Optogenetic manipulation of neuronal and cardiomyocyte functions in zebrafish using microbial rhodopsins and adenylyl cyclases.

Even though microbial photosensitive proteins have been used for optogenetics, their use should be optimized to precisely control cell and tissue functions in vivo. We exploited Gt CCR4 and Kn ChR, cation channelrhodopsins from algae, Be GC1, a guanylyl cyclase rhodopsin from a fungus, and photoactivated adenylyl cyclases (PACs) from cyanobacteria ( Oa PAC) or bacteria ( b PAC), to control cell functions in zebrafish. Optical activation of Gt CCR4 and Kn ChR in the hindbrain reticulospinal V2a neurons, which are involved in locomotion, induced swimming behavior at relatively short latencies, whereas activation of Be GC1 or PACs achieved it at long latencies. Activation of Gt CCR4 and Kn ChR in cardiomyocytes induced cardiac arrest, whereas activation of b PAC gradually induced bradycardia. Kn ChR activation led to an increase in intracellular Ca 2+ in the heart, suggesting that depolarization caused cardiac arrest. These data suggest that these optogenetic tools can be used to reveal the function and regulation of zebrafish neurons and cardiomyocytes.