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Publication : Visualization of synaptic inhibition with an optogenetic sensor developed by cell-free protein engineering automation.

First Author  Grimley JS Year  2013
Journal  J Neurosci Volume  33
Issue  41 Pages  16297-309
PubMed ID  24107961 Mgi Jnum  J:325762
Mgi Id  MGI:7287838 Doi  10.1523/JNEUROSCI.4616-11.2013
Citation  Grimley JS, et al. (2013) Visualization of synaptic inhibition with an optogenetic sensor developed by cell-free protein engineering automation. J Neurosci 33(41):16297-309
abstractText  We describe an engineered fluorescent optogenetic sensor, SuperClomeleon, that robustly detects inhibitory synaptic activity in single, cultured mouse neurons by reporting intracellular chloride changes produced by exogenous GABA or inhibitory synaptic activity. Using a cell-free protein engineering automation methodology that bypasses gene cloning, we iteratively constructed, produced, and assayed hundreds of mutations in binding-site residues to identify improvements in Clomeleon, a first-generation, suboptimal sensor. Structural analysis revealed that these improvements involve halide contacts and distant side chain rearrangements. The development of optogenetic sensors that respond to neural activity enables cellular tracking of neural activity using optical, rather than electrophysiological, signals. Construction of such sensors using in vitro protein engineering establishes a powerful approach for developing new probes for brain imaging.
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