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器官培养后大鼠肠系膜动脉段中收缩性内皮素-B受体的出现

Appearance of contractile endothelin-B receptors in rat mesenteric arterial segments following organ culture.

作者信息

Adner M, Geary G G, Edvinsson L

机构信息

Department of Internal Medicine, Lund University Hospital, Sweden.

出版信息

Acta Physiol Scand. 1998 Jun;163(2):121-9. doi: 10.1046/j.1365-201X.1998.00369.x.

Abstract

The aim of this study was to examine how different procedures for organ culture affect the expression of contractile endothelin(ET)-B receptors in a branch of the rat mesenteric artery. In fresh segments, ET-1 and ET-3 induced similar strong contractions, ET-1 being 20-fold more potent, whereas neither of the selective ETB receptor agonists, sarafotoxin 6c (S6c) nor IRL 1620, induced significant contractions. In segments cultured for 1 day, ET-3 was only 3-fold less potent as ET-1, and S6c and IRL 1620 induced concentration-dependent contractions which were about 60% of the ET-1 induced contraction. The maximum contractile response to S6c was not altered in segments cultured with foetal calf serum or in buffer solution, but was reduced to about 20% of the control value when cultured in glucose-free buffer solution. The contraction to S6c was abolished in segments placed in cold (4 degrees C) buffer solution. Removal of the endothelium had no effect on the S6c-induced contractions. Arteries cultured at isometric tension (at 2 mN) for 1 day achieved the same contractile response for ETB agonists as resting segments. Pressurized arteries (60 mmHg) did not constrict to S6c when mounted as a fresh segment but demonstrated a strong contraction after 1 day at this transmural pressure. This study suggests that the appearance of ETB receptor mediated contraction following organ culture is not dependent on specific nutrients, endothelial factors or absence of intrinsic tension, but is a metabolically active process.

摘要

本研究的目的是考察不同的器官培养程序如何影响大鼠肠系膜动脉分支中收缩型内皮素(ET)-B受体的表达。在新鲜血管段中,ET-1和ET-3诱导相似的强烈收缩,ET-1的效力比ET-3高20倍,而选择性ETB受体激动剂,即6c型蛙皮素(S6c)和IRL 1620,均未诱导出明显的收缩。在培养1天的血管段中,ET-3的效力仅比ET-1低3倍,且S6c和IRL 1620诱导出浓度依赖性收缩,约为ET-1诱导收缩的60%。在含胎牛血清或缓冲溶液中培养的血管段中,对S6c的最大收缩反应未改变,但在无糖缓冲溶液中培养时,该反应降低至对照值的约20%。置于冷(4℃)缓冲溶液中的血管段对S6c的收缩反应消失。去除内皮对S6c诱导的收缩无影响。在等长张力(2 mN)下培养1天的动脉对ETB激动剂的收缩反应与静息血管段相同。新鲜血管段安装时对S6c无收缩反应,但在60 mmHg跨壁压力下放置1天后,加压动脉(60 mmHg)对S6c表现出强烈收缩。本研究表明,器官培养后ETB受体介导的收缩的出现不依赖于特定营养物质、内皮因子或无内在张力,而是一个代谢活跃的过程。

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