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In Situ Measurement of Airway Surface Liquid K+ Using a Ratioable K+-sensitive Fluorescent Dye

机译:使用比例K +敏感的荧光染料原位测量气道表面液体K +

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摘要

The airway surface liquid (ASL) is the thin fluid layer lining airway surface epithelial cells, whose volume and composition are tightly regulated and may be abnormal in cystic fibrosis (CF). We synthesized a two-color fluorescent dextran to measure ASL [K+], TAC-Lime-dextran-TMR, consisting of a green-fluorescing triazacryptand K+ ionophore-Bodipy conjugate, coupled to dextran, together with a red fluorescing tetramethylrhodamine reference chromophore. TAC-Lime-dextran-TMR fluorescence was K+-selective, increasing >4-fold with increasing [K+] from 0 to 40 mm. In well differentiated human airway epithelial cells, ASL [K+] was 20.8 ± 0.3 mm and decreased by inhibition of the Na+/K+ pump (ouabain), ENaC (amiloride), CF transmembrane conductance regulator (CFTRinh-172), or K+ channels (TEA or XE991). ASL [K+] was increased by forskolin but not affected by Na+/K+/2Cl cotransporter inhibition (bumetanide). Functional and expression studies indicated the involvement of [K+] channels KCNQ1, KCNQ3, and KCNQ5 as determinants of ASL [K+]. [K+] in CF cultures was similar to that in non-CF cultures, suggesting that abnormal ASL [K+] is not a factor in CF lung disease. In intact airways, ASL [K+] was also well above extracellular [K+]: 22 ± 1 mm in pig trachea ex vivo and 16 ± 1 mm in mouse trachea in vivo. Our results provide the first noninvasive measurements of [K+] in the ASL and indicate the involvement of apical and basolateral membrane ion transporters in maintaining a high ASL [K+].
机译:气道表面液(ASL)是衬在气道表面上皮细胞上的薄流体层,其体积和成分受到严格调节,在囊性纤维化(CF)中可能异常。我们合成了一种双色荧光右旋糖酐,用于测量ASL [K + ],TAC-Lime-dextran-TMR,它由绿色发荧光的triazacryptand K + ionophore-Bodipy组成。偶联到葡聚糖的偶联物,以及发荧光的红色四甲基罗丹明参考生色团。 TAC-Lime-葡聚糖-TMR荧光具有K + 选择性,随[K + ]从0到40 mm的增加而增加了4倍以上。在分化良好的人气道上皮细胞中,ASL [K + ]为20.8±0.3 mm,并且由于抑制Na + / K + 而降低泵(哇巴因),ENaC(阿米洛利),CF跨膜电导调节剂(CFTRinh-172)或K + 通道(TEA或XE991)。佛司可林可提高ASL [K + ],但不受Na + / K + / 2Cl -共转运蛋白的影响抑制(布美他尼)。功能和表达研究表明[K + ]通道KCNQ1,KCNQ3和KCNQ5参与了ASL [K + ]的决定因素。 CF培养物中的[K + ]与非CF培养物中的[K + ]相似,这表明异常的ASL [K + ]不是CF肺部疾病的一个因素。在完整的气道中,ASL [K + ]也远高于细胞外[K + ]:离体猪气管为22±1 mm,小鼠气管为16±1 mm体内。我们的结果提供了ASL中[K + ]的首次非侵入性测量,并表明了顶端和基底外侧膜离子转运蛋白在维持高ASL [K + ]中的作用。

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