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Improved two-photon imaging of living neurons in brain tissue through temporal gating
Author(s) -
Vini Gautam,
J C Drury,
Julian M. C. Choy,
Christian Stricker,
HansA. Bachor,
Vincent R. Daria
Publication year - 2015
Publication title -
biomedical optics express
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.362
H-Index - 86
ISSN - 2156-7085
DOI - 10.1364/boe.6.004027
Subject(s) - gating , fluorescence , signal (programming language) , femtosecond , optics , frequency resolved optical gating , fluorescence lifetime imaging microscopy , materials science , two photon excitation microscopy , sampling (signal processing) , photon , pulse (music) , physics , laser , femtosecond pulse shaping , biophysics , computer science , biology , detector , programming language
We optimize two-photon imaging of living neurons in brain tissue by temporally gating an incident laser to reduce the photon flux while optimizing the maximum fluorescence signal from the acquired images. Temporal gating produces a bunch of ~10 femtosecond pulses and the fluorescence signal is improved by increasing the bunch-pulse energy. Gating is achieved using an acousto-optic modulator with a variable gating frequency determined as integral multiples of the imaging sampling frequency. We hypothesize that reducing the photon flux minimizes the photo-damage to the cells. Our results, however, show that despite producing a high fluorescence signal, cell viability is compromised when the gating and sampling frequencies are equal (or effectively one bunch-pulse per pixel). We found an optimum gating frequency range that maintains the viability of the cells while preserving a pre-set fluorescence signal of the acquired two-photon images. The neurons are imaged while under whole-cell patch, and the cell viability is monitored as a change in the membrane's input resistance.

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