Paper
19 June 2015 Time-resolved and steady-state fluorescence spectroscopy for the assessment of skin photoaging process
Camila de Paula D'Almeida, Carolina Campos, Marcelo Saito Nogueira, Sebastião Pratavieira, Cristina Kurachi
Author Affiliations +
Proceedings Volume 9531, Biophotonics South America; 953146 (2015) https://doi.org/10.1117/12.2180975
Event: SPIE Biophotonics South America, 2015, Rio de Janeiro, Brazil
Abstract
pathology. The optical properties of these intrinsic fluorophores respond to the microenvironment and the metabolic status, thus making fluorescence spectroscopy a valuable tool to study the conditions of biological tissues. The purpose of this study is to investigate the hairless mice skin metabolic changes during the photoaging process through lifetime and fluorescence measurements targeting NADH and FAD. Two lasers centered at 378 nm and 445 nm, respectively, perform excitation of NADH and FAD. The fluorescence acquisition is carried out at mice dorsal and ventral regions throughout the photoaging protocol and aging process. Differences in fluorescence and lifetime data between young and photoaged mice measurements were observed. The endogenous fluorescence spectrum of photoaged dorsal skin showed an increase compared to young and aged skin. Lifetime of bound NADH and free FAD presented an increase in the first week that continued until the end of the protocol. Aging process is being investigated to complement the information obtained from fluorescence data and lifetime of photoaging process.
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Camila de Paula D'Almeida, Carolina Campos, Marcelo Saito Nogueira, Sebastião Pratavieira, and Cristina Kurachi "Time-resolved and steady-state fluorescence spectroscopy for the assessment of skin photoaging process", Proc. SPIE 9531, Biophotonics South America, 953146 (19 June 2015); https://doi.org/10.1117/12.2180975
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Cited by 6 scholarly publications.
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KEYWORDS
Skin

Luminescence

Fluorescence spectroscopy

Tissues

Ultraviolet radiation

Molecules

Ocean optics

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