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Cloning, sequence and characterization of the human AMPD2 gene: evidence for transcriptional regulation by two closely spaced promoters

机译:人AMPD2基因的克隆,序列和表征:两个紧密间隔的启动子进行转录调控的证据

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摘要

AMP deaminase (AMPD) is manifest through a multigene family in higher eukaryotes, including man. The human AMPDJ and AMPD3 genes have been cloned and partially characterized. This study describes the cloning, chromosomal localization, partial sequence and characterization of the human AMPD2 gene. Composed of nineteen exons and eighteen intervening sequences spanning nearly 14 kb of genomic DNA, the human AMPD2 gene is positioned on the short arm of chromosome 1 near the pl3.3 boundary. Two alternative 5' exons (1A and IB) are remotely located upstream, whereas the other seventeen are compressed into the 3' terminal one-half of the gene. Transient transfections of human retinal pigment epithelial (RPE) cells using heterologous constructs containing 5' flanking and 5' untranslated sequences cloned upstream of a luciterase reporter gene show that promoter activities are associated with exons 1A and IB. Inspection of genomic DNA sequence reveals that AMPD2 promoter regions lack readily identifiable TATA boxes and are G + C-rich, particularly in the region of multiple transcription initiation sites in exon 1A. The regulation and evolution of the entire human AMPD multigene family are discussed.
机译:AMP脱氨酶(AMPD)通过多基因家族在包括人在内的高等真核生物中表现出来。人的AMPDJ和AMPD3基因已被克隆并部分表征。这项研究描述了人AMPD2基因的克隆,染色体定位,部分序列和特征。人类AMPD2基因由19个外显子和18个居间序列组成,跨越近14 kb的基因组DNA,位于第1号染色体的短臂上,靠近pl3.3边界。两个可供选择的5'外显子(1A和IB)位于上游,而其他十七个被压缩到该基因3'末端的一半。使用含有克隆到荧光酶报道基因上游的5'侧翼和5'非翻译序列的异源构建体对人视网膜色素上皮(RPE)细胞进行瞬时转染显示,启动子活性与外显子1A和IB相关。对基因组DNA序列的检查显示,AMPD2启动子区域缺少易于识别的TATA框,富含G + C,特别是在外显子1A中的多个转录起始位点区域。讨论了整个人类AMPD多基因家族的调控和进化。

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