Abstract
The calyx-type synapse of chick ciliary ganglion (CG) has been intensively studied for decades as a model system for the synaptic development, morphology and physiology. Despite recent advances in optogenetics probing and/or manipulation of the elementary steps of the transmitter release such as membrane depolarization and Ca2+ elevation, the current gene-manipulating methods are not suitable for targeting specifically the calyx-type presynaptic terminals. Here, we evaluated a method for manipulating the molecular and functional organization of the presynaptic terminals of this model synapse. We transfected progenitors of the Edinger-Westphal (EW) nucleus neurons with an EGFP expression vector by in ovo electroporation at embryonic day 2 (E2) and examined the CG at E8-14. We found that dozens of the calyx-type presynaptic terminals and axons were selectively labeled with EGFP fluorescence. When a Brainbow construct containing the membrane-tethered fluorescent proteins m-CFP, m-YFP and m-RFP, was introduced together with a Cre expression construct, the color coding of each presynaptic axon facilitated discrimination among inter-tangled projections, particularly during the developmental re-organization period of synaptic connections. With the simultaneous expression of one of the chimeric variants of channelrhodopsins, channelrhodopsin-fast receiver (ChRFR), and R-GECO1, a red-shifted fluorescent Ca2+-sensor, the Ca2+ elevation was optically measured under direct photostimulation of the presynaptic terminal. Although this optically evoked Ca2+ elevation was mostly dependent on the action potential, a significant component remained even in the absence of extracellular Ca2+. It is suggested that the photo-activation of ChRFR facilitated the release of Ca2+ from intracellular Ca2+ stores directly or indirectly. The above system, by facilitating the molecular study of the calyx-type presynaptic terminal, would provide an experimental platform for unveiling the molecular mechanisms underlying the morphology, physiology and development of synapses. © 2013 Egawa et al.
Figures
![Figure 3. Ca2+ imaging of the calyx-type presynaptic terminal. A, Schematic structures of injected plasmid vectors, pCAGGS-ChRFR-EGFP (top) and pCAGGS-R-GECO1 (bottom). B, A confocal EGFP image of a calyx-type presynaptic terminal (E14) (optical slicing at 1.99 mm). C, A colorrated image of the DF/F of R-GECO1 immediately after electrical stimulation of the oculomotor nerve in the same optical slice. D, Overlay of B and C. Note that several hotspots are present in the synaptic face of the calyx. Scale bar, 10 mm. E, Time-dependent plots of bulky magnitudes of DF/F ([DF/ F]B). The concentration of the extracellular Ca 2+ was 5 mM (red), 2.5 mM (blue) and 0 mM (green). The oculomotor nerve was electrically stimulated as indicated (arrow). F, Simultaneous recordings of the [DF/F]B (blue) and the EPSC (red). doi:10.1371/journal.pone.0059179.g003](https://s3-eu-west-1.amazonaws.com/com.mendeley.prod.article-extracted-content/images/caf9cdef-9695-3152-a5cf-99150bb60aee/thumbnail-3abcefdc-2c22-47b8-9c9b-0c92b82436ed-1.png)
![Figure 5. The intracellular Ca2+ transient induced by direct optogenetic stimulation of the presynaptic terminal. A, Sample [DF/F]B of R-GECO1 responses evoked either by electrical stimulation of the oculomotor nerve (blue) or by direct photostimulation of the presynaptic terminal (red). The same calyx-type presynaptic terminal in the presence of 4-AP (1 mM). B–D, Quantitative comparison of Ca2+ transients between electrical stimulation and optogenetic stimulation: the peak [DF/F]B (B), time constant of the rising phase (tR, C) and that of the decaying phase (tD, D). Each symbol indicates an individual presynaptic terminal. doi:10.1371/journal.pone.0059179.g005](https://s3-eu-west-1.amazonaws.com/com.mendeley.prod.article-extracted-content/images/caf9cdef-9695-3152-a5cf-99150bb60aee/thumbnail-4d8fe8aa-ca6e-460a-ace8-1275dc93da5a-2.png)
![Figure 6. Optogenetic Ca2+ mobilization. A, Typical [DF/F]B changes in the TTX-treated presynaptic terminal: the response to a single 20 ms laser pulse (blue), the response to a train of laser pulses (10 Hz) for 1 s (red) and the response to electrical stimulation (10 Hz, 1 s) to the oculomotor nerve (black). Each trace is an average of five consecutive records. B, Summary of peak [DF/F]B changes (mean 6 SEM) in the presence of TTX. Each column indicates (from left to right) the response to the train of electrical stimulations (10 Hz, 1 s), the single optical stimulation and the train of optical stimulations (10 Hz, 1 s). **, P,0.01 (n = 8). C, Sample [DF/F]B responses of the same presynaptic terminal as shown in A, but with the extracellular Ca2+ being removed (EGTA, 1 mM). Each trace is an average of five consecutive records. D, The dependence of TTX-resistant [DF/F]B changes (mean 6 SEM) on the extracellular Ca2+ of 5 mM (left) and 0 mM (right): the response to single optical stimulation (left) and the response to a train of electrical stimulations (10 Hz, 1 s) (right). *P,0.05, two-tailed t-test (n = 5). doi:10.1371/journal.pone.0059179.g006](https://s3-eu-west-1.amazonaws.com/com.mendeley.prod.article-extracted-content/images/caf9cdef-9695-3152-a5cf-99150bb60aee/thumbnail-83fc7556-b544-4061-ba86-23df8442cf2d-4.png)
![Figure 7. Involvement of Ca2+ store. A, Typical [DF/F]B response of a calyx to a single 20 ms laser pulse in the cation-free extracellular solution (black), the response with additional xestospongin C (blue), the response with additional dantrolene (red) and the response after repetitive photostimulation with additional thapsigargin (green). Each trace is an average of five consecutive records. B, Summary of peak [DF/F]B changes (mean6 SEM) in the cation-free solution. Each column indicates the relative value to that without any pharmacological reagents. *, P,0.05 (n = 7). C, Sample [DF/F]B responses of the same presynaptic terminal as shown in A, but in response to a train of electrical stimulations (10 Hz, 1 s); without any pharmacological reagents in cation-free solution (black), with additional xestospongin C (blue), with additional dantrolene (red) and after repetitive photostimulation with additional thapsigargin (green). Each trace is an average of five consecutive records. D, Summary of peak [DF/F]B responses to a train of electrical stimulations (10 Hz, 1 s) (mean 6 SEM) in the cation-free solution. Each column indicates the relative value to that without any pharmacological reagents. *, P,0.05 (n = 7). Note in A and C that the artifactual fluorescence was increased during photostimulation after treatment with dantrolene, which emits green-yellow fluorescence [72]. doi:10.1371/journal.pone.0059179.g007](https://s3-eu-west-1.amazonaws.com/com.mendeley.prod.article-extracted-content/images/caf9cdef-9695-3152-a5cf-99150bb60aee/thumbnail-cb53c775-f1ff-4028-b85d-6692713d2796-5.png)
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CITATION STYLE
Egawa, R., Hososhima, S., Hou, X., Katow, H., Ishizuka, T., Nakamura, H., & Yawo, H. (2013). Optogenetic Probing and Manipulation of the Calyx-Type Presynaptic Terminal in the Embryonic Chick Ciliary Ganglion. PLoS ONE, 8(3). https://doi.org/10.1371/journal.pone.0059179
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