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10.1063/1.4943211

http://scihub22266oqcxt.onion/10.1063/1.4943211
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C4798998!4798998!27036751
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suck abstract from ncbi

pmid27036751      Rev+Sci+Instrum 2016 ; 87 (3): ä
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  • Invited Review Article: Pump-probe microscopy #MMPMID27036751
  • Fischer MC; Wilson JW; Robles FE; Warren WS
  • Rev Sci Instrum 2016[Mar]; 87 (3): ä PMID27036751show ga
  • Multiphoton microscopy has rapidly gained popularity in biomedical imaging and materials science because of its ability to provide three-dimensional images at high spatial and temporal resolution even in optically scattering environments. Currently the majority of commercial and home-built devices are based on two-photon fluorescence and harmonic generation contrast. These two contrast mechanisms are relatively easy to measure but can access only a limited range of endogenous targets. Recent developments in fast laser pulse generation, pulse shaping, and detection technology have made accessible a wide range of optical contrasts that utilize multiple pulses of different colors. Molecular excitation with multiple pulses offers a large number of adjustable parameters. For example, in two-pulse pump-probe microscopy, one can vary the wavelength of each excitation pulse, the detection wavelength, the timing between the excitation pulses, and the detection gating window after excitation. Such a large parameter space can provide much greater molecular specificity than existing single-color techniques and allow for structural and functional imaging without the need for exogenous dyes and labels, which might interfere with the system under study. In this review, we provide a tutorial overview, covering principles of pump-probe microscopy and experimental setup, challenges associated with signal detection and data processing, and an overview of applications.
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