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人肺组织和培养细胞中的中性金属内肽酶。

Neutral metalloendopeptidase in human lung tissue and cultured cells.

作者信息

Johnson A R, Ashton J, Schulz W W, Erdös E G

出版信息

Am Rev Respir Dis. 1985 Sep;132(3):564-8. doi: 10.1164/arrd.1985.132.3.564.

Abstract

The distribution of a neutral metalloendopeptidase (NEP), or "enkephalinase," in human lung tissue and cultured cells was compared with that of angiotensin I converting enzyme (ACE). The specific activities of NEP and ACE were measured in homogenates of fetal lung tissue and in isolated airways and pulmonary vessels. NEP activity was highest in airway tissue, and ACE activity was highest in isolated vessels. Human endothelial cells from either umbilical veins or pulmonary arteries had high ACE activity (80 to 90 nmol/h/10(6) cells) but only a trace of NEP activity (0.5 to 0.6 nmol/h/10(6) cells). Fibroblasts cultured from human lungs were low in ACE but richer in NEP than cultured endothelial cells. Fibroblasts from human foreskins or caesarean section skin were the richest source of NEP activity (60 to 80 nmol/h/10(6) cells). Immunohistochemical studies confirmed the biochemical assays. As expected, ACE was localized on the luminal surface of blood vessels, with a distribution similar to that of factor VIII antigen, an endothelial marker. In contrast, NEP was localized within the alveolar septa. Cultured endothelial cells stained only weakly for NEP in contrast to cultured fibroblasts. The location of these 2 enzymes in different cells and the differences in peptide substrate specificity suggests that they act sequentially on circulating peptides or those released within microvascular beds.

摘要

将一种中性金属内肽酶(NEP),即“脑啡肽酶”,在人肺组织和培养细胞中的分布与血管紧张素I转换酶(ACE)的分布进行了比较。测定了胎儿肺组织匀浆以及分离出的气道和肺血管中NEP和ACE的比活性。NEP活性在气道组织中最高,而ACE活性在分离出的血管中最高。来自脐静脉或肺动脉的人内皮细胞具有高ACE活性(80至90 nmol/h/10⁶个细胞),但只有微量的NEP活性(0.5至0.6 nmol/h/10⁶个细胞)。从人肺培养的成纤维细胞ACE含量低,但NEP比培养的内皮细胞丰富。来自人包皮或剖腹产皮肤的成纤维细胞是NEP活性最丰富的来源(60至80 nmol/h/10⁶个细胞)。免疫组织化学研究证实了生化分析结果。正如预期的那样,ACE定位于血管腔表面,其分布与内皮标志物因子VIII抗原相似。相反,NEP定位于肺泡隔内。与培养的成纤维细胞相比,培养的内皮细胞对NEP的染色很弱。这两种酶在不同细胞中的定位以及肽底物特异性的差异表明它们依次作用于循环肽或在微血管床内释放的肽。

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