首页> 外文期刊>Peritoneal dialysis international: Journal of the International Society for Peritoneal Dialysis >Expression of aquaporin-1 in the peritoneal tissues: localization and regulation by hyperosmolality.
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Expression of aquaporin-1 in the peritoneal tissues: localization and regulation by hyperosmolality.

机译:aquaporin-1在腹膜组织中的表达:高渗性的定位和调节。

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OBJECTIVE: The purpose of this study was to determine the localization of the aquaporin-1 (AQP1) water channel in peritoneal tissues and the effect of hyperosmolality on the peritoneal expression and function of AQP1. METHODS: Immunohistochemical localization of AQP1 was identified in rat peritoneal tissues. Cultured rat peritoneal mesothelial cells (RPMCs) were exposed to hyperosmolality by adding 4% glucose to the culture medium. After 1 hour, 4 hours, 24 hours, and 48 hours, AQP1 was identified by semiquantitative immunoblot and immunocytochemistry. Osmotic water permeability was measured using a light-scattering method. RESULTS: Immunohistochemistry of rat peritoneal tissues showed the presence of AQP1 in mesothelial cells, venular endothelial cells, and capillary endothelial cells, but not in arteriole and interstitial cells. Semiquantitative immunoblot revealed that exposure to hyperosmolality significantly increased AQP1 expression after 24 hours in whole RPMC lysates (3.3-fold at 24 hours and 3.9-fold at 48 hours). Consistent with the immunoblot, osmotic water permeability of RPMC was augmented 1.7-fold and 2.7-fold after 1 hour and 24 hours, respectively, in a hyperosmotic environment. In RPMC membrane fractions, AQP1 expression was significantly increased after 1 hour of exposure to hyperosmolality (3.9-fold at 1 hour, 7.1-fold at 4 hours, and 8.7-fold at 24 hours). Immunocytochemistry of RPMCs showed that AQP1 was gradually redistributed from the perinuclear area to the peripheral cytoplasm, and then to the plasma membrane after a 1-hour hyperosmotic challenge, suggesting hyperosmolality-induced translocation of AQP1. Upregulation of AQP1 was also observed in the omentum of rats loaded intraperitoneally with hyperosmotic dialysate every day for 10 weeks. CONCLUSION: AQP1 is widely distributed in the peritoneal cavity and may provide the major aqueous pathway across the peritoneal barrier. In addition, our findings suggested that hyperosmolality increases AQP1-dependent water permeability in peritoneal tissues by regulatIng the translocation and synthesis of AQP1 protein.
机译:目的:本研究的目的是确定水通道蛋白1(AQP1)水通道在腹膜组织中的定位以及高渗透压对AQP1腹膜表达和功能的影响。方法:在大鼠腹膜组织中鉴定了AQP1的免疫组织化学定位。通过向培养基中添加4%葡萄糖,使培养的大鼠腹膜间皮细胞(RPMC)暴露于高渗。 1小时,4小时,24小时和48小时后,通过半定量免疫印迹和免疫细胞化学鉴定AQP1。渗透水渗透率是使用光散射法测定的。结果:大鼠腹膜组织的免疫组织化学分析显示,间皮细胞,静脉内皮细胞和毛细血管内皮细胞中存在AQP1,而小动脉和间质细胞中不存在AQP1。半定量免疫印迹显示,在整个RPMC裂解物中24小时后,高渗暴露会显着增加AQP1表达(24小时为3.3倍,48小时为3.9倍)。与免疫印迹一致,在高渗环境中,RPMC的渗透水渗透率分别在1小时和24小时后分别增加了1.7倍和2.7倍。在RPMC膜级分中,暴露于高渗的1小时后AQP1表达显着增加(1小时为3.9倍,4小时为7.1倍,24小时为8.7倍)。 RPMC的免疫细胞化学分析显示,在1小时的高渗攻击后,AQP1从核周区域逐渐重新分布到周围的细胞质,然后再分布到质膜,提示高渗性引起的AQP1易位。每天腹膜内充满高渗透析液的大鼠大网膜中也观察到了AQP1的上调,持续10周。结论:AQP1广泛分布在腹膜腔中,并可能提供穿过腹膜屏障的主要水通道。此外,我们的研究结果表明,高渗透压可通过调节AQP1蛋白的易位和合成来增加腹膜组织中AQP1依赖性的水渗透性。

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