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Functional Kir7.1 channels localized at the root of apical processes in rat retinal pigment epithelium.

机译:功能性Kir7.1通道位于大鼠视网膜色素上皮的顶突根部。

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1. The inwardly rectifying K+ channel current (IK(IR)) recorded from isolated retinal pigmented epithelial (RPE) cells showed poor dependence on external K+ ([K+]o) and low sensitivity to block by Ba2+. We examined the molecular identity and specific subcellular localization of the KIR channel in RPE cells. 2. The Kir7.1 channel current heterologously expressed in HEK293T cells (human embryonic kidney cell line) showed identical properties to those of the RPE IK(IR), i.e. poor dependence on [K+]o and low sensitivity to Ba2+ block. 3. Expression of Kir7.1 mRNA and protein was detected in RPE cells by RT-PCR and immunoblot techniques, respectively. 4. Immunohistochemical studies including electron microscopy revealed that the Kir7.1 channel was localized specifically at the proximal roots of the apical processes of RPE cells, where Na+,K+-ATPase immunoreactivity was also detected. 5. The middle-distal portions of apical processes of RPE cells in the intact tissue exhibited immunoreactivity of Kir4.1, a common KIR channel. In the isolated RPE cells, however, Kir4.1 immunoreactivity was largely lost, while Kir7.1 immunoreactivity remained. 6. These data indicate that the only IK(IR) recorded in isolated RPE cells is derived from the functional Kir7.1 channel localized at the root of apical processes. Co-localization with Na+,K+-ATPase suggests that the Kir7.1 channel may provide the pathway for recycling of K+ to maintain pump activity and thus is essential for K+ handling in RPE cells.
机译:1.从孤立的视网膜色素上皮细胞(RPE)记录的向内整流K +通道电流(IK(IR))显示出对外部K +([K +] o)的依赖性差,对Ba2 +的阻滞敏感性低。我们检查了RPE细胞中KIR通道的分子同一性和特定的亚细胞定位。 2.在HEK293T细胞(人类胚胎肾细胞系)中异源表达的Kir7.1通道电流表现出与RPE IK(IR)相同的特性,即,对[K +] o的依赖性差,对Ba2 +阻滞的敏感性低。 3.分别通过RT-PCR和免疫印迹技术检测RPE细胞中Kir7.1 mRNA和蛋白的表达。 4.包括电子显微镜在内的免疫组织化学研究表明,Kir7.1通道专门位于RPE细胞顶突的近端根部,在该处还检测到Na +,K + -ATPase免疫反应性。 5.完整组织中RPE细胞顶突的中远端部分表现出Kir4.1(一种常见的KIR通道)的免疫反应性。然而,在分离的RPE细胞中,Kir4.1免疫反应性大大丧失,而Kir7.1免疫反应性仍然存在。 6.这些数据表明,在分离的RPE细胞中记录的唯一IK(IR)源自位于根尖突根部的功能性Kir7.1通道。与Na +,K + -ATPase的共定位表明,Kir7.1通道可能为K +的循环提供途径,以维持泵的活性,因此对于RPE细胞中K +的处理至关重要。

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