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通过二次离子质谱(SIMS)显微镜直接观察草履虫中巨大的皮质钙区室:可能参与胞吐作用。

Direct visualization of a vast cortical calcium compartment in Paramecium by secondary ion mass spectrometry (SIMS) microscopy: possible involvement in exocytosis.

作者信息

Stelly N, Halpern S, Nicolas G, Fragu P, Adoutte A

机构信息

Laboratoire de Biologie Cellulaire 4 (CNRS, URA 1134), Bâtiment 444, Université Paris-Sud, Orsay, France.

出版信息

J Cell Sci. 1995 May;108 ( Pt 5):1895-909. doi: 10.1242/jcs.108.5.1895.

DOI:10.1242/jcs.108.5.1895
PMID:7657713
Abstract

The plasma membrane of ciliates is underlaid by a vast continuous array of membrane vesicles known as cortical alveoli. Previous work had shown that a purified fraction of these vesicles actively pumps calcium, suggesting that alveoli may constitute a calcium-storage compartment. Here we provide direct confirmation of this hypothesis using in situ visualization of total cell calcium on sections of cryofixed and cryosubstituted cells analyzed by SIMS (secondary ion mass spectrometry) microscopy a method never previously applied to protists. A narrow, continuous, Ca-emitting zone located all along the cell periphery was observed on sections including the cortex. In contrast, Na and K were evenly distributed throughout the cell. Various controls confirmed that emission was from the alveoli, in particular, the emitting zone was still seen in mutants totally lacking trichocysts, the large exocytotic organelles docked at the cell surface, indicating that they make no major direct contribution to the emission. Calcium concentration within alveoli was quantified for the first time in SIMS microscopy using an external reference and was found to be in the range of 3 to 5 mM, a value similar to that for sarcoplasmic reticulum. After massive induction of trichocyst discharge, this concentration was found to decrease by about 50%, suggesting that the alveoli are the main source of the calcium involved in exocytosis.

摘要

纤毛虫的质膜下方是大量连续排列的膜泡,称为皮质泡。先前的研究表明,这些泡的一个纯化组分能主动泵出钙,这表明泡可能构成一个钙储存区室。在这里,我们通过对冷冻固定和冷冻替代细胞切片上的全细胞钙进行原位可视化,利用二次离子质谱(SIMS)显微镜分析,直接证实了这一假设,这种方法以前从未应用于原生生物。在包括皮质的切片上观察到一个狭窄的、连续的、沿细胞周边发射钙的区域。相比之下,钠和钾在整个细胞中均匀分布。各种对照证实发射来自泡,特别是在完全缺乏刺丝泡(停靠在细胞表面的大型胞吐细胞器)的突变体中仍能看到发射区,这表明它们对发射没有主要的直接贡献。在SIMS显微镜下,首次使用外部参考对泡内的钙浓度进行了定量,发现其范围为3至5 mM,与肌浆网的值相似。在大量诱导刺丝泡释放后,发现该浓度下降了约50%,这表明泡是胞吐作用中钙的主要来源。

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