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Estimation of intracellular chloride activity in isolated perfused rabbit proximal convoluted tubules using a fluorescent indicator.

机译:使用荧光指示剂估计离体灌注兔近曲小管中细胞内氯化物的活性。

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摘要

The methodology has been developed to measure cell chloride activity by fluorescence microscopy using the chloride-sensitive dye, 6-methoxy-1-(3-sulfonatopropyl)quinolinium (SPQ). SPQ was loaded into cells of the in vitro microperfused rabbit proximal convoluted tubule by a 10 min luminal perfusion with 20 mM SPQ at 38 degrees C. Fluorescence was excited with a broad band excitation filter (340 and 380 nm) and detected with a 435 nm cut-on filter. The signal to background (autofluorescence) ratio was 4.6 +/- 0.6. The halftime for SPQ leakage from cells at 38 degrees C was 8.6 +/- 1.1 min. In suspended tubules, SPQ did not affect O2 consumption significantly. Intracellular SPQ calibration was performed using the ionophores nigericin and tributyltin, high external potassium concentrations, and varying extracellular chloride concentrations. Cell fluorescence was related to intracellular chloride by a Stern-Volmer relation with a quenching constant of 12 M-1. Apparent chloride concentration in tubules perfused with solutions characteristic for the late proximal convoluted tubule was 27.5 +/- 5 mM (activity 20.6 mM). The halftime of the transient in cell chloride activity upon bath chloride addition was approximately 3 s (38 degrees C). Applications and limitations of this new fluorescence method to study cell chloride transport are discussed.
机译:该方法已经开发出来,通过使用氯化物敏感染料6-甲氧基-1-(3-磺酰基丙基)喹啉鎓(SPQ)的荧光显微镜来测量细胞的氯化物活性。通过在38摄氏度下用20 mM SPQ进行10分钟腔内灌注,将SPQ加载到体外微灌流兔近曲管中的细胞中。用宽带激发滤光片(340和380 nm)激发荧光,并用435 nm检测截止过滤器。信号与背景(自发荧光)之比为4.6 +/- 0.6。在38摄氏度时,SPQ从电池泄漏的中途时间为8.6 +/- 1.1分钟。在悬浮管中,SPQ不会显着影响O2的消耗。细胞内SPQ校准使用离子载体尼日尔霉素和三丁基锡,高外部钾浓度和变化的细胞外氯化物浓度进行。细胞荧光与细胞内氯化物通过Stern-Volmer关系相关,猝灭常数为12 M-1。灌注有晚期近曲小管特有溶液的小管中的表观氯化物浓度为27.5 +/- 5 mM(活性20.6 mM)。加入浴氯化物后,细胞氯化物活性瞬态的半衰期约为3 s(38摄氏度)。讨论了这种新的荧光方法在研究细胞氯化物转运中的应用和局限性。

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