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Analysis of purine receptor expression and functionality in alveolar epithelial cells. | LitMetric

AI Article Synopsis

  • The alveolar epithelium plays a crucial role in gas exchange and serves as an immune barrier, releasing cytokines and surfactant to maintain lung health.
  • Extracellular ATP from alveolar epithelial cells activates purine receptors (P2Rs) and is essential for lung function, but preparing primary isolated type II alveolar epithelial cells (piAECs) is complicated and involves animal sacrifice.
  • This study analyzed the expression and functionality of P2Rs in piAECs compared to immortalized and tumor-derived AEC lines, revealing that while all cell lines expressed P2Y and P2X, only L2 and piAECs showed functional P2XR activity.

Article Abstract

Despite its fundamental role in providing an extensive surface for gas exchange, the alveolar epithelium (AE) serves as an immunological barrier through, e.g., the release of proinflammatory cytokines and secretion of surfactant to prevent alveolar collapse. Thus, AE is important for sustaining lung homeostasis. Extracellular ATP secreted by alveolar epithelial cells (AECs) is involved in physiological and pathological conditions and acts mainly through the activation of purine receptors (P2Rs). When studying P2R-mediated processes, primary isolated type II AECs (piAECs) still represent the gold standard in in vitro research, although their preparation is time-consuming and requires the sacrifice of many animals. Hence, cultivated immortalized and tumor-derived AEC lines may constitute a valuable alternative. In this work, we examined P2R expression and functionality in piAECs, in immortalized and tumor-derived AEC lines with the purpose of gaining a better understanding of purinergic signaling in different cell systems and assisting researchers in the choice of a suitable cell line with a certain P2R in demand. We combined mRNA and protein analysis to evaluate the expression of P2R. For pharmacological testing, we conducted calcium ([Ca]) measurements and siRNA receptor knockdown. Interestingly, the mRNA and protein levels of P2Y, P2Y and P2X were detected on all cell lines. Concerning functionality, P2XR could be narrowed to L2 and piAECs while P2YR were active in all cell lines.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7367966PMC
http://dx.doi.org/10.1007/s11302-020-09696-0DOI Listing

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