De Proost Ian, Brouns Inge, Pintelon Isabel, Timmermans Jean-Pierre, Adriaensen Dirk
Laboratory of Cell Biology and Histology, Department of Veterinary Sciences, University of Antwerp, Groenenborgerlaan 171, BE-2020, Antwerp, Belgium.
Histochem Cell Biol. 2007 Oct;128(4):301-16. doi: 10.1007/s00418-007-0318-2. Epub 2007 Aug 10.
Studying depolarisation induced calcium entry in our recently developed in situ lung slice model for molecular live cell imaging of selectively visualised pulmonary neuroepithelial bodies (NEBs), exemplified the need for information on the localisation of voltage-gated calcium channels (Ca(v)) in lungs in general, and related to sensory airway receptors more specifically. The present study therefore aimed at identifying the expression pattern of all major classes and subtypes of Ca(v) channels, using multiple immunostaining of rat lung cryosections. Ca(v) channel antibodies were combined with antibodies that selectively label NEBs, nerve fibre populations, smooth muscle, endothelium and Clara cells. Ca(v)2.1 (P/Q-type) was the only Ca(v) channel expressed in NEB cell membranes, and appeared to be restricted to the apical membrane of the slender NEB cell processes that reach the airway lumen. Subpopulations of the vagal but not the spinal sensory nerve fibres that contact NEBs showed immunoreactivity (IR) for Ca(v)1.2 (L-type) and Ca(v)2.1. Ca(v)2.3 (R-type) was selectively expressed by the so-called Clara-like cells that cover NEBs only, and appears to be a unique marker to discriminate this epithelial cell type from the much more extensive group of Clara cells in rat airways. The laminar nerve endings of smooth muscle-associated airway receptors (SMARs) revealed IR for both Ca(v)2.1 and Ca(v)2.2 (N-type). More generally, Ca(v)1.2 was seen to be expressed in vascular smooth muscle, Ca(v)2.3 and Ca(v)3.1 (T-type) in bronchial smooth muscle, Ca(v)3.1 and Ca(v)3.2 (T-type) in endothelial cells, and Ca(v)1.3 (L-type) in a limited number of epithelial cells. In conclusion, the present immunocytochemical study has demonstrated that the various subtypes of Ca(v) channels have distinct expression patterns in rat lungs. Special focus on morphologically/neurochemically characterised sensory airway receptors learned us that both NEBs and SMARs present Ca(v) channels. Knowledge of the identification and localisation of Ca(v) channels in airway receptors and surrounding tissues provides a solid basis for interpretation of the calcium mediated activation studied in our ex vivo lung slice model.
在我们最近开发的用于选择性可视化肺神经上皮小体(NEBs)分子活细胞成像的原位肺切片模型中研究去极化诱导的钙内流,例证了总体上需要了解肺中电压门控钙通道(Ca(v))的定位信息,更具体地说,是与气道感觉受体相关的信息。因此,本研究旨在通过对大鼠肺冰冻切片进行多重免疫染色,确定Ca(v)通道所有主要类别和亚型的表达模式。Ca(v)通道抗体与选择性标记NEBs、神经纤维群体、平滑肌、内皮细胞和克拉拉细胞的抗体相结合。Ca(v)2.1(P/Q型)是唯一在NEB细胞膜中表达的Ca(v)通道,且似乎仅限于延伸至气道腔的细长NEB细胞突起的顶端膜。与NEBs接触的迷走神经而非脊髓感觉神经纤维亚群显示出对Ca(v)1.2(L型)和Ca(v)2.1的免疫反应性(IR)。Ca(v)2.3(R型)仅由覆盖NEBs的所谓类克拉拉细胞选择性表达,似乎是区分这种上皮细胞类型与大鼠气道中更广泛的克拉拉细胞群体的独特标志物。平滑肌相关气道受体(SMARs)的层状神经末梢显示出对Ca(v)2.1和Ca(v)2.2(N型)的IR。更普遍地,Ca(v)1.2在血管平滑肌中表达,Ca(v)2.3和Ca(v)3.1(T型)在支气管平滑肌中表达,Ca(v)3.1和Ca(v)3.2(T型)在内皮细胞中表达,Ca(v)1.3(L型)在有限数量的上皮细胞中表达。总之,本免疫细胞化学研究表明,Ca(v)通道的各种亚型在大鼠肺中有不同的表达模式。对形态学/神经化学特征化的气道感觉受体的特别关注使我们了解到NEBs和SMARs都存在Ca(v)通道。了解气道受体和周围组织中Ca(v)通道的鉴定和定位为解释我们在离体肺切片模型中研究的钙介导激活提供了坚实的基础。
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