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内皮源性舒张因子对内皮细胞和平滑肌细胞内钙离子的自分泌和旁分泌作用。通过共培养中的二维图像分析进行鉴定。

Autocrine and paracrine effects of endothelium-derived relaxing factor on intracellular Ca2+ of endothelial cells and vascular smooth muscle cells. Identification by two-dimensional image analysis in coculture.

作者信息

Shin W S, Sasaki T, Kato M, Hara K, Seko A, Yang W D, Shimamoto N, Sugimoto T, Toyo-oka T

机构信息

Second Department of Internal Medicine, Faculty of Medicine, University of Tokyo, Japan.

出版信息

J Biol Chem. 1992 Oct 5;267(28):20377-82.

PMID:1400356
Abstract

To elucidate the effects of endothelium-derived relaxing factor (EDRF) released from vascular endothelial cells (ECs) on handling of intracellular calcium ion (Ca2+i) in ECs themselves and vascular smooth muscle cells (VSMCs), we measured the Ca2+i by two-dimensional digital image analysis of fura-2-loaded ECs and VSMCs in tissue culture. In isoculture of one cell type, adenosine triphosphate (ATP, 1 microM) transiently increased the Ca2+i of both ECs and VSMCs. High-K+ depolarization or angiotensin II also elevated the Ca2+i of VSMCs, whereas neither stimulants changed the Ca2+i of ECs. In coculture of ECs with VSMCs, the same dose of ATP rapidly increased the Ca2+i of ECs and then transiently decreased the Ca2+i of VSMCs to below the resting level. The maximal Ca2+i-modulating effects of ATP on both cell types were reproducible after the second application of ATP. Three kinds of EDRF blockers (L-NG-monomethylarginine, methemoglobin, or methylene blue) potentiated the ATP-induced Ca2+i rise in ECs and attenuated the Ca2+i reduction in VSMCs, suggesting the autocrine and paracrine effects of EDRF on ECs and VSMCs, respectively. However, neither indomethacin, superoxide dismutase, nor neutralizing monoclonal antibody to endothelin-1 altered the second responses. Thus, two-dimensional Ca2+i image analysis of ECs and VSMCs in coculture enabled direct visualization of the EDRF actions in ECs and VSMCs and their modifications.

摘要

为了阐明血管内皮细胞(ECs)释放的内皮源性舒张因子(EDRF)对ECs自身以及血管平滑肌细胞(VSMCs)内钙离子(Ca2+i)处理的影响,我们通过二维数字图像分析,对组织培养中负载fura-2的ECs和VSMCs的Ca2+i进行了测量。在单一细胞类型的同培养中,三磷酸腺苷(ATP,1 microM)可使ECs和VSMCs的Ca2+i短暂升高。高钾去极化或血管紧张素II也可使VSMCs的Ca2+i升高,而这两种刺激物均未改变ECs的Ca2+i。在ECs与VSMCs的共培养中,相同剂量的ATP可迅速升高ECs的Ca2+i,然后使VSMCs的Ca2+i短暂降低至静息水平以下。第二次施加ATP后,ATP对两种细胞类型的最大Ca2+i调节作用具有可重复性。三种EDRF阻断剂(L-NG-单甲基精氨酸、高铁血红蛋白或亚甲蓝)增强了ATP诱导的ECs中Ca2+i的升高,并减弱了VSMCs中Ca2+i的降低,这分别提示了EDRF对ECs和VSMCs的自分泌和旁分泌作用。然而,吲哚美辛、超氧化物歧化酶或抗内皮素-1的中和单克隆抗体均未改变第二次反应。因此,共培养中ECs和VSMCs的二维Ca2+i图像分析能够直接观察到EDRF在ECs和VSMCs中的作用及其修饰。

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