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犬肥大细胞α-糜蛋白酶基因的克隆与表达

Cloning and expression of the dog mast cell alpha-chymase gene.

作者信息

Caughey G H, Blount J L, Koerber K L, Kitamura M, Fang K C

机构信息

Cardiovascular Research Institute and Department of Medicine, University of California, San Francisco 94143-0911, USA.

出版信息

J Immunol. 1997 Nov 1;159(9):4367-75.

PMID:9379034
Abstract

Chymases are chymotrypsin-like serine proteinases secreted by mast cells. Alpha- and beta-chymases differ in structure, function, and mast cell subset- and species-specific expression. Seeking genetic regulatory elements shared by alpha-chymases, we sequenced the dog alpha-gene. Extensive homology was found in intronic and flanking sequences of the dog, human, and mouse alpha-chymase genes, but little in corresponding beta-chymase sequences. Repetitive elements probably derived from retroposons are unique features of the dog flank. DNA blots suggest that the dog alpha-gene, like its human counterpart, may be the genome's sole chymase, unlike in rodents, in which beta-chymases predominate. Nuclear runoff studies predict that transcriptional mechanisms explain differences in steady state chymase and tryptase mRNA levels between mastocytoma and non-mast cells. In dog BR mastocytoma cells incubated with phorbol ester, high steady state levels of alpha-chymase mRNA drop dramatically with little change in tryptase mRNA, whereas dexamethasone decreases expression of both mRNAs. Portions of the dog or human gene 5' flank transfected into BR cells drive expression of a reporter gene and define regions with active promoters. Thus, BR cells express high levels of alpha-chymase mRNA regulated independently of tryptase and support transcription using dog or human promoters. These studies reinforce the alphabeta-chymase dichotomy and suggest the utility of BR cells in probing regulation of alpha-chymase expression.

摘要

糜蛋白酶是肥大细胞分泌的类胰凝乳蛋白酶丝氨酸蛋白酶。α-糜蛋白酶和β-糜蛋白酶在结构、功能、肥大细胞亚群及物种特异性表达方面存在差异。为寻找α-糜蛋白酶共有的基因调控元件,我们对犬α-基因进行了测序。在犬、人及小鼠α-糜蛋白酶基因的内含子和侧翼序列中发现了广泛的同源性,但在相应的β-糜蛋白酶序列中同源性较低。可能源自反转录转座子的重复元件是犬侧翼序列的独特特征。DNA印迹分析表明,与人类的情况类似,犬α-基因可能是基因组中唯一的糜蛋白酶基因,这与啮齿动物不同,在啮齿动物中β-糜蛋白酶占主导。核转录分析预测,转录机制可解释肥大细胞瘤细胞与非肥大细胞之间稳态糜蛋白酶和类胰蛋白酶mRNA水平的差异。在用佛波酯处理的犬BR肥大细胞瘤细胞中,α-糜蛋白酶mRNA的高稳态水平急剧下降,而类胰蛋白酶mRNA变化不大,而地塞米松则降低了两种mRNA的表达。将犬或人类基因5'侧翼的部分序列转染到BR细胞中可驱动报告基因的表达,并确定具有活性启动子的区域。因此,BR细胞高水平表达α-糜蛋白酶mRNA,其表达独立于类胰蛋白酶,并支持使用犬或人类启动子进行转录。这些研究强化了α-和β-糜蛋白酶的二分法,并表明BR细胞在探究α-糜蛋白酶表达调控方面的实用性。

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