CCD camera
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http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal We would like to add a color CCD camera to our Zeiss LSM-510 META confocal to capture color tiled wide field images. We wondered if other users have already done this? What cameras did you add and how well does the LSM 510 software control the image acquisition with the camera you are using? We are particularly interested in tiled images. We have a PixeLINK model PL-A662 color CCD camera on a separate stereo scope. We are told that this camera would not work with the LSM-510. Does anyone have any contrary information about this? Thanks for your help. Alice Alice L. Givan Englert Cell Analysis Laboratory of the Norris Cotton Cancer Center Dartmouth Medical School Lebanon, NH 03756 USA tel 603-650-7661 fax 603-650-6130 [hidden email] www.dartmouth.edu/~celllab |
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Search the CONFOCAL archive at
http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal Hello Alice, As far as I know the LSM510 software can control only the Zeiss Axiovision cameras (for sure it does so with the monochromatic one). Whether it can control also the color ones - I have no idea. If you want to stick with your camera - you should consider buying a separate image acquisition software (or use a freeware). There would be no problem to install it on the LSM 510 computer (so you don't need an additional computer) and many software can control the Zeiss MCU28 stage controller and also the motorized Zeiss microscopes (and is of course capable of doing tile scans....). Cheers Gabor -- Gabor Csucs Light Microscopy Centre, ETH Zurich Schafmattstrasse 18, HPM F16 CH-8093, Zurich, Switzerland Web: www.lmc.ethz.ch Phone: +41 44 633 6221 Fax: +41 44 632 1298 e-mail: [hidden email] |
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In reply to this post by Alice L. Givan
Search the CONFOCAL archive at
http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal Hi, Alice, We did not use the Zeiss camera. However, we had a similar need long time ago as some one tried to correlate histology with immunofluorescence. Here was how we got by (without a camera): use your red, green and blue laser lines and set up a sequential scanning configuration with your transmitted detector. You can get a pseudo-color image which might need some tweaking (mostly gamma) by the end. Most importantly, you can just use the tilscan function of your LSM and get your color tiled images. If you calibrate the stage, you can get a reasonable tiled image out of it. But I think Zeiss software limits the final frame size (in term of number of pixels). It has been a long time we did this and I might forget some details. Initial setting up (gain/offset of the detector) was a bit pain in term of getting correct colors. But once set, you can reuse it and tweak the final image in photoshop. Additionally, If I recall correctly, one critical thing is to remove DIC optics from the optical path or you might get a gradient in your tiled image. Good luck, Xuejun Xue-jun Sun, Ph.D. Dept. Exp. Oncology Cross Cancer Institute 11560 University Ave, Edmonton Alberta T6G 1Z2 Canada Phone: (780) 432-8898 Fax: (780) 432-8425 -----Original Message----- From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Alice L. Givan Sent: Wednesday, November 07, 2007 3:26 PM To: [hidden email] Subject: CCD camera Search the CONFOCAL archive at http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal We would like to add a color CCD camera to our Zeiss LSM-510 META confocal to capture color tiled wide field images. We wondered if other users have already done this? What cameras did you add and how well does the LSM 510 software control the image acquisition with the camera you are using? We are particularly interested in tiled images. We have a PixeLINK model PL-A662 color CCD camera on a separate stereo scope. We are told that this camera would not work with the LSM-510. Does anyone have any contrary information about this? Thanks for your help. Alice Alice L. Givan Englert Cell Analysis Laboratory of the Norris Cotton Cancer Center Dartmouth Medical School Lebanon, NH 03756 USA tel 603-650-7661 fax 603-650-6130 [hidden email] www.dartmouth.edu/~celllab This e-mail and any attachments may contain confidential and privileged information. If you are not the intended recipient, please notify the sender immediately by return e-mail, delete this e-mail and destroy any copies. Any dissemination or use of this information by a person other than the intended recipient is unauthorized and may be illegal. |
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In reply to this post by Alice L. Givan
Search the CONFOCAL archive at
http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal Xuejun is right, this works well to produce a pseudo colour transmission image. We have used it to obtain detailed high resolution images of histological sections (our normal widefield not having as nice objectives). The normal tilescan does limit you to 4096 x 4096 pixels I think, but you can overcome this by using the tilescan feature in the multitime macro if you have a motorised stage. Glyn. On Thu, 8 Nov 2007 09:47:55 -0700, Xuejun Sun <[hidden email]> wrote: >Hi, Alice, > >We did not use the Zeiss camera. However, we had a similar need long time >ago as some one tried to correlate histology with immunofluorescence. Here >was how we got by (without a camera): use your red, green and blue laser >lines and set up a sequential scanning configuration with your transmitted >detector. You can get a pseudo-color image which might need some tweaking >(mostly gamma) by the end. Most importantly, you can just use the tilscan >function of your LSM and get your color tiled images. If you calibrate the >stage, you can get a reasonable tiled image out of it. But I think Zeiss >software limits the final frame size (in term of number of pixels). > >It has been a long time we did this and I might forget some details. Initial >setting up (gain/offset of the detector) was a bit pain in term of getting >correct colors. But once set, you can reuse it and tweak the final image in >photoshop. Additionally, If I recall correctly, one critical thing is to >remove DIC optics from the optical path or you might get a gradient in your >tiled image. > >Good luck, > >Xuejun > > >Xue-jun Sun, Ph.D. >Dept. Exp. Oncology >Cross Cancer Institute >11560 University Ave, >Edmonton Alberta T6G 1Z2 >Canada >Phone: (780) 432-8898 >Fax: (780) 432-8425 > >-----Original Message----- >From: Confocal Microscopy List [mailto:[hidden email]] On >Behalf Of Alice L. Givan >Sent: Wednesday, November 07, 2007 3:26 PM >To: [hidden email] >Subject: CCD camera >We would like to add a color CCD camera to our Zeiss LSM-510 META >to capture color tiled wide field images. We wondered if other users have >already done this? What cameras did you add and how well does the LSM 510 >software control the image acquisition with the camera you are using? We >are particularly interested in tiled images. > >We have a PixeLINK model PL-A662 color CCD camera on a separate stereo >scope. We are told that this camera would not work with the LSM-510. Does >anyone have any contrary information about this? > >Thanks for your help. > >Alice > >Alice L. Givan >Englert Cell Analysis Laboratory >of the Norris Cotton Cancer Center >Dartmouth Medical School >Lebanon, NH 03756 USA >tel 603-650-7661 >fax 603-650-6130 >[hidden email] >www.dartmouth.edu/~celllab |
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