Siroky Brian J, Ferguson William B, Fuson Amanda L, Xie Yi, Fintha Attila, Komlosi Peter, Yoder Bradley K, Schwiebert Erik M, Guay-Woodford Lisa M, Bell P Darwin
Department of Physiology, Univ. of Alabama at Birmingham, Birmingham, AL, USA.
Am J Physiol Renal Physiol. 2006 Jun;290(6):F1320-8. doi: 10.1152/ajprenal.00463.2005. Epub 2006 Jan 5.
Recent genetic analysis has identified a pivotal role of primary cilia in the pathogenesis of polycystic kidney disease (PKD). However, little is known regarding how cilia loss/dysfunction contributes to cyst development. In epithelial cells, changes in apical fluid flow induce cilia-mediated Ca2+ entry via polycystin-2 (PC2), a cation channel. The Oak Ridge Polycystic Kidney (orpk) mouse contains a mutated Tg737 gene that disrupts expression of polaris, a protein required for ciliogenesis. These studies examine the effect of cilia malformation on Ca2+ entry in orpk cilia(-) collecting duct principal cells, and in orpk cells in which wild-type Tg737 was reintroduced, orpk cilia(+). [Ca2+]i was monitored in confluent cell monolayers using fluorescence microscopy. Intrinsic apical Ca2+ entry was measured by Mn2+ quenching and Ca2+ depletion/readdition under flow conditions below the threshold for stimulation. We found that unstimulated apical Ca2+ entry was markedly increased in cilia(-) cells and was sensitive to Gd3+, an inhibitor of PC2. Electrophysiological measurements demonstrate increased abundance of an apical channel, consistent with PC2, in cilia(-) cells. Immunofluorescence studies revealed that PC2, normally expressed on and at the base of cilia in orpk cilia(+) cells, was observed throughout the apical membrane in cilia(-) cells. Furthermore, cilia(-) cells displayed elevated subapical Ca2+ levels measured with the near-membrane Ca2+ indicator FFP-18. We propose that cilia exert a tonic regulatory influence on apical Ca2+ entry, and absence of cilia results in loss of spatial organization of PC2, causing unregulated Ca2+ entry and elevations in subapical [Ca2+], a factor which may contribute to cyst formation.
最近的基因分析已确定初级纤毛在多囊肾病(PKD)发病机制中起关键作用。然而,关于纤毛缺失/功能障碍如何导致囊肿形成知之甚少。在上皮细胞中,顶端液流的变化通过阳离子通道多囊蛋白-2(PC2)诱导纤毛介导的Ca2+内流。橡树岭多囊肾(orpk)小鼠含有突变的Tg737基因,该基因破坏了纤毛发生所需的蛋白质极地蛋白的表达。这些研究考察了纤毛畸形对orpk纤毛缺失(-)的集合管主细胞以及重新引入野生型Tg737的orpk细胞(orpk纤毛(+))中Ca2+内流的影响。使用荧光显微镜在汇合的细胞单层中监测细胞内Ca2+浓度([Ca2+]i)。在低于刺激阈值的流动条件下,通过Mn2+淬灭以及Ca2+耗竭/再添加来测量内在的顶端Ca2+内流。我们发现,在纤毛缺失(-)的细胞中,未受刺激的顶端Ca2+内流显著增加,并且对PC2抑制剂Gd3+敏感。电生理测量表明,在纤毛缺失(-)的细胞中,一种与PC2一致的顶端通道丰度增加。免疫荧光研究显示,PC2通常在orpk纤毛(+)细胞的纤毛上及其基部表达,而在纤毛缺失(-)的细胞中,在整个顶端膜上都能观察到。此外,用近膜Ca2+指示剂FFP-18测量发现,纤毛缺失(-)的细胞顶端下Ca2+水平升高。我们提出,纤毛对顶端Ca2+内流发挥着紧张性调节作用,纤毛缺失导致PC2空间组织丧失,引起Ca2+内流失控以及顶端下[Ca2+]升高,这可能是导致囊肿形成的一个因素。
