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Research Article
1Southern Illinois University School of Medicine
Submitted 30 April 2009 ; revised 28 September 2009 ; accepted in final form 29 September 2009
Exposure of cells to the adenosine receptor (AR) agonists leads to receptor uncoupling from G proteins and down-regulation of the A1AR. The receptor levels on the cell surface generally recover upon withdrawal of the agonist, due to either translocation of the sequestered A1AR back to plasma membrane or to de novo synthesis of A1AR. To examine the mechanism(s) underlying A1AR down-regulation and recovery, we treated ductus deferens tumor (DDT1 MF-2) cells with the agonist, R-phenylisopropyladenosine (R-PIA), and showed a decrease in membrane A1AR levels by 24 h, which was associated with an unexpected 11-fold increase in A1AR mRNA. Acute exposure of these cells to R-PIA resulted in a rapid translocation of β-arrestin1 to the plasma membrane. Knockdown of β-arrestin1 by short interfering (si) RNA blocked R-PIA-mediated down-regulation of the A1AR, suppressed R-PIA-dependent ERK1/2 and activator protein-1 (AP-1) activity, and reduced the induction of A1AR mRNA. Withdrawal of the agonist following a 24 h exposure resulted in rapid recovery of plasma membrane A1AR. This was dependent on the de novo protein synthesis and on the activity of ERK1/2, but independent of β-arrestin1 and nuclear factor (NF)-
B. Taken together, these data suggest that exposure to A1AR agonist stimulates ERK1/2 activity via β-arrestin1 which subserves receptor uncoupling and down-regulation, in addition to the induction of A1AR expression. We propose that such a pathway ensures both the termination of the agonist signal and recovery by priming the cell for rapid de novo synthesis of A1AR once the drug is terminated.
Adenosine A1 Receptor; Desensitization; β-arrestin1; ERK MAP Kinase
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