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通过其特征性的细胞质钙离子浓度动态变化和免疫细胞化学染色来鉴定完整分离的胰岛中的α细胞和β细胞。

Identification of alpha- and beta-cells in intact isolated islets of Langerhans by their characteristic cytoplasmic Ca2+ concentration dynamics and immunocytochemical staining.

作者信息

Asada N, Shibuya I, Iwanaga T, Niwa K, Kanno T

机构信息

Medical Sciences Laboratory, Hokkaido University of Education at Asahikawa, Japan.

出版信息

Diabetes. 1998 May;47(5):751-7. doi: 10.2337/diabetes.47.5.751.

Abstract

Ratiometric images of cytoplasmic Ca2+ concentration ([Ca2+]c) in individual cells were recorded simultaneously with a confocal ultraviolet-laser microscope in the Indo-1-loaded islets isolated from mice. After changes in [Ca2+]c in response to glucose or amino acids were recorded, the islet was fixed, permeabilized, and stained by the indirect immunofluorescence method against insulin or glucagon in situ; the individual cells were then identified in the focal plain identical to that used for the [Ca2+]c imaging. Almost all cells identified as insulin-positive (beta-cells) by their distinct immunofluorescence responded to the increase in glucose concentration from 3 to 11 mmol/l with an increase in [Ca2+]c. Major populations of cells (approximately 65%) identified as glucagon-positive (alpha-cells) responded to the addition of arginine (5-10 mmol/l) to 3 mmol/l glucose solution with an increase in [Ca2+]c. About half of the alpha-cells (47.6%) responded to the addition of alanine (5-10 mmol/l) to 3 mmol/l glucose solution with an increase in [Ca2+]c. In contrast, <13% of beta-cells responded to the addition of alanine (5-10 mmol/l) or arginine (5-10 mmol/l) to 3 mol/l glucose with an increase in [Ca2+]c. More than one-fourth of alpha-cells responded with an increase in [Ca2+]c when glucose concentration in perifusion solution was reduced from 11 to 0 mmol/l. These results indicate that [Ca2+]c changes in islet cells stimulated by glucose or amino acid were characteristic of the cell species, at least in the alpha- and beta-cell. This technique provides a useful tool to investigate not only the intracellular signal transduction but also the intercellular signal transmission in the intact islet.

摘要

使用共聚焦紫外激光显微镜,同时记录从小鼠分离的负载Indo-1的胰岛中单个细胞的细胞质Ca2+浓度([Ca2+]c)的比率图像。记录响应葡萄糖或氨基酸刺激后[Ca2+]c的变化后,将胰岛固定、通透处理,并通过间接免疫荧光法原位染色胰岛素或胰高血糖素;然后在与用于[Ca2+]c成像相同的焦平面上识别单个细胞。几乎所有通过其独特免疫荧光被鉴定为胰岛素阳性(β细胞)的细胞,对葡萄糖浓度从3 mmol/l增加到11 mmol/l的反应都是[Ca2+]c增加。被鉴定为胰高血糖素阳性(α细胞)的主要细胞群体(约65%),对向3 mmol/l葡萄糖溶液中添加精氨酸(5 - 10 mmol/l)的反应是[Ca2+]c增加。约一半的α细胞(47.6%)对向3 mmol/l葡萄糖溶液中添加丙氨酸(5 - 10 mmol/l)的反应是[Ca2+]c增加。相比之下,<13%的β细胞对向3 mol/l葡萄糖中添加丙氨酸(5 - 10 mmol/l)或精氨酸(5 - 10 mmol/l)的反应是[Ca2+]c增加。当灌注溶液中的葡萄糖浓度从11 mmol/l降至0 mmol/l时,超过四分之一的α细胞的反应是[Ca2+]c增加。这些结果表明,至少在α细胞和β细胞中,葡萄糖或氨基酸刺激引起的胰岛细胞[Ca2+]c变化具有细胞类型特异性。该技术不仅为研究完整胰岛中的细胞内信号转导,也为研究细胞间信号传递提供了一个有用的工具。

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