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Contribution of P2X7 receptors to adenosine uptake by cultured mouse astrocytes

✍ Scribed by Hiroto Okuda; Youichirou Higashi; Kentaro Nishida; Sadaki Fujimoto; Kazuki Nagasawa


Publisher
John Wiley and Sons
Year
2010
Tongue
English
Weight
471 KB
Volume
58
Category
Article
ISSN
0894-1491

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✦ Synopsis


Abstract

Nucleotides and nucleosides play important roles by maintaining brain homeostasis, and their extracellular concentrations are mainly regulated by ectonucleotidases and nucleoside transporters expressed by astrocytes. Extracellularly applied NAD^+^ prevents astrocyte death caused by excessive activation of poly(ADP‐ribose) polymerase‐1, of which the molecular mechanism has not been fully elucidated. Recently, exogenous NAD^+^ was reported to enter astrocytes via the P2X7 receptor (P2X7R)‐associated channel/pore. In this study, we examined whether the intact form of NAD^+^ is incorporated into astrocytes. A large portion of extracellularly added NAD^+^ was degraded into metabolites such as AMP and adenosine in the extracellular space. The uptake of adenine ring‐labeled [^14^C]NAD^+^, but not nicotinamide moiety‐labeled [^3^H]NAD^+^, showed time‐ and temperature‐dependency, and was significantly enhanced on addition of apyrase, and was reduced by 8‐Br‐cADPR and ARL67156, inhibitors of CD38 and ectoapyrase, respectively, and P2X7R knockdown, suggesting that the detected uptake of [^14^C]NAD^+^ resulted from [^14^C]adenosine acting as a metabolite of [^14^C]NAD^+^. Pharmacological and genetic inhibition of P2X7R with brilliant blue G, KN‐62, oxATP, and siRNA transfection resulted in a decrease of [^3^H]adenosine uptake, and the uptake was also reduced by low concentration of carbenoxolone and pannexin1 selective peptide blocker ^10^panx. Taken together, these results indicate that exogenous NAD^+^ is degraded by ectonucleotidases and that adenosine, as its metabolite, is taken up into astrocytes via the P2X7R‐associated channel/pore. © 2010 Wiley‐Liss, Inc.


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