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P2 receptor regulation of [Ca2+]i in cultured mouse mesangial cells.

Authors :: Rivera, Ian
Shali Zhang
Fuller, B. Scott
Edwards, Brentan
Tsugio Seki
Mong-heng Wang
Marrero, Mario B.
Inscho, Edward W.
Source :: American Journal of Physiology: Renal Physiology; May2007, Vol. 292, pF1380-F1389, 10p, 3 Diagrams, 3 Charts, 6 Graphs
Publication Year :: 2007
Abstract: Experiments were performed to establish the pharmacological profile of purinoceptors and to identify the signal transduction pathways responsible for increases in intracellular calcium concentration ([Ca<superscript>2+</superscript>]<subscript>i</subscript>) for cultured mouse mesangial cells. Mouse mesangial cells were loaded with fura 2 and examined using fluorescent spectrophotometry. Basal [Ca<superscript>2+</superscript>]<subscript>i</subscript> averaged 102 ± 2 nM (n = 346). One hundred micromolar concentrations of ATP, ADP, 2′,3′-(benzoyl-4-benzoyl)-ATP (BzATP), ATP-γ-S, and UTP in normal Ca<superscript>2+</superscript> medium evoked peak increases in [Ca<superscript>2+</superscript>]<subscript>i</subscript> of 866 ± 111, 236 ± 18, 316 ± 26, 427 ± 37, and 808 ± 73 nM, respectively. UDP or 2-methylthio-ATP (2MeSATP) failed to elicit significant increases in [Ca<superscript>2+</superscript>]<subscript>i</subscript>, whereas identical concentrations of adenosine, AMP, and α,β-methylene ATP (α,β-MeATP) had no detectable effect on [Ca<superscript>2+</superscript>]<subscript>i</subscript>. Removal of Ca<superscript>2+</superscript> from the extracellular medium had no significant effect on the peak increase in [Ca<superscript>2+</superscript>]<subscript>i</subscript> induced by ATP, ADP, BzATP, ATP-γ-S, or UTP compared with normal Ca<superscript>2+</superscript> however, Ca<superscript>2+</superscript>-free conditions did accelerate the rate of decline in [Ca<superscript>2+</superscript>]<subscript>i</subscript> in cells treated with ATP and UTP. [Ca<superscript>2+</superscript>]<subscript>i</subscript> was unaffected by membrane depolarization with 143 mM KCI. Western blot analysis for P2 receptors revealed expression of P2X<subscript>2</subscript>, P2X<subscript>4</subscript>, P2X<subscript>7</subscript>, P2Y<subscript>2</subscript>, and P2Y<subscript>4</subscript> receptors. No evidence of P2X<subscript>1</subscript> and P2X<subscript>3</subscript> receptor expression was detected, whereas RT-PCR analysis reveals mRNA expression for P2X<subscript>1</subscript>, P2X<subscript>2</subscript>, P2X<subscript>3</subscript>, P2X<subscript>4</subscript>, P2X<subscript>7</subscript>, P2Y<subscript>2</subscript>, and P2Y<subscript>4</subscript> receptors. These data indicate that receptor-specific P2 receptor activation increases [Ca<superscript>2+</superscript>]<subscript>i</subscript> by stimulating calcium influx from the extracellular medium and through mobilization of Ca<superscript>2+</superscript> from intracellular stores in cultured mouse mesangial cells. [ABSTRACT FROM AUTHOR]