Integration of G-Protein Coupled Receptor Signaling Pathways for Activation of a Transcription Facto

来源 :基因组、蛋白质组与生物信息学报(英文版) | 被引量 : 0次 | 上传用户:fanrend
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We recently reported the use of a gene-trapping approach to isolate cell clones in which a reporter gene had integrated into genes modulated by T-cell activation. We have now tested a panel of clones from that report and identified the one that responds to a variety of G-protein coupled receptors (GPCR). The βlactamase tagged EGR-3 Jurkat cell was used to dissect specific GPCR signaling in vivo. Three GPCRs were studied, including the chemokine receptor CXCR4 (Gicoupled) that was endogenously expressed, the platelet activation factor (PAF) receptor (Gq-coupled), andβ2 adrenergic receptor (Gs-coupled) that was both stably transfected. Agonists for each receptor activated transcription of theβ-lactamase tagged EGR-3 gene. Induction of EGR-3 through CXCR4 was blocked by pertussis toxin and PD58059, a specific inhibitor of MEK (MAPK/ERK kinase). Neither of these inhibitors blocked isoproterenol or PAF-mediated activation of EGR-3. Conversely, β2- and PAF-mediated EGR-3 activation was blocked by the p38, specific inhibitor SB580. In addition, bothβ2- and PAF-mediated EGR-3 activation could be synergistically activated by CXCR4 activation. This combined result indicates that EGR-3 can be activated through distinct signal transduction pathways by different GPCRs and that signals can be integrated and amplified to efficiently tune the level of activation.
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