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Ilka Mathar, Rudi Vennekens, Marcel Meissner, Frieder Kees, Gerry Van der Mieren, Juan E. Camacho Londoño, Sebastian Uhl, Thomas Voets, Björn Hummel, An van den Bergh, Paul Herijgers, Bernd Nilius, Veit Flockerzi, Frank Schweda, Marc Freichel
Published in Volume 120, Issue 9
J Clin Invest. 2010; 120(9):3267–3279 doi:10.1172/JCI41348
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Figure 6
Adrenal gland phenotype in Trpm4–/– mice.

Increased rate of acetylcholine-induced catecholamine release from TRPM4-deficient chromaffin cells. (A) Representative examples of H&E-stained adrenal gland sections from WT and Trpm4–/– mice. Scale bars: 100 μm (upper panels) and 20 μm (lower panels). (B) Amplification of Trpm4 and Hprt transcripts by RT-PCR from RNA of cell clusters dissected from the adrenal medulla. neg Trpm4 and neg HPRT indicate amplifications without template cDNA. (C) Representative traces of carbon fiber amperometry and simultaneous measurements of intracellular calcium concentration ([Ca2+]cyt) in chromaffin cells from WT and Trpm4–/– mice. (D) Averaged [Ca2+]cyt before (baseline) and at indicated time points after application of acetylcholine (ACh; 10 μM) in chromaffin cells from WT (n = 9) and Trpm4–/– mice (n = 14). (E) Number of amperometric events under basal conditions during 5 minutes before stimulation in WT (n = 9) and Trpm4–/– (n = 14) chromaffin cells. (F) Box plot (left) and cumulative analysis (right) of amperometric events after stimulation with 10 μM acetylcholine in WT (n = 9) and Trpm4–/– (n = 14) chromaffin cells. *P < 0.01; WT and Trpm4–/– values in the cumulative probability plot are significantly different (Kolmogorov-Smirnov test, P = 0.015).