Literature DB >> 28612034

Effects of laser polarization on responses of the fluorescent Ca2+ indicator X-Rhod-1 in neurons and myelin.

Ileana Micu1, Craig Brideau1, Li Lu1, Peter K Stys1.   

Abstract

Laser-scanning optical microscopes generally do not control the polarization of the exciting laser field. We show that laser polarization and imaging mode (confocal versus two photon) exert a profound influence on the ability to detect [Formula: see text] changes in both cultured neurons and living myelin. With two-photon excitation, increasing ellipticity resulted in a [Formula: see text] reduction in resting X-Rhod-1 fluorescence in homogeneous bulk solution, cell cytoplasm, and myelin. In contrast, varying the angle of a linearly polarized laser field only had appreciable effects on dyes that partitioned into myelin in an ordered manner. During injury-induced [Formula: see text] increases, larger ellipticities resulted in a significantly greater injury-induced signal increase in neurons, and particularly in myelin. Indeed, the traditional method of measuring [Formula: see text] changes using one-photon confocal mode with linearly polarized continuous wave laser illumination produced no appreciable X-Rhod-1 signal increase in ischemic myelin, compared to a robust [Formula: see text] fluorescence increase with two-photon excitation and optimized ellipticity with the identical injury paradigm. This underscores the differences in one- versus two-photon excitation and, in particular, the under-appreciated effects of laser polarization on the behavior of certain [Formula: see text] reporters, which may lead to substantial underestimates of the real [Formula: see text] fluctuations in various cellular compartments.

Entities:  

Keywords:  Ca2+ imaging; confocal; myelin; neuron; polarization; two-photon

Year:  2017        PMID: 28612034      PMCID: PMC5459219          DOI: 10.1117/1.NPh.4.2.025002

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


  35 in total

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Journal:  Physiol Rev       Date:  2001-04       Impact factor: 37.312

2.  Polarization induced control of single and two-photon fluorescence.

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5.  Real-time measurement of free Ca2+ changes in CNS myelin by two-photon microscopy.

Authors:  Ileana Micu; Andrew Ridsdale; Lingqing Zhang; John Woulfe; Jeff McClintock; Christine A Brantner; S Brian Andrews; Peter K Stys
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Journal:  Nat Rev Neurosci       Date:  2017-11-09       Impact factor: 34.870

2.  Orthogonally-polarized excitation for improved two-photon and second-harmonic-generation microscopy, applied to neurotransmitter imaging with GPCR-based sensors.

Authors:  Mauro Pulin; Kilian E Stockhausen; Olivia A Masseck; Martin Kubitschke; Björn Busse; J Simon Wiegert; Thomas G Oertner
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  3 in total

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