Literature DB >> 19588156

[Comparison of parameters of time-resolved autofluorescence between healthy subjects and patients suffering from early AMD].

D Schweitzer1, S Quick, S Schenke, M Klemm, S Gehlert, M Hammer, S Jentsch, J Fischer.   

Abstract

BACKGROUND: A fluorescence lifetime mapper (FLM) was tested for quantitative estimation of early alterations in age-related macular degeneration (AMD) which are assumed to be in cellular metabolism.
METHOD: In FLM time-resolved autofluorescence of the fundus is excited by picosecond (ps) laser impulses at 448 nm and detected in 2 spectral ranges (K1=490-560 nm and K2=560-700 nm) by time-correlated single photon counting. The time-dependent decrease in fluorescence intensity was approximated using 3 decay rates. The calculated lifetimes allow a comparison with endogenous fluorophores of cellular metabolism.
RESULTS: Initially mean lifetimes were determined for 8 healthy subjects (K1: tau1=118 ps, tau2=584 ps, tau3=2826 ps, K2: tau1=104 ps, tau2=477 ps, tau3=1623 ps). In 15 AMD patients (AREDS categories I and II) the lifetimes were longer (K1: tau1=166 ps, tau2=986 ps, tau3=3309 ps, K2: tau1=137 ps, tau2=583 ps, tau3=1924 ps). The best separation between healthy subjects and patients with early AMD was possible by parameters 1 and 2 in the short-wave channel. Fluorophore-specific alterations in the macula could be demonstrated in isolated cases with advanced AMD.
CONCLUSION: Measurements in the 30 degrees fundus field demonstrated that specific alterations were already present even in early AMD and also outside the macula. These act in the neuronal retina, because parameter tau2 is related to this layer. Increases in the lifetime of parameter tau2 in the short wave channel could at least partially be determined by an increase of protein bound NADH, the content of which increases with reduced cellular respiration.

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Year:  2009        PMID: 19588156     DOI: 10.1007/s00347-009-1975-4

Source DB:  PubMed          Journal:  Ophthalmologe        ISSN: 0941-293X            Impact factor:   1.059


  17 in total

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3.  Characterization of native retinal fluorophores involved in biosynthesis of A2E and lipofuscin-associated retinopathies.

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4.  Oxidation of A2E results in the formation of highly reactive aldehydes and ketones.

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5.  Characterization of peroxy-A2E and furan-A2E photooxidation products and detection in human and mouse retinal pigment epithelial cell lipofuscin.

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8.  Isolation and characterization of a retinal pigment epithelial cell fluorophore: an all-trans-retinal dimer conjugate.

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  15 in total

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2.  Fluorescence lifetime imaging ophthalmoscopy in glaucoma.

Authors:  L Ramm; S Jentsch; R Augsten; M Hammer
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3.  Estimation of fluorescence lifetime of lipofuscin fluorophores contained in lipofuscin granules of retinal pigment epithelium of human cadaver eyes without signs of pathology.

Authors:  M A Yakovleva; T B Feldman; P M Arbukhanova; S A Borzenok; V A Kuzmin; M A Ostrovsky
Journal:  Dokl Biochem Biophys       Date:  2017-04-19       Impact factor: 0.788

4.  The fluorescence lifetime of lipofuscin granule fluorophores contained in the retinal pigment epithelium cells from human cadaver eyes in normal state and in the case of visualized pathology.

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5.  Spectral analysis of fundus autofluorescence pattern as a tool to detect early stages of degeneration in the retina and retinal pigment epithelium.

Authors:  Tatiana B Feldman; Marina A Yakovleva; Andrey V Larichev; Patimat M Arbukhanova; Alexandra Sh Radchenko; Sergey A Borzenok; Vladimir A Kuzmin; Mikhail A Ostrovsky
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