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通过共培养细胞中fura-2的荧光成像同时测量单个牛肾上腺嗜铬细胞中的胞质钙和分泌。

Simultaneous measurements of cytosolic calcium and secretion in single bovine adrenal chromaffin cells by fluorescent imaging of fura-2 in cocultured cells.

作者信息

Cheek T R, Jackson T R, O'Sullivan A J, Moreton R B, Berridge M J, Burgoyne R D

机构信息

Agricultural and Food Research Council Unit of Insect Neurophysiology and Pharmacology, Department of Zoology, Cambridge, England.

出版信息

J Cell Biol. 1989 Sep;109(3):1219-27. doi: 10.1083/jcb.109.3.1219.

Abstract

The cytosolic free calcium concentration ([Ca2+]i) and exocytosis of chromaffin granules were measured simultaneously from single, intact bovine adrenal chromaffin cells using a novel technique involving fluorescent imaging of cocultured cells. Chromaffin cell [Ca2+]i was monitored with fura-2. To simultaneously follow catecholamine secretion, the cells were cocultured with fura-2-loaded NIH-3T3t cells, a cell line chosen because of their irresponsiveness to chromaffin cell secretagogues but their large Ca2+ response to ATP, which is coreleased with catecholamine from the chromaffin cells. In response to the depolarizing stimulus nicotine (a potent secretagogue), chromaffin cell [Ca2+]i increased rapidly. At the peak of the response, [Ca2+]i was evenly distributed throughout the cell. This elevation in [Ca2+]i was followed by a secretory response which originated from the entire surface of the cell. In response to the inositol 1,4,5-trisphosphate (InsP3)-mobilizing agonist angiotensin II (a weak secretagogue), three different responses were observed. Approximately 30% of chromaffin cells showed no rise in [Ca2+]i and did not secrete. About 45% of the cells responded with a large (greater than 200 nM), transient elevation in [Ca2+]i and no detectable secretory response. The rise in [Ca2+]i was nonuniform, such that peak [Ca2+]i was often recorded only in one pole of the cell. And finally, approximately 25% of cells responded with a similar Ca2+-transient to that described above, but also gave a secretory response. In these cases secretion was polarized, being confined to the pole of the cell in which the rise in [Ca2+]i was greatest.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

采用一种涉及共培养细胞荧光成像的新技术,同时测量单个完整牛肾上腺嗜铬细胞的胞质游离钙浓度([Ca2+]i)和嗜铬颗粒的胞吐作用。用fura-2监测嗜铬细胞的[Ca2+]i。为了同时追踪儿茶酚胺分泌,将这些细胞与负载fura-2的NIH-3T3t细胞共培养,选择该细胞系是因为它们对嗜铬细胞促分泌剂无反应,但对ATP有较大的Ca2+反应,而ATP与儿茶酚胺从嗜铬细胞中共同释放。对去极化刺激物尼古丁(一种强效促分泌剂)的反应中,嗜铬细胞的[Ca2+]i迅速增加。在反应峰值时,[Ca2+]i均匀分布于整个细胞。[Ca2+]i的这种升高之后是源于细胞整个表面的分泌反应。对肌醇1,4,5-三磷酸(InsP3)动员激动剂血管紧张素II(一种弱促分泌剂)的反应中,观察到三种不同反应。约30%的嗜铬细胞[Ca2+]i无升高且不分泌。约45%的细胞以[Ca2+]i大幅(大于200 nM)、短暂升高做出反应且无可检测的分泌反应。[Ca2+]i的升高不均匀,以至于[Ca2+]i峰值常仅在细胞的一极记录到。最后,约25%的细胞以与上述类似的Ca2+瞬变做出反应,但也有分泌反应。在这些情况下,分泌是极化的,局限于[Ca2+]i升高最大的细胞极。(摘要截短于250词)

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