In vivo measurement of time-resolved autofluorescence at the human fundus

被引:114
|
作者
Schweitzer, D
Hammer, M
Schweitzer, F [1 ]
Anders, R
Doebbecke, T
Schenke, S
Gaillard, ER
Gaillard, ER
机构
[1] Univ Jena, Dept Expt Ophthalmol, Eye Clin, Bachstr 18, D-07740 Jena, Germany
[2] No Illinois Univ, Dept Biochem & Chem, De Kalb, IL 60115 USA
关键词
time-resolved autofluorescence; fluorescence lifetime imaging; human fundus; time-correlated single photon counting; scanning laser ophthalmoscopy; lipofuscin; coenzymes;
D O I
10.1117/1.1806833
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
An experimental setup for measurement of time-resolved autofluorescence of the human eye funclus is demonstrated. The method combines laser scanning technique and time-correlated single photon counting. The light source is a laser diode, delivering pulses of about 100 ps duration at a repetition rate of 40 MHz. The excitation wavelength is 446 nm and the cutoff wavelength of fluorescence detection is at 475 nm. The autofluorescence can be determined with a spatial resolution of 80X80 mum(2) and 25 ps time resolution. The fluorescence decay is optimally approximated by a biexponential model. The dominating lifetime lambda1 is shortest in the macula (320 to 380 ps) and reaches 1500 ps in the optic disk. The lifetime lambda2 varies between 2 ns and 5 ns, but the spatial distribution is more homogeneous. Respiration of 100% oxygen for 6 min leads to changes in the fluorescence lifetime pointing to detection of coenzymes. Diagrams of lifetime lambda2 versus -lambda1 are well suited for comparison of substances. Such lifetime clusters of a 20 deg macular field of a young healthy subject and of a patient suffering from dry age-related macular degeneration overlap only partially with lambda2-lambda1 clusters of lipofuscin. (C) 2004 Society of Photo-Optical Instrumentation Engineers.
引用
收藏
页码:1214 / 1222
页数:9
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