2011
DOI: 10.1007/s10895-011-0965-5
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Label-Free Spatial Analysis of Free and Enzyme-Bound NAD(P)H in the Presence of High Concentrations of Melanin

Abstract: The analysis of autofluorescence, often regarded as undesired noise during the imaging of biological samples, allows label free, unbiased detection of NAD(P)H and melanin in native samples. Because both the emission and absorption spectra of these fluorophores overlap and they can hence not be differentiated using emission filters or with different excitation wavelengths, fluorescence lifetime imaging microscopy (FLIM) is used to differentiate between them. In the present paper the application of two-photon ex… Show more

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Cited by 12 publications
(14 citation statements)
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“…Another strategy uses offline techniques to measure and characterize the general autofluorescence signature of selected bioaerosol types. In some studies fluorescence microscopy is used to understand general fluorescence patterns and fluorophore locations in bioaerosol proxies (e.g., Roshchina et al, 2004;Herbrich et al, 2012). Other studies have applied fluorescence spectroscopy to understand characteristic emission signatures (e.g., O'Connor et al, 2011).…”
Section: Autofluorescence In Bioaerosol Detectionmentioning
confidence: 99%
“…Another strategy uses offline techniques to measure and characterize the general autofluorescence signature of selected bioaerosol types. In some studies fluorescence microscopy is used to understand general fluorescence patterns and fluorophore locations in bioaerosol proxies (e.g., Roshchina et al, 2004;Herbrich et al, 2012). Other studies have applied fluorescence spectroscopy to understand characteristic emission signatures (e.g., O'Connor et al, 2011).…”
Section: Autofluorescence In Bioaerosol Detectionmentioning
confidence: 99%
“…The fluorescence lifetime of most biofluorophores, serving as targets for bioaerosol detection, are usually below 10 ns (e.g., Chorvat & Chorvatova, 2009;Herbrich, et al, 2012;O'Connor et al, 2014;Richards-Kortum & Sevick-Muraca, 1996). However, by choosing xenon lamps as excitation source, recording relevant fluorescence lifetimes in this ns range is hampered by the relatively long decay time of the xenon lamp excitation pulse (~1.5 µs).…”
Section: Spectrally Resolved Fluorescence Detectionmentioning
confidence: 99%
“…The latest WIBS model is currently the WIBS-NEO, whose design is based on a WIBS-4A but with an extended particle size detection range between ∼ 500 nm and 30 µm (nominal). Both UV-APS and WIBS models have been examined in a variety of laboratory validations (e.g., Agranovski et al, 2003Agranovski et al, , 2004Brosseau et al, 2000;Healy et al, 2012;Hernandez et al, 2016;Kanaani et al, 2007;O'Connor et al, 2013;Saari et al, 2013Saari et al, , 2014Savage et al, 2017;Toprak and Schnaiter, 2013) and have been deployed to investigate both indoor and outdoor atmospheric aerosol via longer-term measurements (e.g., Bhangar et al, 2014;Calvo et al, 2018;Crawford et al, 2016;Fernández-Rodríguez et al, 2018;Foot et al, 2008;Gabey et al, 2010Gabey et al, , 2013Gosselin et al, 2016;Healy et al, 2014;Huffman et al, 2010Huffman et al, , 2012Ma et al, 2019;Perring et al, 2015;Schumacher et al, 2013;Twohy et al, 2016;Ziemba et al, 2016).…”
Section: Introductionmentioning
confidence: 99%
“…For example, the quantification of PBAPs by LIF instruments is hindered by the fact that some biological materials reveal weak fluorescence characteristics that do not rise above detection thresholds (Huffman et al, 2012). In addition to this complication, the detection threshold is not a universally defined parameter and varies for each channel between different units of the same type of instrument (e.g., Hernandez et al, 2016;Savage et al, 2017). Furthermore, the unambiguous spectroscopic characterization of bioparticles is fundamentally challenging because fluorescence spectra of even individual molecules in condensed matter are relatively broad due to radiative decay pathways of excited electrons.…”
Section: Introductionmentioning
confidence: 99%