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English: Superresolution Microscopy/ Optical nanoscopy using SPDMphymod as a new localization microscopy technique for standard fluorescent dyes

SPDMphymod image of protein distribution in a human cancer cell. Enlarged inserts above and below: Positions of single fluorescent molecules in Gaussian intensity shape of 5 nm standard deviation. Typical distance measurements in the 15 nm range are highlighted

Fundamental to SPDMphymod are blinking phenomena (flashes of fluorescence), induced by reversible bleaches (metastable dark states). Individual molecules of the same spectral emission color can be detected. Counting individual molecules up to a density of 1000/µm2 – at present, this is possible in an area of up to 5000 µm2.

Christoph Cremer, emeritus at Heidelberg university [1] Basic publications:

Lemmer P, Gunkel M, Baddeley D, Kaufmann R, Urich A, Weiland Y, Reymann J, Müller P, Hausmann M, Cremer C: SPDM – Light Microscopy with Single Molecule Resolution at the Nanoscale. In: Applied Physics B 2008; 93: 1–12

Manuel Gunkel, Fabian Erdel, Karsten Rippe, Paul Lemmer, Rainer Kaufmann, Christoph Hörmann, Roman Amberger and Christoph Cremer: Dual color localization microscopy of cellular nanostructures. In: Biotechnology Journal, 2009, 4, 927-938. ISSN 1860-6768
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Author Andy Nestl
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Original upload log

This image was originally uploaded in BMP format as File:Single_YFP_molecule_superresolution_microscopy.tif. The original upload history (excluding reverts) is shown below:

  • 2009-12-01T12:00:38Z Andy Nestl 340x686 (699774 Bytes, image/x-bmp) test2
  • 2009-12-01T11:45:07Z Andy Nestl 340x686 (700634 Bytes, image/tiff) {{Information |Description={{en|1=Superresolution Microscopy using SPDMphymod as a new localization microscopy technique for standard fluorescent dyes}} |Source={{own}} |Author=Andy Nestl |Date=2009-12-01 |Permission=given by Christoph
  1. https://www.physik.uni-heidelberg.de/personen/lsf.php?details=1537 |titel=Fakultät für Physik und Astronomie |abruf=2020-10-01

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