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膜电位调节过程中分离的大鼠壁细胞的功能和结构变化。

Functional and structural changes of isolated rat parietal cells during membrane potential modulation.

作者信息

Ostrowski J, Jarosz D, Zych W, Wojciechowski K

机构信息

Department of Gastroenterology, Medical Center of Postgraduate Education, Warsaw, Poland.

出版信息

J Physiol Pharmacol. 1994 Sep;45(3):351-60.

PMID:7841448
Abstract

The present experiments were undertaken to extent our earlier observations (J Physiol Pharmacol 1991, 42, 367-79) relating membrane potential with membrane recycling of parietal cells. Studies were performed in vitro using gastric glands that were isolated through the use of rat stomachs transformed into "everted sacs" and filled with hyperosmolar NaCl-EDTA solution. Acid production was indirectly determined by accumulation of 14C-aminopyrine (AP) and its translocation by measurement of acridine orange fluorescence. H+/K(+)-ATPase activity was assayed by measurement of K(+)-stimulated p-nitrophenylphosphatase (pNPPase) of the proton pump. Morphologic state of parietal cells in relation to their functional activity was observed using electron microscopy. Changes in the membrane potential were obtained by the treatment of gastric glands with protonophore carbonyl cyanide m-chlorophenylhydrazone (CCCP) in the incubation media of different pH. CCCP caused time-dependent decrease in AP accumulation by parietal cells from the medium of pH 6.6 but not that of pH 7.8. pNPPase activity increased in aplical and decreased in tubulovesical membrances prepared from CCCP treated glands which were incubated in the medium being more acidic than cell cytoplasm. Electron microscopic assessment showed morphological transformation of resting parietal cells treated with CCCP in pH 6.6 from nonsecreting to secreting state. CCCP acting in acidic incubation medium also caused the decrease in acridine orange fluorescence in the cytoplasm of parietal cells with some temporary increase of its fluorescence in the lumen o gastric glands. These findings support our hypothesis that changes in parietal cell membrane potential by protonophore CCCP may translocate HCl from tubulovesicles to secretory canaliculi. While the above explanation is suggestive, the exact mechanisms controlling a membrane recycling during the secretory response of parietal cells in vitro remain to be elucidated.

摘要

进行本实验是为了扩展我们早期的观察结果(《生理药理学杂志》1991年,第42卷,第367 - 379页),该结果涉及壁细胞膜电位与膜再循环的关系。实验在体外进行,使用通过将大鼠胃转化为“外翻囊”并填充高渗NaCl - EDTA溶液而分离出的胃腺。通过14C - 氨基比林(AP)的积累及其通过吖啶橙荧光测量的转运来间接测定酸分泌。通过测量质子泵的K⁺刺激的对硝基苯磷酸酶(pNPPase)来测定H⁺/K⁺ - ATP酶活性。使用电子显微镜观察壁细胞与其功能活性相关的形态状态。通过在不同pH的孵育培养基中用质子载体羰基氰化物间氯苯腙(CCCP)处理胃腺来获得膜电位的变化。CCCP导致壁细胞从pH 6.6的培养基中积累的AP随时间减少,但从pH 7.8的培养基中积累的AP则没有减少。在比细胞质更酸性的培养基中孵育的经CCCP处理的腺体制备的顶端膜中,pNPPase活性增加,而在微管泡膜中则降低。电子显微镜评估显示,在pH 6.6条件下用CCCP处理的静息壁细胞从非分泌状态转变为分泌状态。在酸性孵育培养基中起作用的CCCP还导致壁细胞胞质中吖啶橙荧光减少,同时胃腺管腔中其荧光有一些暂时增加。这些发现支持了我们的假设,即质子载体CCCP引起的壁细胞膜电位变化可能将HCl从小管泡转运到分泌小管。虽然上述解释具有启发性,但体外壁细胞分泌反应期间控制膜再循环的确切机制仍有待阐明。

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