The Japanese Journal of Pharmacology | |
Effect of Endothelin-1(1-31)on Human Mesangial Cell Proliferation | |
Hiroyuki Fukui2  Masanori Yoshizumi3  Tetsuhiro Hisayama2  Toshiaki Tamaki3  Yuki Suzaki3  Shoji Kagami1  Hitoshi Houchi3  Koichiro Tsuchiya3  | |
[1] Department of Pediatrics,The University of Tokushima School of Medicine,Tokushima 770-8503,Japan;Department of Pharmacology,Faculty of Pharmaceutical Sciences,The University of Tokushima,Tokushima 770-8505,Japan;Department of Pharmacology and The University of Tokushima School of Medicine,Tokushima 770-8503,Japan | |
关键词: Endothelin-1(1-31); Human chymase; Extracellular signal-regulated kinase; Protein kinase C; | |
DOI : 10.1254/jjp.84.146 | |
学科分类:药理学 | |
来源: Nihon Yakuri Gakkai Henshuubu / Japanese Pharmacological Society | |
【 摘 要 】
References(45)Cited-By(11)It was previously found that human chymase cleaves big endothelins(ETs)at the Tyr31−Gly32 bond and produces 31−amino acid ETs(1−31).In the present study, human plasma concentrations of ET−1(1−31)and ET−1 were examined and the effect of synthetic ET−1(1−31)on the proliferation of cultured human mesangial cells(HMCs)was investigated.The proliferative effect of ET−1(1−31)was evaluated from the [3H]−thymidine uptake.The activity of extracellular signal−regulated kinase(ERK)and DNA binding activity of activator protein−1 were determined by using an in−gel kinase assay and gel mobility shift assay, respectively.Immunoreactive ET−1(1−31)was detectable in plasma, but the level was slightly lower than that of ET−1.ET−1(1−31)increased [3H]−thymidine incorporation in HMCs to a degree similar to that induced by ET−1.ET−1(1−31)also activated ERK1/2.Inhibition of protein kinase C and ERK kinase caused a reduction of ET−1(1−31)−induced ERK1/2 activation.The ERK1/2 activation was followed by an increase in transcription factor activator protein−1 DNA binding activity.These findings suggest that ET−1(1−31)is a bioactive peptide in humans and ET−1(1−31)itself stimulates HMC proliferation.
【 授权许可】
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