gene and introduced into the Drosophila germline by P-element-mediated transformation. Expression of the E. coli genes was then used to assay the ability of various sequences from the ninaE gene to confer the ninaE pattern of expression. Fragments containing between 2.8 kb and 215 bp of the sequences upstream of the start of transcription plus the first 67 bp of the untranslated leader were able to direct nearly wild-type expression. We have identified three separable control regions in the ninaE promoter. The first, which has the properties of an enhancer element, is located between nucleotides -501 and -219. The removal of this sequence had little effect on promoter function; this sequence appears to be redundant. However, it appears to be able to substitute for the second control region which is located between nucleotides -215 and -162, and which also affects the level of output from this promoter. Removal of these two control regions resulted in a 30-fold decrease in expression; however tissue specificity was not affected. The third control region, located downstream from nucleotide -120, appears to be absolutely necessary for promoter function in the absence of the first two regulatory sequences. Examination of larvae containing fusion genes expressing beta-galactosidase suggests that the ninaE gene is also expressed in a subset of cells in the larval photoreceptor organ.

摘要

我们分析了ninaE基因的顺式作用调控序列。该基因编码果蝇主要的视蛋白,即成年果蝇复眼中R1 - R6感光细胞初级发色团的蛋白质成分。将包含ninaE基因转录起始点的DNA片段与大肠杆菌氯霉素乙酰转移酶基因或lacZ(β - 半乳糖苷酶)基因融合,并通过P因子介导的转化导入果蝇生殖系。然后利用大肠杆菌基因的表达来检测ninaE基因的各种序列赋予ninaE基因表达模式的能力。包含转录起始点上游2.8 kb至215 bp序列以及未翻译前导序列的前67 bp的片段能够指导近乎野生型的表达。我们在ninaE启动子中鉴定出三个可分离的控制区域。第一个区域具有增强子元件的特性,位于核苷酸 - 501和 - 219之间。去除该序列对启动子功能影响不大;该序列似乎是冗余的。然而,它似乎能够替代位于核苷酸 - 215和 - 162之间的第二个控制区域,该区域也影响该启动子的输出水平。去除这两个控制区域导致表达下降30倍;然而组织特异性不受影响。第三个控制区域位于核苷酸 - 120下游,在没有前两个调控序列的情况下,对于启动子功能似乎是绝对必要的。对含有表达β - 半乳糖苷酶融合基因的幼虫的检查表明,ninaE基因也在幼虫感光器官的一部分细胞中表达。

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