Combined hyperspectral imaging, monolayer stress microscopy, and S8 image analysis approaches for simultaneously interrogating cellular signals and biomechanics

Silas J Leavesley; Santina Johnson; Sunita S Paudel; Jennifer Knighten; Dhananjay T Tambe; Michael Francis; Na Gong; Mark S Taylor; Thomas C Rich

doi:10.1117/12.2650653

Combined hyperspectral imaging, monolayer stress microscopy, and S8 image analysis approaches for simultaneously interrogating cellular signals and biomechanics

Proc SPIE Int Soc Opt Eng. 2023 Jan-Feb:12383:123830D. doi: 10.1117/12.2650653. Epub 2023 Mar 15.

Authors

Silas J Leavesley^{1

2

3}, Santina Johnson², Sunita S Paudel^{3

4}, Jennifer Knighten⁴, Dhananjay T Tambe^{2

3

5}, Michael Francis^{3

4}, Na Gong⁶, Mark S Taylor^{3

4}, Thomas C Rich^{2

3}

Affiliations

¹ Department of Chemical and Biomolecular Engineering.
² Department of Pharmacology.
³ Center for Lung Biology.
⁴ Department of Physiology and Cell Biology.
⁵ William B. Burnsed Jr. Department of Mechanical, Aerospace, and Biomedical Engineering.
⁶ Department of Electrical and Computer Engineering, University of South Alabama, Mobile, AL, USA 36688.

Abstract

Second messenger signals, e.g., Ca²⁺ and cyclic nucleotides, orchestrate a wide range of cellular events. The methods by which second messenger signals determine specific physiological responses are complex. Recent studies point to the importance of temporal and spatial encoding in determining signal specificity. Studies also indicate the importance of mechanical stimuli, substrate stiffness, and mechanical responses - the "mechanosome" - in regulating physiology. Hence, approaches that probe both chemical and mechanical signals are needed. Here, we report preliminary efforts to combine hyperspectral imaging for second messenger signal measurements, monolayer stress microscopy for mechanical force measurements, and S8 analysis software for quantifying localized signals - specifically, Ca²⁺ dynamics and mechanical forces in human airway smooth muscle cells (HASMCs). HASMCs were prepared as confluent monolayers on 11 kPa gels with embedded fluorescent microparticles that serve as fiducial markers as well as smaller microparticles to measure deformation (strain). Imaging was performed using a custom excitation-scanning hyperspectral microscope. Hyperspectral images were unmixed to identify signals from cellular fluorescent labels (e.g., CAL 590-AM) and fluorescent microparticles. Images were analyzed to quantify localized force dynamics through monolayer stress microscopy. S8 software was used to identify, track, and quantify spatially-localized Ca²⁺ activity. Results indicate that localized and transient cellular signals and forces can be quantified and mapped within cell populations. Importantly, these results establish a method for simultaneous interrogation of cellular signals and mechanical forces that may play synergistic roles in regulating downstream cellular physiology in confluent monolayers. This work was supported by NIH P01HL066299, R01HL137030, R01HL058506, and NSF MRI1725937. Drs. Leavesley and Rich disclose financial interest in a university start-up company, SpectraCyte LLC, to commercialize spectral imaging technologies.

Keywords: Spectral; cell signaling; forces; mechanobiology; second messenger; signature; spectroscopy.

Abstract

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