Lee Robert J, Limberis Maria P, Hennessy Michael F, Wilson James M, Foskett J Kevin
Department of Physiology, Division of Medical Genetics, University of Pennsylvania, Philadelphia, PA 19104-6085, USA.
J Physiol. 2007 Aug 1;582(Pt 3):1099-124. doi: 10.1113/jphysiol.2007.131995. Epub 2007 May 24.
Airway submucosal glands are sites of high expression of the cystic fibrosis transmembrane conductance regulator (CFTR) Cl(-) channel and contribute to fluid homeostasis in the lung. However, the molecular mechanisms of gland ion and fluid transport are poorly defined. Here, submucosal gland serous acinar cells were isolated from murine airway, identified by immunofluorescence and gene expression profiling, and used in physiological studies. Stimulation of isolated acinar cells with carbachol (CCh), histamine or ATP was associated with marked decreases in cell volume (20 +/- 2% within 62 +/- 5 s) that were tightly correlated with increases in cytoplasmic Ca(2+) concentration (Ca(2+)) as revealed by simultaneous DIC and fluorescent indicator dye microscopy. Simultaneous imaging of cell volume and the Cl(-)-sensitive fluorophore SPQ indicated that the 20% shrinkage was associated with a fall of Cl(-) from 65 mm to 28 mm, reflecting loss of 67% of cell Cl(-) content, accompanied by parallel efflux of K(+). Upon agonist removal, Ca(2+) relaxed and the cells swelled back to resting volume via a bumetanide-sensitive Cl(-) influx pathway, likely to be NKCC1. Accordingly, agonist-induced serous acinar cell shrinkage and swelling are caused by activation of solute efflux and influx pathways, respectively, and cell volume reflects the secretory state of these cells. In contrast, elevation of cAMP failed to elicit detectible volume responses, or enhance those induced by submaximal [CCh], because the magnitude of the changes were likely to be below the threshold of detection using optical imaging. Finally, when stimulated with cholinergic or cAMP agonists, cells from mice that lacked CFTR, as well as wild-type cells treated with a CFTR inhibitor, exhibited identical rates and magnitudes of shrinkage and Cl(-) efflux compared with control cells. These results provide insights into the molecular mechanisms of salt and water secretion by lung submucosal glands, and they suggest that while murine submucosal gland fluid secretion in response to cholinergic stimulation can originate from CFTR-expressing serous acinar cells, it is not dependent upon CFTR function.
气道黏膜下腺是囊性纤维化跨膜传导调节因子(CFTR)氯离子通道高表达的部位,对肺内液体稳态起作用。然而,腺体离子和液体转运的分子机制尚不清楚。在此,从小鼠气道分离出黏膜下腺浆液性腺泡细胞,通过免疫荧光和基因表达谱进行鉴定,并用于生理学研究。用卡巴胆碱(CCh)、组胺或ATP刺激分离的腺泡细胞,细胞体积显著减小(62±5秒内减小20±2%),这与细胞质钙离子浓度([Ca²⁺]i)升高密切相关,同时的微分干涉对比(DIC)和荧光指示剂染料显微镜检查揭示了这一点。细胞体积和氯离子敏感荧光团SPQ的同步成像表明,20%的细胞收缩与[Cl⁻]i从65 mM降至28 mM有关,反映细胞氯离子含量损失67%,同时伴有钾离子的平行外流。去除激动剂后,[Ca²⁺]i恢复正常,细胞通过布美他尼敏感的氯离子内流途径(可能是NKCC1)肿胀回到静息体积。因此,激动剂诱导的浆液性腺泡细胞收缩和肿胀分别是由溶质外流和内流途径的激活引起的,细胞体积反映了这些细胞的分泌状态。相比之下,环磷酸腺苷(cAMP)升高未能引发可检测到的体积反应,也未增强次最大浓度[CCh]诱导的反应,因为变化幅度可能低于光学成像检测阈值。最后,用胆碱能或cAMP激动剂刺激时,缺乏CFTR的小鼠细胞以及用CFTR抑制剂处理的野生型细胞,与对照细胞相比,表现出相同的收缩率和幅度以及氯离子外流。这些结果为肺黏膜下腺盐和水分泌的分子机制提供了见解,并且表明虽然小鼠黏膜下腺对胆碱能刺激的液体分泌可能起源于表达CFTR的浆液性腺泡细胞,但它不依赖于CFTR功能。