文化大學機構典藏 CCUR:Item 987654321/19174
English  |  正體中文  |  简体中文  |  Items with full text/Total items : 46867/50733 (92%)
Visitors : 11890231      Online Users : 794
RC Version 6.0 © Powered By DSPACE, MIT. Enhanced by NTU Library IR team.
Scope Tips:
  • please add "double quotation mark" for query phrases to get precise results
  • please goto advance search for comprehansive author search
    •  Adv. Search
    HomeLoginUploadHelpAboutAdminister Goto mobile version


    Please use this identifier to cite or link to this item: https://irlib.pccu.edu.tw/handle/987654321/19174


    Title: Differential Effects of Endothelin-1 on Calcium Mobility in Cultured Porcine Pigment Epithelial Cells of Iris and Retina
    Authors: 吳國揚
    洪秀貞
    馮濟敏
    王惠珠
    Contributors: 生應系
    Keywords: Calcium signaling
    Endothelin-1
    Pigment epithelium of the eye
    Receptors
    endothelin
    Date: 2003-07
    Issue Date: 2011-01-27 11:58:52 (UTC+8)
    Abstract: Background and Purpose: Photoreceptor function depends on an intact retina pigment epithelial (RPE) cell layer. Transplantation of iris pigment epithelial (IPE) cells to the subretinal space offers a potential alternative to RPE transplantation in patients with severe retinal diseases such as macular degeneration. Whether the functions of IPE and RPE are similar or different is not well established. The purpose of this study was to identify the characteristics of IPE cells and RPE cells by detecting the effects of endothelin-1 (ET-1) on intracellular free Ca²+ ([Ca²+]i) mobility in these cells. Methods: Iris and retina pigment epithelial cells were cultured from porcine eyeballs. After the cells were loaded with fura-2/AM, fluorescence was monitored with a fluorescent spectrophotometer by continuously recording excitation signals at 340 nm and 380 nm and emission signals at 510 nm. Results: IPE and RPE cells induced a significant increase in [Ca²+]i under exposure to 10-7, 10-8 and 10-9 mol/L ET-1 in Ca²+ -containing buffer. In the presence of Ca²+-free buffer, ET-1 alone induced an increase in [Ca²+]i in iris but not in retina pigment epithelial cells. In Ca²+-free buffer, pretreatment of the IPE cells with 10-7 mol/L ET-1 partially inhibited thapsigargin-induced [Ca²+]i increase and carbonylcyanide m-chlorophenylhydrazone (CCCP)-induced Ca²+ release. Similarly, pretreatment of the IPE cells with thapsigargin or CCCP also partially inhibited ET-1-induced [Ca²+]i increase. The [Ca²+]i release induced by 10-7 mol/L ET-1 was not inhibited by the phospholipase C inhibitor U73122. In Ca²+-containing buffer, the ETA receptor antagonist BQ123 and ETB receptor antagonist BQ788 partially inhibited 10-7 mol/L ET-1-induced [Ca²+]i increase in IPE cells. However, BQ123 partially inhibited the 10-7 mol/L ET-1-induced [Ca²+]i increase in RPE cells. Nifedipine partially inhibited 10-7 mol/L ET-1-induced [Ca²+]i increase in both types of pigment cells. Conclusions: These results suggest that iris and retina pigment epithelial cells possess distinguishing characteristics because the ET-1-induced [Ca²+]i increases in theses 2 types of pigment epithelial cells are regulated by distinct mechanisms.
    Relation: Journal of the Formosan Medical Association 102卷7期 P.465-473
    Appears in Collections:[Department of Applied Science of Living & Graduate Institute of Applied Science of Living ] journal articles

    Files in This Item:

    File Description SizeFormat
    index.html0KbHTML521View/Open


    All items in CCUR are protected by copyright, with all rights reserved.

    DSpace Software Copyright © 2002-2004  MIT &  Hewlett-Packard  /   Enhanced by   NTU Library IR team Copyright ©   - Feedback