Multifaceted mirror array illuminator for fluorescence excitation-scanning spectral imaging microscopy

Marina Parker; Samuel A Mayes; Craig M Browning; Joshua Deal; Samantha Gunn-Mayes; Naga S Annamdevula; Thomas C Rich; Silas J Leavesley

doi:10.1117/1.JBO.28.2.026502

Multifaceted mirror array illuminator for fluorescence excitation-scanning spectral imaging microscopy

J Biomed Opt. 2023 Feb;28(2):026502. doi: 10.1117/1.JBO.28.2.026502. Epub 2023 Feb 7.

Authors

Marina Parker^{1

2}, Samuel A Mayes^{1

2}, Craig M Browning^{1

2}, Joshua Deal^{3

4}, Samantha Gunn-Mayes¹, Naga S Annamdevula^{1

3

4}, Thomas C Rich^{3

4}, Silas J Leavesley^{1

2

3

4}

Affiliations

¹ University of South Alabama, Department of Chemical and Biomolecular Engineering, Mobile, Alabama, United States.
² University of South Alabama, Systems Engineering, Mobile, Alabama, United States.
³ University of South Alabama, Department of Pharmacology, Mobile, Alabama, United States.
⁴ University of South Alabama, Center for Lung Biology, Mobile, Alabama, United States.

Abstract

Significance: Hyperspectral imaging (HSI) technologies offer great potential in fluorescence microscopy for multiplexed imaging, autofluorescence removal, and analysis of autofluorescent molecules. However, there are also associated trade-offs when implementing HSI in fluorescence microscopy systems, such as decreased acquisition speed, resolution, or field-of-view due to the need to acquire spectral information in addition to spatial information. The vast majority of HSI fluorescence microscopy systems provide spectral discrimination by filtering or dispersing the fluorescence emission, which may result in loss of emitted fluorescence signal due to optical filters, dispersive optics, or supporting optics, such as slits and collimators. Technologies that scan the fluorescence excitation spectrum may offer an approach to mitigate some of these trade-offs by decreasing the complexity of the emission light path.

Aim: We describe the development of an optical technique for hyperspectral imaging fluorescence excitation-scanning (HIFEX) on a microscope system.

Approach: The approach is based on the design of an array of wavelength-dependent light emitting diodes (LEDs) and a unique beam combining system that uses a multifurcated mirror. The system was modeled and optimized using optical ray trace simulations, and a prototype was built and coupled to an inverted microscope platform. The prototype system was calibrated, and initial feasibility testing was performed by imaging multilabel slide preparations.

Results: We present results from optical ray trace simulations, prototyping, calibration, and feasibility testing of the system. Results indicate that the system can discriminate between at least six fluorescent labels and autofluorescence and that the approach can provide decreased wavelength switching times, in comparison with mechanically tuned filters.

Conclusions: We anticipate that LED-based HIFEX microscopy may provide improved performance for time-dependent and photosensitive assays.

Keywords: excitation scanning; fluorescence microscopy; hyperspectral imaging; light emitting diode; spectral imaging; spectroscopy.

Publication types

Research Support, U.S. Gov't, Non-P.H.S.
Research Support, N.I.H., Extramural

MeSH terms

Carmustine*
Microscopy, Fluorescence / methods
Optics and Photonics*
Radionuclide Imaging
Spectrometry, Fluorescence / methods

Substances

Carmustine

Abstract

Publication types

MeSH terms

Substances

Grants and funding