Literature DB >> 19427524

Laser photolysis of caged compounds at 405 nm: photochemical advantages, localisation, phototoxicity and methods for calibration.

Federico F Trigo1, John E T Corrie, David Ogden.   

Abstract

Rapid, localised photolytic release of neurotransmitters from caged precursors at synaptic regions in the extracellular space is greatly hampered at irradiation wavelengths in the near-UV, close to the wavelength of maximum absorption of the caged precursor, because of inner-filtering by strong absorption of light in the cage solution between the objective and cell. For this reason two-photon excitation is commonly used for photolysis, particularly at multiple points distributed over large fields; or, with near-UV, if combined with local perfusion of the cage. These methods each have problems: the small cross-sections of common cages with two-photon excitation require high cage concentrations and light intensities near the phototoxic limit, while local perfusion gives non-uniform cage concentrations over the field of view. Single-photon photolysis at 405 nm, although less efficient than at 330-350 nm, with present cages is more efficient than two-photon photolysis. The reduced light absorption in the bulk cage solution permits efficient wide-field uncaging at non-toxic intensities with uniform cage concentration. Full photolysis of MNI-glutamate with 100 micros pulses required intensities of 2 mW microm(-2) at the preparation, shown to be non-toxic with repeated exposures. Light scattering at 405 nm was estimated as 50% at 18 microm depth in 21-day rat cerebellum. Methods are described for: (1) varying the laser spot size; (2) photolysis calibration in the microscope with the caged fluorophore NPE-HPTS over the wavelength range 347-405 nm; and (3) determining the point-spread function of excitation. Furthermore, DM-Nitrophen photolysis at 405 nm was efficient for intracellular investigations of Ca2+-dependent processes.

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Year:  2009        PMID: 19427524     DOI: 10.1016/j.jneumeth.2009.01.032

Source DB:  PubMed          Journal:  J Neurosci Methods        ISSN: 0165-0270            Impact factor:   2.390


  35 in total

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2.  Three-dimensional imaging and photostimulation by remote-focusing and holographic light patterning.

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5.  Readily releasable pool of synaptic vesicles measured at single synaptic contacts.

Authors:  Federico F Trigo; Takeshi Sakaba; David Ogden; Alain Marty
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6.  Superresolving dendritic spine morphology with STED microscopy under holographic photostimulation.

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8.  Selective silencing of individual dendritic branches by an mGlu2-activated potassium conductance in dentate gyrus granule cells.

Authors:  János Brunner; Jeanne Ster; Susan Van-Weert; Tibor Andrási; Máté Neubrandt; Corrado Corti; Mauro Corsi; Francesco Ferraguti; Urs Gerber; János Szabadics
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9.  Holographic photolysis for multiple cell stimulation in mouse hippocampal slices.

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10.  Combining Ca2+ imaging with -glutamate photorelease.

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Journal:  Cold Spring Harb Protoc       Date:  2013-12-01
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