Abstract
AbstractCalcium mediates many important signals in dendrites. However, the basic transport properties of calcium in dendrites have been difficult to measure: how far and how fast does a local influx of calcium propagate? We developed an all-optical system for simultaneous targeted Ca2+import and concentration mapping. We co-expressed a blue light-activated calcium selective channelrhodopsin, CapChR2, with a far-red calcium sensor, FR-GECO1c, in cultured rat hippocampal neurons, and used patterned optogenetic stimulation to introduce calcium into cells with user-defined patterns of space and time. We determined a mean steady-state length constant for Ca2+transportϕ∼ 5.8 μm, a half-life for return to baselinet1/2∼ 1.7 s, and an effective diffusion coefficientD∼ 20 μm2/s, though there were substantial differences in Ca2+dynamics between proximal and distal dendrites. At high Ca2+concentration, distal dendrites showed nonlinear activation of Ca2+efflux, which we pharmacologically ascribed to the NCX1 antiporter. Genetically encoded tools for all-optical study of Ca2+transport and handling provide a powerful capability for studying this important messenger.
Publisher
Cold Spring Harbor Laboratory