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. 2016 Jul 26;113(32):E4716–E4725. doi: 10.1073/pnas.1605737113

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Fig. 1. — AZ heterogeneity: Those with larger ribbons have more Ca²⁺ channels. (A, Left) Stack of confocal sections covering an exemplary IHC filled with TAMRA-RIBEYE-binding peptide via the patch pipette. (A, Upper Right) Fluo-8FF fluorescence reports Ca²⁺ influx (arrowheads) as spot-like maxima near the membrane during depolarization. (A, Lower Right) Corresponding image of TAMRA-RIBEYE-binding peptide fluorescence labeling synaptic ribbons (arrowheads), where Ca²⁺ influx occurs. White square indicates where the background fluorescence (F_nearby) was measured. (Scale bar: 1 µm.) (B) Measurement of Ca²⁺ influx at individual AZs in an exemplary IHC. Depolarizations to −7 mV (Upper) evoked similar whole-cell Ca²⁺ currents with each stimulus (superimposed, Middle). Focusing on single AZs during each repetition revealed major heterogeneity of maximal Ca²⁺-indicator fluorescence amplitudes (Lower, ΔF₋₇ _mV/F₀, 100-Hz frame rate; panel superimposes one trace per AZ, each marked by a different color). (C) Confocal projections of immunolabeled presynaptic Ca²⁺ channels (Ca_v1.3), presynaptic ribbons (CtBP2/RIBEYE), and postsynaptic AMPA receptors (GluA2) with overlay on far right. (Scale bar: 2 µm.) (D) Green: distribution of the maximal ΔF₋₇ _mV/F₀ for each AZ from live imaging. Blue: distribution of the integrated Ca_v1.3 immunofluorescence pixel intensities for each AZ in fixed tissue. (E) Red: distribution of the maximal fluorescence intensity of TAMRA-peptide labeled ribbons, normalized to the cytosolic fluorescence (F_ribbon/F_nearby). Brown: distribution of the integrated CtBP2/RIBEYE immunofluorescence pixel intensites for each AZ. (F) Distributions of the c.v. estimated within individual IHCs for AZ parameters: maximal Ca²⁺ influx (ΔF₋₇ _mV/F₀, dashed green), TAMRA-RIBEYE-binding peptide fluorescence (solid red), Ca_v1.3 immunofluorescence (solid blue), and CtBP2/RIBEYE immunofluorescence (solid brown). (G) Scatter plot of maximal ΔF₋₇ _mV/F₀ vs. TAMRA-RIBEYE-binding fluorescence intensity (green) and of Ca_v1.3 vs. CtBP2/RIBEYE immunofluorescence (blue). Dashed lines are linear regressions and r is Pearson’s correlation coefficient.