Abstract

The purpose of this project is to develop a multifocal optical coherence microscope (OCM). The proposed OCM will allow noninvasive imaging of unstained biological specimens, with millisecond temporal resolution and sub-cellular spatial resolution in three dimensions. During this project, we expect to achieve three specific aims as follows: 1) Construction of a full-field OCM: We plan to develop a digital camera based full-filed OCM. An electro- optic phase modulator will be used for rapid, vibration-free phase modulation of the reference beam. A near infrared light will be employed to ensure high penetrating depth of OCM imaging. A four-step phase shifting algorithm will be used for concurrent reconstruction of intensity-sensitive and phase-sensitive OCM images. Polarization-sensitive imaging capability will be added to achieve high contrast imaging of biological specimens with birefringence characteristics. 2) Development of a multifocal OCM: In order to ensure the stability of sampling volume, we will employ a multifocal illumination and virtual pinhole confocal imaging strategy for further improvement of the full-field OCM. The combination of the virtual pinhole confocal imaging and low coherence gating mechanism will provide a two-stage `filtering'system for effective rejection of undesired noise light: 1) Computer- synthesized virtual pinholes will be used to reject out-of-focus light;2) Low coherence gating mechanism will be used to reject cross-talk noise light between adjacent sampling volumes. Using a near infrared light (center wavelength: ~800 nm) with 100 nm bandwidth, we anticipate a depth resolution better than 3 ?m. The lateral (perpendicular to the light axis) resolution will be optical diffraction limited. 3) Functional test of the multifocal OCM: A series of biological tissues/cells will be used to assess the intensity-sensitive, phase-sensitive, and polarization-sensitive imaging capabilities of the proposed OCM. Multi-modal OCM imaging of human skin will be also implemented for preliminary test of imaging stability of the proposed instrument for in vivo application. Although the proposed OCM promises a versatile imaging platform for a variety of biomedical applications, this project will focus on proof-of-concept of the imaging system.

Public Health Relevance

The proposed multifocal optical coherence microscope can provide fast, noninvasive imaging with sub-cellular spatial resolution in three dimensions. We anticipate that the multifocal OCM will find a wide range of applications in cell biology, neurobiology, tissue engineering, dermatology, and ophthalmology.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Center for Research Resources (NCRR)
Type
Exploratory/Developmental Grants (R21)
Project #
5R21RR025788-02
Application #
7914238
Study Section
Special Emphasis Panel (ZRR1-BT-B (01))
Program Officer
Friedman, Fred K
Project Start
2009-08-13
Project End
2012-08-12
Budget Start
2010-08-13
Budget End
2012-08-12
Support Year
2
Fiscal Year
2010
Total Cost
$249,400
Indirect Cost

  Institution

Name
University of Alabama Birmingham
Department
Biomedical Engineering
Type
Schools of Engineering
DUNS #
063690705
City
Birmingham
State
AL
Country
United States
Zip Code
35294

  Publications

Wang, Benquan; Lu, Rongwen; Zhang, Qiuxiang et al. (2013) En face optical coherence tomography of transient light response at photoreceptor outer segments in living frog eyecup. Opt Lett 38:4526-9
Zhang, Qiu-Xiang; Lu, Rong-Wen; Curcio, Christine A et al. (2012) In vivo confocal intrinsic optical signal identification of localized retinal dysfunction. Invest Ophthalmol Vis Sci 53:8139-45
Lu, Rong-Wen; Curcio, Christine A; Zhang, Youwen et al. (2012) Investigation of the hyper-reflective inner/outer segment band in optical coherence tomography of living frog retina. J Biomed Opt 17:060504
Yao, Xin-Cheng; Li, Yi-Chao (2012) Functional imaging of retinal photoreceptors and inner neurons using stimulus-evoked intrinsic optical signals. Methods Mol Biol 884:277-85
Yao, Xin-Cheng; Cui, Wan-Xing; Li, Yi-Chao et al. (2012) Functional imaging of glucose-evoked rat islet activities using transient intrinsic optical signals. J Mod Opt 59:
Li, Yi-Chao; Luo, Jian-Min; Lu, Rong-Wen et al. (2012) Dynamic intrinsic optical signal monitoring of electrically stimulated inner retinal neural response. J Mod Opt 59:
Zhang, Qiu-Xiang; Zhang, Youwen; Lu, Rong-Wen et al. (2012) Comparative intrinsic optical signal imaging of wild-type and mutant mouse retinas. Opt Express 20:7646-54
Zhang, Qiu-Xiang; Lu, Rong-Wen; Li, Yang-Guo et al. (2011) In vivo confocal imaging of fast intrinsic optical signals correlated with frog retinal activation. Opt Lett 36:4692-4
Lu, Rong-Wen; Li, Yi-Chao; Ye, Tong et al. (2011) Two-photon excited autofluorescence imaging of freshly isolated frog retinas. Biomed Opt Express 2:1494-503
Li, Yi-Chao; Cui, Wan-Xing; Wang, Xu-Jing et al. (2011) Intrinsic optical signal imaging of glucose-stimulated insulin secreting ?-cells. Opt Express 19:99-106

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