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  • 發布時間:2019-04-28 20:05 原文鏈接: Setupanduseofatwolasermultiphotonmicroscope

    Setup and use of a two-laser multiphoton microscope for multichannel intravital fluorescence imaging
    David Entenberg,1 Jeffrey Wyckoff,1 Bojana Gligorijevic,1 Evanthia T Roussos,1 Vladislav V Verkhusha,1 Jeffrey W Pollard1 & John Condeelis1 
    Affiliations Contributions Corresponding author Journal name: 
    Nature Protocols Volume:6,Pages:1500–1520  Year published: (2011) 
    DOI: 
    doi:10.1038/nprot.2011.376 
    Published online 08 September 2011 

    Abstract
    Characterizing biological mechanisms dependent upon the interaction of many cell types in vivo requires both multiphoton microscope systems capable of expanding the number and types of fluorophores that can be imaged simultaneously while removing the wavelength and tunability restrictions of existing systems, and enhanced software for extracting critical cellular parameters from voluminous 4D data sets. We present a procedure for constructing a two-laser multiphoton microscope that extends the wavelength range of excitation light, expands the number of simultaneously usable fluorophores and markedly increases signal to noise via 'over-clocking' of detection. We also utilize a custom-written software plug-in that simplifies the quantitative tracking and analysis of 4D intravital image data. We begin by describing the optics, hardware, electronics and software required, and finally the use of the plug-in for analysis. We demonstrate the use of the setup and plug-in by presenting data collected via intravital imaging of a mouse model of breast cancer. The procedure may be completed in ~24 h.


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