Literature DB >> 28055837

Modulated-Alignment Dual-Axis (MAD) Confocal Microscopy Optimized for Speed and Contrast.

Steven Y Leigh, Jonathan T C Liu.   

Abstract

Modulated-alignment dual-axis (MAD) confocal microscopy combines the benefits of dual-axis confocal (DAC) microscopy and focal-modulation microscopy (FMM) for rejecting out-of-focus and multiply scattered light in tissues. The DAC architecture, which utilizes off-axis and separated beam paths for illumination and detection, has previously been shown to be superior to single-axis confocal (SAC) microscopy for the spatial filtering (rejection) of unwanted background light. With the MAD approach, a modulation of the alignment between the illumination and collection beam paths tags ballistic photons emanating from the focal volume with a characteristic radio frequency that can be extracted and separated from background signal using lock-in detection. We report here an optimized form of MAD confocal microscopy where we have fully mitigated tradeoffs in performance in an initial proof-of-concept system in order to recover the imaging speed of DAC microscopy while retaining contrast enhancement of 6 dB (signal-to-background ratio) with a secondary improvement in optical-sectioning and in-plane resolution. Validation is demonstrated with light-scattering tissue phantoms and freshly excised tissues.

Entities:  

Mesh:

Year:  2015        PMID: 28055837      PMCID: PMC5047853          DOI: 10.1109/TBME.2015.2511581

Source DB:  PubMed          Journal:  IEEE Trans Biomed Eng        ISSN: 0018-9294            Impact factor:   4.756


  23 in total

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5.  Modulated-alignment dual-axis (MAD) confocal microscopy for deep optical sectioning in tissues.

Authors:  Steven Y Leigh; Ye Chen; Jonathan T C Liu
Journal:  Biomed Opt Express       Date:  2014-04-30       Impact factor: 3.732

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9.  Deep-tissue focal fluorescence imaging with digitally time-reversed ultrasound-encoded light.

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