首页> 美国卫生研究院文献>The Journal of Physiology >K+ and Cl- transport mechanisms in bovine pigment epithelium that could modulate subretinal space volume and composition.
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K+ and Cl- transport mechanisms in bovine pigment epithelium that could modulate subretinal space volume and composition.

机译:牛色素上皮中的K +和Cl-转运机制可调节视网膜下空间的体积和组成。

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摘要

1. Conventional and ion-selective double-barrelled microelectrodes were used in an in vitro bovine retinal pigment epithelium (RPE)-choroid preparation to measure the changes in membrane voltage, resistance and intracellular K+ and Cl- activities produced by small, physiological changes in extracellular potassium ([K+]o). 2. In the intact eye, light-induced changes in [K+]o occur in the extracellular (or subretinal) space that separates the neural retina and the RPE apical membrane. These [K+]o changes can be approximated in vitro by decreasing apical bath [K+]o from 5 to 2 mM. 3. This in vitro change in [K+]o simultaneously decreased intracellular Cl- and K+ activities (aCli and aKi) by 25 +/- 6 mM (n = 8) and 19 +/- 7 mM (n = 4) (mean +/- S.D.), respectively. In control Ringer solution (5 mM [K+]o) aCli and aKi were 65 +/- 10 mM (n = 28) and 65 +/- 8 mM (n = 6), respectively. 4. The [K+]o-induced decreases in aCli and aKi were both significantly inhibited, either by blocking the apical membrane K+ conductance with Ba2+ or the basolateral membrane Cl- conductance with DIDS (4,4'-diisothiocyano-stilbene-2,2'-disulphonic acid). 5. Transepithelial current pulses were used to determine the relative basolateral membrane Cl- conductance, TClBAS, was approximately 0.6 (n = 3), and the relative apical membrane K+ conductance, TKAP, was approximately 0.7 (n = 2). Step changes in basal bath [K+]o were used to estimate the relative basolateral membrane K+ conductance, TKBAS, was approximately 0.34 (n = 3). 6. These data show that the apical membrane K+ conductance and the basolateral membrane Cl- conductance are electrically coupled. In vivo, this coupling could have significant functional importance by modulating the relative hydration of the subretinal space, regulating RPE cell volume, and buffering the chemical composition of the subretinal space.
机译:1.在体外牛视网膜色素上皮(RPE)-脉络膜制剂中使用常规和离子选择性双管微电极,以测量因生理中微小的变化而产生的膜电压,电阻以及细胞内K +和Cl-活性的变化。细胞外钾([K +] o)。 2.在完整的眼睛中,[K +] o的光诱导变化发生在将神经视网膜和RPE顶膜分开的细胞外(或视网膜下)空间。这些[K +] o的变化可以通过将顶浴[K +] o从5 mM降低到2 mM在体外进行估算。 3. [K +] o的这种体外变化同时使细胞内Cl-和K +活性(aCli和aKi)降低25 +/- 6 mM(n = 8)和19 +/- 7 mM(n = 4)(平均值+/- SD)。在对照林格溶液(5 mM [K +] o)中,aCli和aKi分别为65 +/- 10 mM(n = 28)和65 +/- 8 mM(n = 6)。 4. [K +] o诱导的aCli和aKi的降低均被显着抑制,通过用Ba2 +阻断根尖膜K +电导或用DIDS(4,4'-diisothiocyano-stilbene-2, 2'-二磺酸)。 5.使用上皮电流脉冲确定相对基底外侧膜Cl-电导率TC1BAS约为0.6(n = 3),相对顶端膜K +电导率TKAP约为0.7(n = 2)。基底浴[K +] o的阶跃变化用于估计相对基底外侧膜K +电导率TKBAS约为0.34(n = 3)。 6.这些数据表明,顶端膜K +电导和基底外侧膜Cl-电导是电耦合的。在体内,通过调节视网膜下间隙的相对水合作用,调节RPE细胞体积并缓冲视网膜下间隙的化学成分,这种偶联可能具有重要的功能重要性。

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