Literature DB >> 26158002

Linker length and fusion site composition improve the optical signal of genetically encoded fluorescent voltage sensors.

Arong Jung1, Jessica E Garcia1, Eunha Kim1, Bong-June Yoon2, Bradley J Baker1.   

Abstract

Several genetically encoded fluorescent sensors of voltage were created by systematically truncating the length of the linker sequence between the voltage-sensing domain and the position of the fluorescent protein, Super Ecliptic A227D. In addition to varying the length, the amino acid composition at the fusion site for the fluorescent protein was modified. Both linker length and amino acid composition affected the size and voltage sensitivity of the optical signal. The truncation mutants revealed a potential structural periodicity with a maximum signal three amino acids from the voltage-sensing domain and another maximum 11 amino acids from the voltage-sensing domain. These results confirm that the linker length and composition can fine tune the size and voltage range of the sensor. The potential periodicity suggests that the orientation of the fluorescent protein could be important for improving the signal size implicating dimerization of the fluorescent protein.

Entities:  

Keywords:  fluorescent protein; voltage imaging; voltage sensor

Year:  2015        PMID: 26158002      PMCID: PMC4478964          DOI: 10.1117/1.NPh.2.2.021012

Source DB:  PubMed          Journal:  Neurophotonics        ISSN: 2329-423X            Impact factor:   3.593


  11 in total

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Authors:  Lei Jin; Zhou Han; Jelena Platisa; Julian R A Wooltorton; Lawrence B Cohen; Vincent A Pieribone
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Authors:  François St-Pierre; Jesse D Marshall; Ying Yang; Yiyang Gong; Mark J Schnitzer; Michael Z Lin
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  15 in total

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Review 7.  Toward Better Genetically Encoded Sensors of Membrane Potential.

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8.  Mechanism of ArcLight derived GEVIs involves electrostatic interactions that can affect proton wires.

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9.  Developing Fast Fluorescent Protein Voltage Sensors by Optimizing FRET Interactions.

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10.  Pado, a fluorescent protein with proton channel activity can optically monitor membrane potential, intracellular pH, and map gap junctions.

Authors:  Bok Eum Kang; Bradley J Baker
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