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上皮细胞单层在粘蛋白分泌过程中钙的时间分辨释放。

Time-resolved release of calcium from an epithelial cell monolayer during mucin secretion.

机构信息

Department of Biomedical Engineering, Case School of Engineering, Case Western Reserve University, Cleveland, OH 44106, USA.

出版信息

Eur Biophys J. 2011 Feb;40(2):165-74. doi: 10.1007/s00249-010-0636-5. Epub 2010 Oct 26.

DOI:10.1007/s00249-010-0636-5
PMID:20976596
Abstract

A significant amount of Ca²+ is contained in secretory mucin granules. Exchange of Ca²+ for monovalent cations drives the process of mucin decondensation and hydration after fusion of granules with the plasma membrane. Here we report direct observation of calcium secretion with a Ca²+ ion-selective electrode (ISE) in response to apical stimulation with ATP from HT29-Cl.16E cells, a subclone of the human colonic cancer cell line HT29. No increase in Ca²+ level was seen for the sister cell line Cl.19A, which lacks mucin granules, or for Cl.16E cells after inhibition of granule fusion with wortmannin. Further, the measured concentration was used to estimate the time-resolved rate of release of Ca²+ from the cell monolayer, by use of a deconvolution-based method developed previously (Nair and Gratzl in Anal Chem 77:2875-2881, 2005). The results argue that Ca²+ release by Cl.16E cells is associated specifically with mucin secretion, i.e., that the measured Ca²+ increase in the apical solution is derived from granules after fusion and mucin exocytosis. The Ca²+ ISE in conjunction with deconvolution provides a minimally disturbing method for assessment of Ca²+ secretion rates. The release rates provide estimates of exocytosis rates and, when combined with earlier capacitance measurements, estimates of post-stimulation endocytosis rates also.

摘要

大量的 Ca²+ 存在于分泌粘蛋白颗粒中。Ca²+ 与单价阳离子的交换驱动了粘蛋白去凝聚和水合的过程,该过程发生在颗粒与质膜融合之后。在这里,我们报道了通过 Ca²+ 离子选择性电极 (ISE) 对 HT29-Cl.16E 细胞(人结肠癌细胞系 HT29 的一个亚克隆)的顶端刺激用 ATP 进行钙分泌的直接观察。来自缺乏粘蛋白颗粒的姐妹细胞系 Cl.19A 的细胞或在用渥曼青霉素抑制颗粒融合后的 Cl.16E 细胞均未观察到 Ca²+ 水平的增加。此外,通过使用先前开发的基于解卷积的方法(Nair 和 Gratzl 在 Anal Chem 77:2875-2881, 2005 年),根据测量的浓度来估计细胞单层中 Ca²+ 从细胞中释放的时间分辨速率。结果表明,Cl.16E 细胞的 Ca²+ 释放与粘蛋白分泌特异性相关,即,在顶端溶液中观察到的 Ca²+ 增加是来自融合后的颗粒和粘蛋白胞吐作用。与解卷积相结合的 Ca²+ ISE 提供了一种最小干扰的方法来评估 Ca²+ 分泌速率。释放速率提供了胞吐作用速率的估计值,当与早期的电容测量值结合时,还提供了刺激后内吞作用速率的估计值。

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