Affiliation:
1. Institute of Biological Information Processing IBI‐3 Forschungszentrum Jülich GmbH 52428 Jülich Germany
2. Faculty of Mathematics Computer Science and Natural Sciences RWTH Aachen University 52062 Aachen Germany
3. Institute of Biological Information Processing IBI‐2 Forschungszentrum Jülich GmbH 52428 Jülich Germany
Abstract
AbstractOptogenetics is a powerful approach in neuroscience research. However, other tissues of the body may benefit from controlled ion currents and neuroscience may benefit from more precise optogenetic expression. The present work constructs three subcellularly‐targeted optogenetic actuators based on the channelrhodopsin ChR2‐XXL, utilizing 5, 10, or 15 tandem repeats (TR) from mucin as N‐terminal targeting motifs and evaluates expression in several polarized and non‐polarized cell types. The modified channelrhodopsin maintains its electrophysiological properties, which can be used to produce continuous membrane depolarization, despite the expected size of the repeats. This work then shows that these actuators are subcellularly localized in polarized cells. In polarized epithelial cells, all three actuators localize to just the lateral membrane. The TR‐tagged constructs also express subcellularly in cortical neurons, where TR5‐ChR2XXL and TR10‐ChR2XXL mainly target the somatodendrites. Moreover, the transfection efficiencies are shown to be dependent on cell type and tandem repeat length. Overall, this work verifies that the targeting motifs from epithelial cells can be used to localize optogenetic actuators in both epithelia and neurons, opening epithelia processes to optogenetic manipulation and providing new possibilities to target optogenetic tools.
Funder
China Scholarship Council
Helmholtz Association