Large-scale profiling of signalling pathways reveals an asthma specific signature in bronchial smooth muscle cells

Bronchial smooth muscle (BSM) cells from asthmatic patients maintain in vitro a distinct hyper-reactive ("primed") phenotype, characterized by increased release of pro-inflammatory factors and mediators, as well as hyperplasia and/or hypertrophy. This "primed" phenotype helps to...

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Veröffentlicht in:Oncotarget 2016-05, Vol.7 (18), p.25150-25161
Hauptverfasser: Alexandrova, Elena, Nassa, Giovanni, Corleone, Giacomo, Buzdin, Anton, Aliper, Alexander M, Terekhanova, Nadezhda, Shepelin, Denis, Zhavoronkov, Alexander, Tamm, Michael, Milanesi, Luciano, Miglino, Nicola, Weisz, Alessandro, Borger, Pieter
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Sprache:eng
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Zusammenfassung:Bronchial smooth muscle (BSM) cells from asthmatic patients maintain in vitro a distinct hyper-reactive ("primed") phenotype, characterized by increased release of pro-inflammatory factors and mediators, as well as hyperplasia and/or hypertrophy. This "primed" phenotype helps to understand pathogenesis of asthma, as changes in BSM function are essential for manifestation of allergic and inflammatory responses and airway wall remodelling. To identify signalling pathways in cultured primary BSMs of asthma patients and non-asthmatic subjects by genome wide profiling of differentially expressed mRNAs and activated intracellular signalling pathways (ISPs). Transcriptome profiling by cap-analysis-of-gene-expression (CAGE), which permits selection of preferentially capped mRNAs most likely to be translated into proteins, was performed in human BSM cells from asthmatic (n=8) and non-asthmatic (n=6) subjects and OncoFinder tool were then exploited for identification of ISP deregulations. CAGE revealed >600 RNAs differentially expressed in asthma vs control cells (p≤0.005), with asthma samples showing a high degree of similarity among them. Comprehensive ISP activation analysis revealed that among 269 pathways analysed, 145 (p
ISSN:1949-2553
1949-2553
DOI:10.18632/oncotarget.7209