Selecting optimal spectral bands for improved detection of autofluorescent biomarkers in multiphoton microscopy.
biomarkers
fluorescence spectrum
functional imaging
hyperspectral imaging
multiphoton microscopy
redox ratio
spectroscopy
two-photon excitation fluorescence
Journal
Journal of biomedical optics
ISSN: 1560-2281
Titre abrégé: J Biomed Opt
Pays: United States
ID NLM: 9605853
Informations de publication
Date de publication:
07 2020
07 2020
Historique:
received:
18
11
2019
accepted:
22
06
2020
entrez:
9
7
2020
pubmed:
9
7
2020
medline:
25
9
2021
Statut:
ppublish
Résumé
In multiphoton microscopy, two-photon excited fluorescence (TPEF) spectra carry valuable information on morphological and functional biological features. For measuring these biomarkers, separation of different parts of the fluorescence spectrum into channels is typically achieved by the use of optical band pass filters. However, spectra from different biomarkers can be unknown or overlapping, creating a crosstalk in between the channels. Previously, establishing these channels relied on prior knowledge or heuristic testing. The presented method aims to provide spectral bands with optimal separation between groups of specimens expressing different biomarkers. We have developed a system capable of resolving TPEF with high spectral resolution for the characterization of biomarkers. In addition, an algorithm is created to simulate and optimize optical band pass filters for fluorescence detection channels. To demonstrate the potential improvements in cell and tissue classification using these optimized channels, we recorded spectrally resolved images of cancerous (HT29) and normal epithelial colon cells (FHC), cultivated in 2D layers and in 3D to form spheroids. To provide an example of an application, we relate the results with the widely used redox ratio. We show that in the case of two detection channels, our system and algorithm enable the selection of optimized band pass filters without the need of knowing involved fluorophores. An improvement of 31,5% in separating different 2D cell cultures is achieved, compared to using established spectral bands that assume NAD(P)H and FAD as main contributors of autofluorescence. The compromise is a reduced SNR in the images. We show that the presented method has the ability to improve imaging contrast and can be used to tailor a given label-free optical imaging system using optical band pass filters targeting a specific biomarker or application.
Identifiants
pubmed: 32638570
pii: JBO-190404SSRR
doi: 10.1117/1.JBO.25.7.071206
pmc: PMC7338838
doi:
Substances chimiques
Biomarkers
0
Fluorescent Dyes
0
Types de publication
Journal Article
Research Support, Non-U.S. Gov't
Langues
eng
Sous-ensembles de citation
IM
Pagination
1-13Références
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