Spinning disk vs point scanner
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simon walker (BI) |
Spinning disk vs point scanner
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy ***** A confocal question! We have been imaging single live fluorescent cells in aqueous buffer held in suspension at a distance of ~80 um from the coverslip surface. We need to visualise rapid changes in the 3D structure of the cells so have been trying to capture image stacks using spinning disk confocal (EM-CCD camera, CSU-10, 60x water immersion 1.27 NA lens). The images we obtain are useless - really noisy, and the round cells apprear highly distorted (the fuzzy mass becomes elongated in x and then y as you focus up and down through the cell). We then tried the same experiment on a point scanning confocal using exactly the same microscope body and lens, and got really nice images (but not obtained with sufficient speed to make the experiment viable). So my (ignorant) question is, why should the spinning disk microscope perform so badly imaging a small fluorescent object at depth in an aqueous buffer? I know (older) spinning disk systems are not so good at imaging at depth into thicker specimens due to out-of-focus light entering adjacent pinholes, but I thought that imaging a small fluorescent object at depth with an RI-matched lens would be ok. Any explanations would be appreciated.. Thanks, Simon P.S. I tried playing with the correction collar on the lens, but that made no difference. |
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Mark Cannell-2 |
Re: Spinning disk vs point scanner
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy ***** H Simon The extended z is due to the effective pinhole size in the spinning disk. Can you use a higher magnification objective? Cheers On 25/04/2013, at 10:55 AM, Simon Walker <[hidden email]> wrote: > ***** > To join, leave or search the confocal microscopy listserv, go to: > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy > ***** > > A confocal question! > We have been imaging single live fluorescent cells in aqueous buffer held in > suspension at a distance of ~80 um from the coverslip surface. We need to > visualise rapid changes in the 3D structure of the cells so have been trying to > capture image stacks using spinning disk confocal (EM-CCD camera, CSU-10, > 60x water immersion 1.27 NA lens). The images we obtain are useless - really > noisy, and the round cells apprear highly distorted (the fuzzy mass becomes > elongated in x and then y as you focus up and down through the cell). We > then tried the same experiment on a point scanning confocal using exactly the > same microscope body and lens, and got really nice images (but not obtained > with sufficient speed to make the experiment viable). So my (ignorant) > question is, why should the spinning disk microscope perform so badly imaging > a small fluorescent object at depth in an aqueous buffer? I know (older) > spinning disk systems are not so good at imaging at depth into thicker > specimens due to out-of-focus light entering adjacent pinholes, but I thought > that imaging a small fluorescent object at depth with an RI-matched lens > would be ok. > Any explanations would be appreciated.. > Thanks, > Simon > P.S. I tried playing with the correction collar on the lens, but that made no > difference. Mark B. Cannell Ph.D. FRSNZ Professor of Cardiac Cell Biology School of Physiology & Pharmacology Medical Sciences Building University of Bristol Bristol BS8 1TD UK [hidden email] |
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Martin Wessendorf-2 |
Re: Spinning disk vs point scanner
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In reply to this post by simon walker (BI)
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy ***** Dear Simon-- On 4/25/2013 4:55 AM, Simon Walker wrote: > We have been imaging single live fluorescent cells in aqueous buffer held in > suspension at a distance of ~80 um from the coverslip surface. We need to > visualise rapid changes in the 3D structure of the cells so have been trying to > capture image stacks using spinning disk confocal (EM-CCD camera, CSU-10, > 60x water immersion 1.27 NA lens). The images we obtain are useless - really > noisy, and the round cells apprear highly distorted (the fuzzy mass becomes > elongated in x and then y as you focus up and down through the cell). We > then tried the same experiment on a point scanning confocal using exactly the > same microscope body and lens, and got really nice images (but not obtained > with sufficient speed to make the experiment viable). Can the spinning disk instrument image a fluorescent bead or other similar test specimen without distortion? Or is the problem only with your thick specimen? Good luck! Martin -- Martin Wessendorf, Ph.D. office: (612) 626-0145 Assoc Prof, Dept Neuroscience lab: (612) 624-2991 University of Minnesota Preferred FAX: (612) 624-8118 6-145 Jackson Hall, 321 Church St. SE Dept Fax: (612) 626-5009 Minneapolis, MN 55455 e-mail: [hidden email] |
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