Second harmonic imaging of membrane potential of neurons with retinal

We present a method to optically measure and image the membrane potential of neurons, using the nonlinear optical phenomenon of second harmonic generation (SHG) with a photopigment retinal as the chromophore [second harmonic retinal imaging of membrane potential (SHRIMP)]. We show that all-trans ret...

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Published inJournal of biomedical optics Vol. 9; no. 5; p. 873
Main Authors Nemet, Boaz A, Nikolenko, Volodymyr, Yuste, Rafael
Format Journal Article
LanguageEnglish
Published United States 01.09.2004
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Abstract We present a method to optically measure and image the membrane potential of neurons, using the nonlinear optical phenomenon of second harmonic generation (SHG) with a photopigment retinal as the chromophore [second harmonic retinal imaging of membrane potential (SHRIMP)]. We show that all-trans retinal, when adsorbed to the plasma membrane of living cells, can report on the local electric field via its change in SHG. Using a scanning mode-locked Ti-sapphire laser, we collect simultaneous two-photon excited fluorescence (TPEF) and SHG images of retinal-stained kidney cells and cultured pyramidal neurons. Patch clamp experiments on neurons stained with retinal show an increase of 25% in SHG intensity per 100-mV depolarization. Our data are the first demonstration of optical measurements of membrane potential of mammalian neurons with SHG. SHRIMP could have wide applicability in neuroscience and, by modifying rhodopsin, could in principle be subject for developing genetically engineered voltage sensors.
AbstractList We present a method to optically measure and image the membrane potential of neurons, using the nonlinear optical phenomenon of second harmonic generation (SHG) with a photopigment retinal as the chromophore [second harmonic retinal imaging of membrane potential (SHRIMP)]. We show that all-trans retinal, when adsorbed to the plasma membrane of living cells, can report on the local electric field via its change in SHG. Using a scanning mode-locked Ti-sapphire laser, we collect simultaneous two-photon excited fluorescence (TPEF) and SHG images of retinal-stained kidney cells and cultured pyramidal neurons. Patch clamp experiments on neurons stained with retinal show an increase of 25% in SHG intensity per 100-mV depolarization. Our data are the first demonstration of optical measurements of membrane potential of mammalian neurons with SHG. SHRIMP could have wide applicability in neuroscience and, by modifying rhodopsin, could in principle be subject for developing genetically engineered voltage sensors.
Author Yuste, Rafael
Nikolenko, Volodymyr
Nemet, Boaz A
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  fullname: Yuste, Rafael
BackLink https://www.ncbi.nlm.nih.gov/pubmed/15447008$$D View this record in MEDLINE/PubMed
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Snippet We present a method to optically measure and image the membrane potential of neurons, using the nonlinear optical phenomenon of second harmonic generation...
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StartPage 873
SubjectTerms Animals
Animals, Newborn
Cells, Cultured
Image Enhancement - methods
Kidney - cytology
Kidney - physiology
Membrane Potentials - physiology
Microscopy, Confocal - methods
Neurons - cytology
Neurons - physiology
Patch-Clamp Techniques - methods
Rats
Rats, Sprague-Dawley
Retinaldehyde
Staining and Labeling - methods
Title Second harmonic imaging of membrane potential of neurons with retinal
URI https://www.ncbi.nlm.nih.gov/pubmed/15447008
Volume 9
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