The preparation, staining, visualization, and interpretation of histological images of tissue is well-accepted as the gold standard process for the diagnosis of disease. These methods were developed historically, and are used ubiquitously in pathology, despite being highly time and labor intensive. Here we introduce a unique optical imaging platform and methodology for label-free multimodal multiphoton microscopy that uses a novel photonic crystal fiber source to generate tailored chemical contrast based on programmable supercontinuum pulses. We demonstrate collection of optical signatures of the tumor microenvironment, including evidence of mesoscopic biological organization, tumor cell migration, and (lymph-)angiogenesis collected directly from fresh ex vivo mammary tissue. Acquisition of these optical signatures and other cellular or extracellular features, which are largely absent from histologically processed and stained tissue, combined with an adaptable platform for optical alignment-free programmable-contrast imaging, offers the potential to translate stain-free molecular histopathology into routine clinical use.
Label-free microscopy with chemical contrast and high acquisition speed up to video-rate has recently been made possible by stimulated Raman scattering (SRS) microscopy. While SRS imaging offers superb sensitivity, the spectral specificity of the original narrowband implementation is limited, making distinguishing chemical species with overlapping Raman bands difficult. Here we present a highly specific imaging method that allows mapping of a particular chemical species in the presence of interfering species based on tailored multiplex excitation of its vibrational spectrum. This is done by spectral modulation of a broadband pump beam at a high-frequency (>1MHz), allowing detection of the stimulated Raman gain signal of the narrowband Stokes beam with high sensitivity. Using the scheme, we demonstrate quantification of cholesterol in the presence of lipids, and real-time three-dimensional spectral imaging of protein, stearic acid and oleic acid in live C.elegans.
The inherent brevity of ultrashort laser pulses prevents a direct measurement of their electric field as a function of time; therefore different approaches based on autocorrelation have been used to characterize them. We present a discussion, guided by experimental studies, regarding accurate measurement, compression, and shaping of ultrashort laser pulses without autocorrelation or interferometry. Our approach based on phase shaping, multiphoton intrapulse interference phase scan, provides a direct measurement of the spectral phase. Illustrations of this method include new results demonstrating wavelength independence, compatibility with sub-5 fs pulses, and a perfect match for experimental coherent control and biomedical imaging applications.
We report the detection of characteristic Raman lines for several chemicals using a single-beam coherent anti-Stokes Raman scattering (CARS) technique from a 12 meter standoff distance. Single laser shot spectra are obtained with sufficient signal to noise ratio to allow molecular identification. Background and spectroscopic discrimination are achieved through binary phase pulse shaping for optimal excitation of a single vibrational mode. These results provide a promising approach to standoff detection of chemicals, hazardous contaminants, and explosives.
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