Broadband stimulated Raman imaging based on multi-channel lock-in detection for spectral histopathology

Author:

De la Cadena Alejandro1ORCID,Vernuccio Federico1ORCID,Ragni Andrea2ORCID,Sciortino Giuseppe2ORCID,Vanna Renzo3ORCID,Ferrante Carino4567ORCID,Pediconi Natalia4ORCID,Valensise Carlo8ORCID,Genchi Luca9ORCID,Laptenok Sergey P.9ORCID,Doni Andrea10ORCID,Erreni Marco10ORCID,Scopigno Tullio457ORCID,Liberale Carlo11ORCID,Ferrari Giorgio2ORCID,Sampietro Marco2ORCID,Cerullo Giulio13ORCID,Polli Dario13ORCID

Affiliation:

1. Physics Department, Politecnico di Milano, Milan, Italy

2. Electronics, Information, and Bioengineering Department, Politecnico di Milano, Italy

3. Institute for Photonics and Nanotechnologies, CNR (IFN-CNR), Milan, Italy

4. Physics Department, Universitá di Roma “La Sapienza,” Roma, Italy

5. Italian Institute of Technology, Center for Life Nano-and Neuro-Science, Roma, Italy

6. ENEA, FSN-FISS-SNI Laboratory, Roma, Italy

7. Italian Institute of Technology, Graphene Labs, Genoa, Italy

8. Enrico Fermi Research Center, Roma, Italy

9. Biological and Environmental Science and Engineering Division, King Abdullah University of Science and Technology (KAUST), 23955 Thuwal, Saudi Arabia

10. Unit of Advanced Optical Microscopy, IRCCS Humanitas Research Hospital, Milan, Italy

11. Computer, Electrical and Mathematical Sciences Division, King Abdullah University of Science and Technology (KAUST), 23955 Thuwal, Saudi Arabia

Abstract

Spontaneous Raman microscopy reveals the chemical composition of a sample in a label-free and non-invasive fashion by directly measuring the vibrational spectra of molecules. However, its extremely low cross section prevents its application to fast imaging. Stimulated Raman scattering (SRS) amplifies the signal by several orders of magnitude thanks to the coherent nature of the nonlinear process, thus unlocking high-speed microscopy applications that provide analytical information to elucidate biochemical mechanisms with subcellular resolution. Nevertheless, in its standard implementation, narrowband SRS provides images at only one frequency at a time, which is not sufficient to distinguish constituents with overlapping Raman bands. Here, we report a broadband SRS microscope equipped with a home-built multichannel lock-in amplifier simultaneously measuring the SRS signal at 32 frequencies with integration time down to 44 µs, allowing for detailed, high spatial resolution mapping of spectrally congested samples. We demonstrate the capability of our microscope to differentiate the chemical constituents of heterogeneous samples by measuring the relative concentrations of different fatty acids in cultured hepatocytes at the single lipid droplet level and by differentiating tumor from peritumoral tissue in a preclinical mouse model of fibrosarcoma.

Funder

European Union’s Horizon 2020 research and innovation programme

Regione Lombardia

Global Collaborative Research, King Abdullah University of Science and Technology

Publisher

AIP Publishing

Subject

Computer Networks and Communications,Atomic and Molecular Physics, and Optics

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