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3 June 2011 Dynamic staining of bacteria at a single-cell level
Vicente Nuñez, Srigokul Upadhyayula, Adam Lin, Kenny Chau, Valentine I. Vullev
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Proceedings Volume 8018, Chemical, Biological, Radiological, Nuclear, and Explosives (CBRNE) Sensing XII; 80180A (2011) https://doi.org/10.1117/12.884186
Event: SPIE Defense, Security, and Sensing, 2011, Orlando, Florida, United States
Abstract
Bacterial infectious diseases remain one of the major health hazards nation- and worldwide. The expedience of detection and identification of bacterial pathogens determines how early the diagnosis is, and hence, what the treatment and the outcome of the illness would be. As we have previously reported, the dynamics of fluorescence staining provides venues for the development of expedient assays for detection and identification of bacterial species[1]. We measured the kinetics of bacterial staining with cyanine and thioflavin dyes and investigated their photophysical properties. We demonstrated that the pseudo first-order kinetic constants of the fluorescence staining processes have species specificity without contrition dependence. Combining the dynamics of staining with real-time fluorescence microscopy we characterized the fluorescence staining process at the single-cell level with improved sensitivity and contrast.
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Vicente Nuñez, Srigokul Upadhyayula, Adam Lin, Kenny Chau, and Valentine I. Vullev "Dynamic staining of bacteria at a single-cell level", Proc. SPIE 8018, Chemical, Biological, Radiological, Nuclear, and Explosives (CBRNE) Sensing XII, 80180A (3 June 2011); https://doi.org/10.1117/12.884186
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KEYWORDS
Luminescence
Bacteria
Pathogens
Microscopy
Statistical analysis
Biological research
Signal processing
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