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Surgical microscope with integrated fluorescence lifetime imaging for 5-aminolevulinic acid fluorescence-guided neurosurgery

by Roetzer, Thomas , Drexler, Wolfgang , Andreana, Marco , Reichert, David , Hauger, Christoph , Widhalm, Georg , Unterhuber, Angelika , Kiesel, Barbara , Gesperger, Johanna , Erkkilä, Mikael T , Leitgeb, Rainer A , Wilzbach, Marco , Hecker-Denschlag, Nancy

in Accuracy / Aminolevulinic acid / Brain cancer / Cameras / Feasibility / Fluorescence / Glioma / Histopathology / Imaging / Lasers / Letter / Lifetime / Microscopes / Microscopy / Neurosurgery / Special Section on Selected Topics in Biophotonics: Fluorescence Lifetime Imaging and Optical Micromechanics / Surgeons / Tumors / White light

2020

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Surgical microscope with integrated fluorescence lifetime imaging for 5-aminolevulinic acid fluorescence-guided neurosurgery

2020

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Surgical microscope with integrated fluorescence lifetime imaging for 5-aminolevulinic acid fluorescence-guided neurosurgery

2020

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Journal Article

Surgical microscope with integrated fluorescence lifetime imaging for 5-aminolevulinic acid fluorescence-guided neurosurgery

Roetzer, Thomas,

Drexler, Wolfgang,

Andreana, Marco,

Reichert, David,

Hauger, Christoph,

Widhalm, Georg,

Unterhuber, Angelika,

Kiesel, Barbara,

Gesperger, Johanna,

Erkkilä, Mikael T,

Leitgeb, Rainer A,

Wilzbach, Marco,

Hecker-Denschlag, Nancy

2020

Overview

Significance: 5-Aminolevulinic acid (5-ALA)-based fluorescence guidance in conventional neurosurgical microscopes is limited to strongly fluorescent tumor tissue. Therefore, more sensitive, intrasurgical 5-ALA fluorescence visualization is needed. Aim: Macroscopic fluorescence lifetime imaging (FLIM) was performed ex vivo on 5-ALA-labeled human glioma tissue through a surgical microscope to evaluate its feasibility and to compare it to fluorescence intensity imaging. Approach: Frequency-domain FLIM was integrated into a surgical microscope, which enabled parallel wide-field white-light and fluorescence imaging. We first characterized our system and performed imaging of two samples of suspected low-grade glioma, which were compared to histopathology. Results: Our imaging system enabled macroscopic FLIM of a 6.5 × 6.5 mm2 field of view at spatial resolutions <20 μm. A frame of 512 × 512 pixels with a lifetime accuracy <1 ns was obtained in 65 s. Compared to conventional fluorescence imaging, FLIM considerably highlighted areas with weak 5-ALA fluorescence, which was in good agreement with histopathology. Conclusions: Integration of macroscopic FLIM into a surgical microscope is feasible and a promising method for improved tumor delineation.

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Publisher

Society of Photo-Optical Instrumentation Engineers,S P I E - International Society for

Subject

Accuracy

/ Aminolevulinic acid

/ Brain cancer

/ Cameras

/ Feasibility

/ Fluorescence

/ Glioma