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Developing a Bigger Palette to Elucidate Intricate Biologic Interactions

Published online by Cambridge University Press:  31 August 2017

Stephen W. Carmichael
Stephen W. Carmichael*
Affiliation:
Mayo Clinic, Rochester, MN 55905
*
[email protected]

Abstract

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Type
Carmichael’s Concise Review
Information
Microscopy Today , Volume 25 , Issue 5 , September 2017 , pp. 8 - 11
Copyright
Copyright © Microscopy Society of America 2017 

Fluorescence microscopy has proven to be a valuable method to localize molecules of biologic interest. However, the nature of broad fluorescence spectra limits the number of resolvable colors to about 5 (or with complicated instrumentation and analysis up to 9). Stimulated Raman scattering (SRS) microscopy avoids this limitation and provides peaks about 100 times narrower than fluorescence by relying on the interaction between the vibrational motion from the chemical bonds in the molecule of interest and laser beams. Lu Wei, Wei Min, and their colleagues have developed a methodology and an assortment of dyes to create a palette of 24 resolvable colors, with the potential for further expansion [Reference Wei1].

In SRS microscopy two laser beams (referred to as Stokes photons and pump photons) with different energies are collinearly focused onto cell samples. When the energy differences between the two beams matches the vibrational frequency of the targeted chemical bonds, the chemical bonds are efficiently excited to the vibrational excited state. A method to detect the intensity loss of the pump beam was used to spatially and temporally resolve molecules with selected chemical bonds. All previous SRS imaging is in the non-resonance region where the laser wavelengths are far away from molecular absorptions and thus have inadequate sensitivity for general applicability. Wei et al. exploited and determined a special region by carefully adjusting the two laser beams to be close to the electronic absorption of the molecules that could obtain signal enhancement with optimal contrast between vibrational signal and electronic background. They termed this electronic pre-resonance SRS (epr-SRS). Combining epr-SRS with selected dyes provided an improvement in sensitivity of about 1,000 over other non-resonance SRS imaging, which was comparable to confocal fluorescence microscopy, while retaining distinct vibrational contrast.

Wei et al. created a palette of triple-bond-conjugated (with, for example, alkynes) near-infrared dyes. Each displays a single peak in the Raman spectral window where background noise is non-existent (cell-silent). Combining this palette with available fluorescent probes provided 24 resolvable colors. They called this super-multiplex vibrational imaging.

Proof-of-principle experiments on both fixed and living cells demonstrated several successful applications. For example, imaging of proteome turnover dynamics in hippocampal neuronal cultures demonstrated that misfolded proteins were sequestered within inclusions in astrocytes rather than neurons (Figure 1). This may serve a protective function by sequestering potentially harmful proteins. This in turn suggests that the astrocyte resistance that has been observed previously could be due to their ability to actively form protein inclusions that isolate toxic proteins, something neurons are unable to do.

Figure 1 Super-multiplex optical imaging for investigation of proteome turnover dynamics in hippocampal neuronal cultures. (a) Pulse-chase (HPG-AHA) experimental design. MG132: proteasome inhibitor. (b–e) Cytosolic aggregations (indicated by arrowheads) are mostly from proteins synthesized in the chase period (b-c) and appear mostly in astrocytes (d) but not in neurons (e). HPG: 1-homopropargylglyceine. AHA: 1-azidohomoalanine. GFAP: glial fibrillary acidic protein. MBP: myelin basic protein. Scale bars = 10 μm.

These and other studies demonstrated improved sensitivity, resolution, labeling versatility, and biocompatibility that complement fluorescence microscopy. In addition, Wei et al. suggested that their technique can be further improved in at least 3 ways. First, the dye palette could potentially be expanded to 50 or more colors by filling the rather broad cell-silent window with individual sharp peaks from new vibrational moieties. Secondly, genetically encoded infrared proteins could be engineered to serve as vibrational reporters. Third, techniques (such as hyper-spectral imaging) could be implemented to realize faster and simultaneous signal acquisition. Because of all the improvements and potential improvements in the 24-color (super-multiplex) optical imaging approach developed by Wei et al., we can expect this new technology to find wide application in the probing of complex biologic systems.

References

[1] Wei, L et al., Nature 544 (2017) 465470.CrossRefGoogle Scholar
[2] The author gratefully acknowledges Drs. Lu Wei and Wei Min for reviewing this article.Google Scholar
Figure 0

Figure 1 Super-multiplex optical imaging for investigation of proteome turnover dynamics in hippocampal neuronal cultures. (a) Pulse-chase (HPG-AHA) experimental design. MG132: proteasome inhibitor. (b–e) Cytosolic aggregations (indicated by arrowheads) are mostly from proteins synthesized in the chase period (b-c) and appear mostly in astrocytes (d) but not in neurons (e). HPG: 1-homopropargylglyceine. AHA: 1-azidohomoalanine. GFAP: glial fibrillary acidic protein. MBP: myelin basic protein. Scale bars = 10 μm.