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. 2020 Apr 9;7(2):ENEURO.0369-19.2020. doi: 10.1523/ENEURO.0369-19.2020

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Copyright © 2020 Song

This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license, which permits unrestricted use, distribution and reproduction in any medium provided that the original work is properly attributed.

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Figure 5. — Presynaptic infusion of G85R-SOD1-His increased Ca²⁺ levels in the presynaptic terminal. Ratiometric live Ca²⁺ imaging was performed every 30 s after electrophoretic (100 nA current) infusion of a Ca²⁺ indicator, 1 mM fura-2 in 100 mM KCl, into the presynaptic axon through the first presynaptic stimulation electrode inserted into the palm (Fig. 1A). Fura-2 injection continued for 10 min, and the synapse was allowed to equilibrate for 30 min before SOD1 injection through the second electrode to ensure fura-2 was diffused evenly throughout the whole presynaptic terminal at roughly 100 μM. Ratiometric images were taken at Ex360 nm and Ex390 nm assisted by ultra-high-speed wavelength switching λ DG-4/5 xenon arc lamp system. Ratios at various locations (A) were calculated as (fluorescent intensity^360nm)/(fluorescent intensity^390nm) to provide a measure of intracellular Ca²⁺ concentrations. The blue arrow indicates the injection site for SOD1 proteins. 1: palm, 2–6: PreG, 4: infusion site, 7: PreS, an adjacent presynaptic axon branch which is smaller in size. B, G85R-SOD1-His induced Ca²⁺ increases while WT-SOD1-His had no effect on Ca²⁺ concentration. Raw Ca²⁺ concentrations were derived from the equation [Ca²⁺] = $K d ′ (R - R m i n) / (R m a x - R)$ and averaged across 12 WT- and 19 G85R-SOD1-injected presynaptic terminals (PreG) respectively. Kd′, Rmin, and Rmax were calculated from standards as described in Materials and Methods. Although different synapses varied in their baseline Ca²⁺ concentrations, G85R consistently increased [Ca²⁺] at around 60 min after protein injection whereas WT had no effect. C, D, Baseline normalized Ca²⁺ ratio defined as (R₁₂₀ – R₀)/R₀ (R₁₂₀: 60 min after SOD1 injection, R₀: before SOD1 injection) were plotted at four sites for WT (n = 12) and G85R (n = 19). G85R-SOD1 caused increases in [Ca²⁺] at all sites including the palm where Ca²⁺ channels are sparse or absent. The increase in [Ca²⁺] correlated roughly with G85R-SOD1 concentration, with the highest levels at the injection site and lowest in PreS, a smaller presynaptic axonal branch infused with fura-2 at a comparable concentration but with a lower SOD1 concentration due to slower diffusion from the injection site in PreG. E, F, iHFS applied at 30 min after SOD1 injection seemed to restore Ca²⁺ homeostasis in G85R-SOD1-injected synapses (n = 19), and this equilibrium lasted at least 2 h after iHFS, similar to that in WT (n = 12), this suggested the possibility that redistribution of Ca²⁺ is induced by iHFS. As expected, Ca²⁺ levels increased during HFS in synapses infused with either WT or G85R-SOD1 proteins (Extended Data Fig. 5-1).