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Omar Nelson, Huiping Tu, Tianhua Lei, Mostafa Bentahir, Bart de Strooper, Ilya Bezprozvanny
Published in Volume 117, Issue 5
J Clin Invest. 2007; 117(5):1230–1239 doi:10.1172/JCI30447
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Figure 7
Ca2+ signals in human primary fibroblasts from the FAD patient.

(A) The representative Fura-2 images of BK-induced Ca2+ responses are shown for hFs from symptomatic PS1-A246E FAD patient and for hFs from the unaffected spouse. The Fura-2 340:380 ratios are presented as explained in the Figure 2 legend. (B) The time course of BK-induced Ca2+ signals in representative experiments with hFs and hF-A246E cells. (C) The average basal cytosolic Ca2+ levels (gray bars) and the amplitude of BK-induced Ca2+ responses (black bars) are shown as mean ± SD for hFs and hF-A246E cells (the number of cells analyzed is shown above each set of bars). When compared with hFs, the basal Ca2+ levels were significantly lower and the amplitude of BK-induced Ca2+ response was significantly larger in hF-A246E cells. (D) The time course of IO-induced Ca2+ signals in representative experiments with hFs and hF-A246E cells. (E) The average size of IO-sensitive Ca2+ pool is shown as mean ± SD for hFs and hF-A246E cells (the number of cells analyzed is shown above each bar). When compared with hFs, the size of IO-sensitive Ca2+ pool was significantly larger in hF-A246E cells. (F) Representative ER Ca2+ traces recorded by ER-loaded Mag-Fura-2 in hFs and hF-A246E cells. The cells were loaded with Mag-fura-2 and permeabilized by 10 μM digitonin (DG) in a buffer containing 170 nM Ca2+ and 3 mM ATP. The ER membrane was permeabilized with 5 μM IO in Ca2+-free buffer at the end of the experiment. The Mag-Fura-2 340:380 ratios were converted to [Ca2+ ]ER as described in Methods. (G) The average [Ca2+]ER determined for hFs and hF-A246E cells are shown as mean ± SD (the number of cells analyzed is shown above each bar). When compared with control hFs, the ER Ca2+ concentration was significantly higher in hF-A246E cells. ***P < 0.05 by ANOVA.