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Miyasaka Lab. Ikegami Takahiro 100nm Ke Xu, H. P. Babcock, X. Zhuang, Nature Methods, 2012, 9, 185–188. Sub-diffraction limited point spread function achieved.

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Presentation on theme: "Miyasaka Lab. Ikegami Takahiro 100nm Ke Xu, H. P. Babcock, X. Zhuang, Nature Methods, 2012, 9, 185–188. Sub-diffraction limited point spread function achieved."— Presentation transcript:

1 Miyasaka Lab. Ikegami Takahiro 100nm Ke Xu, H. P. Babcock, X. Zhuang, Nature Methods, 2012, 9, 185–188. Sub-diffraction limited point spread function achieved by using photo-switchable fluorescence of diarylethene derivatives

2 I. Background Microscopy Fluorescence Microscopy Super-resolution Microscopy ( STED, PALM & STORM ) II. My work Principle Simulation Experience III. Summary IV. Future work

3 I. Background Microscopy Fluorescence Microscopy Super-resolution Microscopy ( STED, PALM & STORM ) II. My work Principle Simulation Experience III. Summary IV. Future work Have you ever used a microscope?

4 20 μm Shigeru Amemiya, Jidong Guo, Hui Xiong, Darrick A. Gross, Anal Bioanal Chem, 2006, 386, 458–471. 500 nm 5 μm 0.5 μm Scanning Electron Microscopy ( SEM ) Atomic Force Microscopy ( AFM ) Fluorescence Microscopy Various Microscopy L. Schermelleh, R. Heintzmann, H. Leonhard, THE JOURNAL OF CELL BIOLOGY, 2010, 190, 165-175. S. Sharma, R. W. Johnson, T. A. Desai, Biosensors and Bioelectronics, 2004, 20, 227-239.

5 Dye Sample example Imaging Shtengel et al., PNAS. 2009, 10,1073. Fluorescence microscopy Observation target ・ Biological tissue ・ Polymer film CCD camera Laser Scanning Laser Glass SiO 2 Trajectory of dye in PolyHEA Arai Yuhei, graduation thesis, 2014 3D trajectory of dye in PolyHEA Taga Yuhei, thesis for master degree, 2014

6 ・ Internal observation ・ Contactless ・ Time resolution Advantage of fluorescence microscopy Spatial resolution Fluorescence Microscopy λ/2 ( ≧ 200 nm ) Scanning Electron Microscopy ( SEM ) Atomic Force Microscopy ( AFM ) ( ≧ 0.1 nm ) << 0.5 μm 5 μm L. Schermelleh, R. Heintzmann, H. Leonhard, THE JOURNAL OF CELL BIOLOGY, 2010, 190, 165-175.

7 Resolution of fluorescence microscopy Low Resolution High Resolution Large LASER Spot Small LASER Spot Point Spread Function ( PSF ) Fluorescence PSF Objective smaller than diffraction limit Super-Resolution Microscopy

8 STED ( Stimulated Emission depletion ) Super-Resolution Microscopy h(v) v Δν FWHM Dye : RhodamineB λ STED = 600 nm : STED beam wavelength λ exc = 490 nm : Ecitation beam wavelength N.A.= 1.4 : Numerical aperture of objective FWHM of effective PSF 50 nm S. W. Hell, J. Wichmann, OPICS LETTERS. 1994, 19, 11. STED beam Excitation beam

9 PALM ( PhotoActivated Localization Microscopy ) & STORM ( Stochastic Optical Reconstruction Microscopy ) Super-Resolution Microscopy CCD camera B. Huang, W. Wang, M. Bates, X. Zhuang, Science, 2008, 319, 810-813. Low Resolution Fluorescence PSF Localization (A) Normal PALM & STORM Normal (B) STORM

10 I. Background Microscopy Fluorescence Microscopy Super-resolution Microscopy ( STED, PALM & STORM ) II. My work Principle Simulation Experience III. Summary IV. Future work

11 diarylethene derivative (DE1) Fluorescent UV (Φ oc = 0.43) Closed-form Open-form Vis. (Φ co = 1.6×10 -4 ) Φ F =0.88 non-Fluorescent Super-resolution by using photo-switchable fluorescent molecule

12 PSF Objective Dye (DAE1) Principle Visible position is shifted. UV Vis. Effective fluorescent spot size is changed by modulating a overlap of UV and Visible light. ※ UV Vis. Closed-form Open-form Fluorescent

13 Relation between Inter-spot distance & FWHM Vis. position = 0 nm Vis. position= - 550 nm FWHM = 230 nm FWHM = 40 nm ※ FWHM : 半値全幅 Simulation Laser & Fluorescence Intensity Distribution parameter Φ : Ring reaction yield I : Intensity C : Concentration Laser Dyes PMMA cover glass

14 Fluorescent intensity EFS by Simulation Experimental result Guest DE1 Host PMMA ※ Position of visible light was shifted to left. 1μm Parameter Sample preparation Intensity ( UV & Vis.) Irradiated position (Vis.) Relation between Inter-spot distance & FWHM

15 Stage scan imaging with APD A B C D E Measure photon number ※ Depended on the distribution of laser intensity single molecule PMMA cover glass Condition Principle APD Laser A B C D E Distribution of laser intensity Objective Stage ・ a few dye in several micrometers square ・ only a dye in laser light ・ Laser intensity is measured. ・ A fluorescence spot which is smaller than diffraction limit can be got. ・ The resolution is depended on the laser spot size and the step length of a stage. Optical setup Lens DM Pinhole Objective Stage

16 FWHM = 772 nm UV & Vis. completely overlaped. 300nm FWHM = 241 nm UV Vis. UV 300nm Stage scan imaging with APD UV & Vis. partly overlaped. Laser spot model Stage scan imaging Distribution of photon number

17 Summary ・ I explained about super-resolution microscopes such as STED, STORM, and PALM. ・ We observed that the smaller UV & Visible light overlap was, the smaller a fluorescence spot size became. UV Vis.

18 UV beam Visible donuts beam EFS Future work ・ Smaller spots than diffraction limit are made. ・ The visible donuts beam is used, and isotropic fluorescent spots is made. ・ Biological tissues or structures of polymer are modified by DE1, and they are observed.

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