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增殖细胞核抗原基因的多个启动子元件在果蝇发育过程中的作用。

Roles of multiple promoter elements of the proliferating cell nuclear antigen gene during Drosophila development.

作者信息

Yamaguchi M, Hirose F, Matsukage A

机构信息

Laboratory of Cell Biology, Aichi Cancer Centre Research Institute, Nagoya, Japan.

出版信息

Genes Cells. 1996 Jan;1(1):47-58. doi: 10.1046/j.1365-2443.1996.03003.x.

DOI:10.1046/j.1365-2443.1996.03003.x
PMID:9078366
Abstract

The expression of genes involved in DNA replication is closely correlated with the proliferating state of cells and is repressed with the progression of differentiation during development. Promoter regions of the Drosophila proliferating cell nuclear antigen (PCNA) gene and the DNA polymerase alpha gene contain a common 8-base pair promoter element (DRE: DNA replication-related element). The examination of a common expression mechanism for DNA replication-related genes, which is regulated positively by growth signals and negatively by differentiation signals would be of interest. We generated PCNA-LacZ fusion genes in which the 5'-flanking sequence of the PCNA gene has been mutated. An examination of the expression of these fusion genes, introduced into flies by germ-line transformation, led to the identification of another distinct regulatory element, URE (upstream regulatory element), within the region from -168 to -119 with respect to the transcription initiation site. During embryogenesis, the region containing the DRE sequence (-108 to -91) greatly stimulated the PCNA gene minimal promoter (-86 to +130), when it was placed upstream of the promoter in both normal and reverse orientations. Addition of the URE sequence further stimulated the promoter activity twofold. During larval stages, both DRE and URE were indispensable to the promoter activity, since neither of the sequences alone activated the minimal promoter. Demonstration of beta-galactosidase activity indicated URE plays an essential role in various larval tissues such as salivary gland and imaginal disc. While the minimal promoter region alone directed maternal expression of lacZ in ovaries of adult females, both DRE and URE further stimulated promoter activity. These results show several elements of the PCNA gene promoter play roles during Drosophila development.

摘要

参与DNA复制的基因表达与细胞的增殖状态密切相关,并在发育过程中随着分化进程而受到抑制。果蝇增殖细胞核抗原(PCNA)基因和DNA聚合酶α基因的启动子区域含有一个共同的8碱基对启动子元件(DRE:DNA复制相关元件)。研究DNA复制相关基因的共同表达机制,即受生长信号正向调控和分化信号负向调控,将是很有意义的。我们构建了PCNA-LacZ融合基因,其中PCNA基因的5'侧翼序列已发生突变。对这些通过种系转化导入果蝇的融合基因的表达进行检测,结果在相对于转录起始位点-168至-119的区域内鉴定出另一个不同的调控元件,即上游调控元件(URE)。在胚胎发生过程中,包含DRE序列(-108至-91)的区域,无论以正向还是反向置于启动子上游时,都能极大地刺激PCNA基因最小启动子(-86至+130)。添加URE序列可使启动子活性进一步提高两倍。在幼虫阶段,DRE和URE对启动子活性都是不可或缺的,因为单独的任何一个序列都不能激活最小启动子。β-半乳糖苷酶活性的检测表明URE在各种幼虫组织如唾液腺和成虫盘等中起着至关重要的作用。虽然单独的最小启动子区域可指导成年雌性果蝇卵巢中lacZ的母源表达,但DRE和URE都能进一步刺激启动子活性。这些结果表明PCNA基因启动子的几个元件在果蝇发育过程中发挥作用。

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