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肾近端小管内吞小泡中ATP依赖的酸化作用的异质性。在无细胞系统中对单个内吞小泡pH值的测量。

Heterogeneity in ATP-dependent acidification in endocytic vesicles from kidney proximal tubule. Measurement of pH in individual endocytic vesicles in a cell-free system.

作者信息

Shi L B, Fushimi K, Bae H R, Verkman A S

机构信息

Department of Medicine, University of California, San Francisco 94143-0532.

出版信息

Biophys J. 1991 Jun;59(6):1208-17. doi: 10.1016/S0006-3495(91)82336-0.

Abstract

Measurement of membrane transport in suspensions of isolated membrane vesicles provides averaged information over a potentially very heterogeneous vesicle population. To examine the regulatory mechanisms for ATP-dependent acidification, methodology was developed to measure pH in individual endocytic vesicles. Endocytic vesicles from proximal tubule apical membrane of rat kidney were labeled in vivo by intravenous infusion of FITC-dextran (9 kD); a microsomal fraction was obtained from dissected renal cortex by homogenization and differential centrifugation. Vesicles were immobilized on a polylysine coated coverglass and imaged at high magnification by a silicon intensified target camera. ATP-dependent acidification was not influenced by endosome immobilization. Endosome pH was determined from the integrated fluorescence intensity of individual labeled vesicles after background subtraction. Calibration studies with high K and nigericin showed nearly identical fluorescence vs. pH curves for different endosomes with a standard deviation for a single pH measurement in a single endosome of approximately 0.2 pH units. In response to addition of 1 mM MgATP in the presence of K and valinomycin, endosome pH decreased from 7.2 to a mean of 6.4 with a unimodal distribution with width at half-maximum of approximately 1 pH unit. The drop in endosome pH increased and the shape of the distribution changed when the time between FITC-dextran infusion and kidney removal was increased from 5 to 20 min. Differences in ATP-dependent acidification could not be attributed to heterogeneity in passive proton conductance. These results establish a direct method to measure pH in single endocytic vesicles and demonstrate remarkable heterogeneity in ATP-dependent acidification which was interpreted in terms of heterogeneity in the number and/or activity of proton pumps at serial stages of endocytosis.

摘要

对分离的膜囊泡悬浮液中的膜转运进行测量,可提供关于潜在非常异质的囊泡群体的平均信息。为了研究ATP依赖性酸化的调节机制,开发了一种方法来测量单个内吞囊泡中的pH值。通过静脉注射异硫氰酸荧光素标记的葡聚糖(9 kD),在体内对大鼠肾近端小管顶膜的内吞囊泡进行标记;通过匀浆和差速离心从解剖的肾皮质中获得微粒体部分。将囊泡固定在聚赖氨酸包被的盖玻片上,并用硅增强靶相机进行高倍成像。内吞体固定不影响ATP依赖性酸化。在扣除背景后,根据单个标记囊泡的积分荧光强度确定内吞体pH值。用高钾和尼日利亚菌素进行的校准研究表明,不同内吞体的荧光与pH曲线几乎相同,单个内吞体单次pH测量的标准差约为0.2 pH单位。在钾离子和缬氨霉素存在的情况下,加入1 mM MgATP后,内吞体pH值从7.2降至平均6.4,呈单峰分布,半峰宽约为1 pH单位。当异硫氰酸荧光素标记的葡聚糖注射与肾切除之间的时间从5分钟增加到20分钟时,内吞体pH值的下降增加,分布形状改变。ATP依赖性酸化的差异不能归因于被动质子传导的异质性。这些结果建立了一种直接测量单个内吞囊泡pH值的方法,并证明了ATP依赖性酸化中存在显著的异质性,这可以根据内吞作用连续阶段质子泵数量和/或活性的异质性来解释。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/69fb/1281201/eacbd4a0971f/biophysj00113-0061-a.jpg

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