Collagen Glycation Detected by Its Intrinsic Fluorescence | Zendy

Rhona Muir | Zendy; Shareen Forbes | Zendy; David J. S. Birch | Zendy; Vladislav Vyshemirsky | Zendy; Olaf J. Rolinski | Zendy

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Collagen Glycation Detected by Its Intrinsic Fluorescence

Author(s) -

Rhona Muir,

Shareen Forbes,

David J. S. Birch,

Vladislav Vyshemirsky,

Olaf J. Rolinski

Publication year - 2021

Publication title -

the journal of physical chemistry b

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.864

H-Index - 392

eISSN - 1520-6106

pISSN - 1520-5207

DOI - 10.1021/acs.jpcb.1c05001

Subject(s) - glycation , fluorescence , chemistry , kinetics , biomarker , biophysics , excitation wavelength , biochemistry , optics , biology , receptor , physics , quantum mechanics

Collagen's long half-life (in skin approximately 10 years) makes this protein highly susceptible to glycation and formation of the advanced glycation end products (AGEs). Accumulation of cross-linking AGEs in the skin collagen has several detrimental effects; thus, the opportunity for non-invasive monitoring of skin glycation is essential, especially for diabetic patients. In this paper, we report using the time-resolved intrinsic fluorescence of collagen as a biomarker of its glycation. Contrary to the traditional fluorescence intensity decay measurement at the arbitrarily selected excitation and detection wavelengths, we conducted systematic wavelength- and time-resolved measurements to achieve time-resolved emission spectra. Changes in the intrinsic fluorescence kinetics, caused by both collagen aggregation and glycation, have been detected.

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