Mammalian Glutamyl Aminopeptidase Genes (ENPEP) and Proteins: Comparative Studies of a Major Contributor to Arterial Hypertension.

Roger S Holmes, Kimberly D Spradling-Reeves, Laura A Cox
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Abstract

Glutamyl aminopeptidase (ENPEP) is a member of the M1 family of endopeptidases which are mammalian type II integral membrane zinc-containing endopeptidases. ENPEP is involved in the catabolic pathway of the renin-angiotensin system forming angiotensin III, which participates in blood pressure regulation and blood vessel formation. Comparative ENPEP amino acid sequences and structures and ENPEP gene locations were examined using data from several mammalian genome projects. Mammalian ENPEP sequences shared 71-98% identities. Five N-glycosylation sites were conserved for all mammalian ENPEP proteins examined although 9-18 sites were observed, in each case. Sequence alignments, key amino acid residues and predicted secondary and tertiary structures were also studied, including transmembrane and cytoplasmic sequences and active site residues. Highest levels of human ENPEP expression were observed in the terminal ileum of the small intestine and in the kidney cortex. Mammalian ENPEP genes contained 20 coding exons. The human ENPEP gene promoter and first coding exon contained a CpG island (CpG27) and at least 6 transcription factor binding sites, whereas the 3'-UTR region contained 7 miRNA target sites, which may contribute to the regulation of ENPEP gene expression in tissues of the body. Phylogenetic analyses examined the relationships of mammalian ENPEP genes and proteins, including primate, other eutherian, marsupial and monotreme sources, using chicken ENPEP as a primordial sequence for comparative purposes.

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哺乳动物谷氨酰氨基肽酶基因(ENPEP)和蛋白质:动脉高血压主要诱因的比较研究。
谷氨酰氨肽酶(ENPEP)是哺乳动物内肽酶 M1 家族的成员,属于哺乳动物 II 型整膜含锌内肽酶。ENPEP 参与肾素-血管紧张素系统的分解代谢途径,形成血管紧张素 III,参与血压调节和血管形成。利用几个哺乳动物基因组项目的数据,研究了ENPEP氨基酸序列和结构的比较以及ENPEP基因的位置。哺乳动物的ENPEP序列具有71-98%的相同性。在所研究的所有哺乳动物ENPEP蛋白中,5个N-糖基化位点是保守的,尽管在每种情况下都观察到9-18个位点。此外,还研究了序列比对、关键氨基酸残基以及预测的二级和三级结构,包括跨膜序列、胞质序列和活性位点残基。在小肠末端回肠和肾皮质中观察到了最高水平的人类ENPEP表达。哺乳动物的ENPEP基因包含20个编码外显子。人类ENPEP基因启动子和第一个编码外显子含有一个CpG岛(CpG27)和至少6个转录因子结合位点,而3'-UTR区域含有7个miRNA靶位点,这些位点可能有助于调控ENPEP基因在身体组织中的表达。系统发育分析研究了哺乳动物ENPEP基因和蛋白质的关系,包括灵长类、其他有蹄类、有袋类和单脊类动物,并以鸡的ENPEP基因作为原始序列进行比较。
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