4Pi Superresolution Microscopy Literature References

Taking advantage of dual juxtaposed objectives, 4Pi microscopy is able to converge the excitation illumination at a common focal plane to generate constructive interference that reduces the axial resolution to a value near 100 nanometers. The resulting point-spread function is approximately 1.5-fold sharper in the lateral dimensions and nearly 7-fold sharper in the axial dimension compared to laser scanning confocal microscopy. 4Pi microscopy involves scanning the specimen pixel-by-pixel, similar to confocal, but can also be implemented with multi-photon laser sources and CCD camera systems.

Recommended Literature

Bahlmann, K., Jakobs, S. and Hell, S. W. 4Pi-confocal microscopy of live cells.Ultramicroscopy 87: 155-164 (2001).
Bewersdorf, J., Schmidt, R. and Hell, S. W. Comparison of I5M and 4Pi-microscopy. Journal of Microscopy 222: 105-117 (2006).
Egner, A. and Hell, S. W. Fluorescence microscopy with super-resolved optical sections.Trends in Cell Biology 15: 207-215 (2005).
Egner, A., Jakobs, S. and Hell, S. W. Fast 100-nm resolution three-dimensional microscope reveals structural plasticity of mitochondria in live yeast. Proceedings of the National Academy of Sciences (USA) 99: 3370-3375 (2002).
Egner, A., Verrier, S., Goroshkov, A., Soling, H. D. and Hell, S. W. 4Pi-microscopy of the Golgi apparatus in live mammalian cells. Journal of Structural Biology 147: 70-76 (2004).
Gugel, H., Bewersdorf, J., Jakobs, S., Engelhardt, J., Storz, R. and Hell, S. W. Cooperative 4Pi excitation and detection yields sevenfold sharper optical sections in live-cell microscopy.Biophysical Journal 87: 4146-4152 (2004).
Hell, S. W., Lindek, S. and Stelzer, E. H. K. Enhancing the axial resolution in far-field light microscopy: two-photon 4Pi confocal fluorescence microscopy. Journal of Modern Optics41: 675-681 (1994).
Hell, S. W. and Nagorni, M. 4Pi confocal microscopy with alternate interference. Optics Letters 23: 1567-1569 (1998).
Hell, S. W., Schmidt, R. and Egner, A. Diffraction-unlimited three-dimensional optical nanoscopy with opposing lenses. Nature Photonics 3: 381-387 (2009).
Hell, S. W., Schrader, M. and Van Der Voort, H. T. M. Far-field fluorescence microscopy with three-dimensional resolution in the 100-nm range. Journal of Microscopy 187: 1-7 (1997).
Hell, S. W. and Stelzer, E. H. K. Properties of a 4Pi confocal fluorescence microscope.Journal of the Optometric Society of America A 9: 2159-2166 (1992).
Hell, S. W. and Stelzer, E. H. K. Fundamental improvement of resolution with a 4Pi-confocal fluorescence microscope using two-photon excitation. Optics Communications 93: 277-282 (1992).
Lang, M. C., Staudt, T., Engelhardt, J. and Hell, S. W. 4Pi microscopy with negligible sidelobes. New Journal of Physics 10: 043041-13 (2008).
Schrader, M. and Hell, S. W. 4Pi-confocal images with axial superresolution. Journal of Microscopy 183: 110-115 (1996).
Schrader, M., Hell, S. W. and van der Vorrt, H. T. M. Three-dimensional super-resolution with a 4pi-confocal microscope using image restoration. Journal of Applied Physics 84: 4033-4042 (1998).

Additional Literature Sources

Arkhipov, A. and Schulten, K. Limits for reduction of effective focal volume in multiple-beam light microscopy. Optics Express 17: 2861-2870 (2009).
Arkhipov, A., Huve, J. H., Kahms, M., Peters, R. and Schulten, K. Continuous fluorescence microphotolysis and correlation spectroscopy using 4Pi microscopy. Biophysical Journal93: 4006-4017 (2007).
Bahlmann, K. and Hell, S. W. Polarization effects in 4Pi confocal microscopy studied with water-immersion lenses. Applied Optics 39: 1652-1658 (2000).
Bewersdorf, J., Bennett, B. T. and Knight, K. L. H2AX chromatin structures and their response to DNA damage revealed by 4Pi microscopy. Proceedings of the National Academy of Sciences (USA) 103: 18137-18142 (2006).
Egner, A., Schrader, M. and Hell, S. W. Refractive index mismatch induced intensity and phase variations in fluorescence confocal, multiphoton and 4Pi-microscopy. Optics Communications 153: 211-217 (1998).
Glaschick, S., Rocker, C., Deuschle, K., Wiedenmann, J., Oswald, F., Mailander, V. and Nienhaus, G. U. Axial resolution enhancement by 4Pi confocal fluorescence microscopy with two-photon excitation. Journal of Biological Physics 33: 433-443 (2007).
Haeberle, O., Xu, C., Dieterlen, A. and Jacquey, S. Multiple-objective microscopy with three-dimensional resolution near 100 nm and a long working distance. Optics Letters 26: 1684-1686 (2001).
Hanninen, P. E., Hell, S. W., Salo, J. and Soini, E. Two-photon excitation 4Pi confocal microscope: Enhanced axial resolution microscope for biological research. Applied Physics Letters 66: 1698-1700 (1995).
Hell, S. W., Lindek, S., Cremer, C. and Stelzer, E. H. K. Measurement of the 4Pi-confocal point spread function proves 75 nm axial resolution. Applied Physics Letters 64: 1335-1337 (1994).
Hell, S. W., Soukka, J. and Hanninen, P. E. Two- and multiphoton detection as an imaging mode and means of increasing the resolution in far-field light microscopy: A study based on photon-optics. Bioimaging 3: 64-69 (1995).
Hell, S. W., Stelzer, E. H. K., Lindek, S. and Cremer, C. Confocal microscopy with an increased detection aperture: Type-B 4Pi confocal microscopy. Optics Letters 19: 222-224 (1994).
Huve, J., Wesselmann, R., Kahms, M. and Peters, R. 4Pi microscopy of the nuclear pore complex. Biophysical Journal 95: 877-885 (2008).
Ivanchenko, S., Glaschick, S., Rocker, C., Oswald, F., Wiedenmann, J. and Nienhaus, G. Two-photon excitation and photoconversion of EosFP in dual-color 4Pi confocal microscopy.Biophysical Journal 92: 4451-4457 (2007).
Kano, H., Jakobs, S., Nagorni, M. and Hell, S. W. Dual-color 4Pi-confocal microscopy with 3D-resolution in the 100 nm range. Ultramicroscopy 90: 207-213 (2002).
Lang, M., Jegou, T., Chung, I., Richter, K., Munch, S., Udvarhelyi, A., Cremer, C., Hemmerich, P., Engelhardt, J., Hell, S. W. and Rippe, K. Three-dimensional organization of promyelocytic leukemia nuclear bodies. Journal of Cell Science 123: 392-400 (2010).
Lang, M. C., Engelhardt, J. and Hell, S. W. 4Pi microscopy with linear fluorescence excitation. Optics Letters 32: 259-261 (2007).
Lang, M. C., Muller, T., Engelhardt, J. and Hell, S. W. 4Pi microscopy of type A with 1-photon excitation in biological fluorescence imaging. Optics Express 15: 2459-2467 (2007).
Mar Blanca, C. M. and Hell, S. W. Sharp spherical focal spot by dark ring 4pi-confocal microscopy. Single Molecules 2: 207-210 (2001).
Nagorni, M. and Hell, S. W. 4Pi-confocal microscopy provides three-dimensional images of the microtubule network with 100- to 150-nm resolution. Journal of Structural Biology 123:236-247 (1998).
Nagorni, M. and Hell, S. W. Coherent use of opposing lenses for axial resolution increase. II. Power and limitation of nonlinear image restoration. Journal of the Optical Society of America A 18: 49-54 (2001).
Perinetti, G., Muller, T., Spaar, A., Polishchuk, R., Luini, A. and Egner, A. Correlation of 4Pi and electron microscopy to study transport through single Golgi stacks in living cells with super resolution. Traffic 10: 379-391 (2009).
Plecita-Hlavata, L., Lessard, M., Santorova, J., Bewersdorf, J. and Jezek, P. Mitochondrial oxidative phosphorylation and energetic status are reflected by morphology of mitochondrial network in INS-1E and HEP-G2 cells viewed by 4Pi microscopy. Biochimica et Biophysica Acta - Bioenergetics 1777: 834-846 (2008).
Schrader, M., Bahlmann, K., Giese, G. and Hell, S. W. 4Pi-confocal imaging in fixed biological specimens. Biophysical Journal 75: 1659-1668 (1998).
Schrader, M., Kozubek, M. Hell, S. W. and Wilson, T. Optical transfer functions of 4Pi confocal microscopes: Theory and experiment. Optics Letters 22: 436-438 (1997).
Vicidomini, G., Hell, S. W. and Schonle, A. Automatic deconvolution of 4Pi-microscopy data with arbitrary phase. Optics Letters 34: 3583-3585 (2009).
Vicidomini, G., Schmidt, R., Egner, A., Hell, S. W. and Schonle, A. Automatic deconvolution of 4Pi-microscopy with variable phase. Optics Express 18: 10154-10167 (2010).
von Middendorff, C., Egner, A., Geisler, C., Hell, S. W. and Schonle, A. Isotropic 3D nanoscopy based on single emitter switching. Optics Express 16: 20774-20788 (2008)

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