[No authors listed]
Lysophospholipase1 (LYPLA1) also known as acylâprotein thioesterase1 (APT1) belongs to the superfamily of α/β hydrolase. It has been found to have the properties of a homodimer by manifesting depalmitoylation as well as lysophospholipase activity. LYPLAs are under the control of both microRNAs, miRâ138 and miRâ424. They were observed to be significantly overexpressed in chronic lymphocytic leukemia cells. To date, LYPLAs are the sole enzymes recognized to activate depalmitoylation. In this study, we provide the expression pattern of LYPLA1 in nonâsmall cell lung cancer (NSCLC) using four different NSCLC cell lines. Western blot analysis and RTâPCR were performed to detect the protein expression and mRNA expression of LYPLA1 in NSCLC cell lines. We detected the highest LYPLA1 protein expression level in SPCâAâ1 cells followed by A549 cells, and the highest LYPLA1 mRNA expression level was detected in the SPCâAâ1 cells followed by the H1299 cell line. We found that suppression of LYPLA1 expression using smallâinterfering RNA significantly inhibited proliferation, migration and invasion of the LYPLA1âtransfected NSCLC cells. Furthermore, we explored the involvement of LYPLA1 in the regulation of epithelialâmesenchymal transition (EMT). The epithelial marker Eâcadherin was significantly increased, while mesenchymal markers Nâcadherin, vimentin and SNAIL were markedly decreased in the LYPLA1âsilenced cells. Collectively the results of the present study suggest that the LYPLA1 gene plays a tumorâpromotor role in NSCLC cells in vitro.
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