Bacterial fixation issue
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** Dear Members, I am having problems with my method of fixation. I am attempting to fix my bacteria to poly - l - lysine slides. My cells are grown in 98 microtiter plates (used for antimicrobial investigations) and one well contains ~ 200 ul of 1 x 10^5 CFU/ml in media. I have attempted centrifuging to obtain a pellet, but no luck. So my last attempt was to remove the 200 ul of cells in the media and place them in fixative (2.5 % v/v FA and GA for AFM and 4 % v/v FA for confocal in 1 x PBS). I place ~ 50 - 100 ul of the sample on a slide and allow to fix to for ~ 30 min at room temperature. I then rinse with 1 x PBS and dH2O. Almost no cells are being fixed to slide and I can't understand why? If there are any suggestions, that would be great. Would it be better to avoid this method of fixation and rather use heat? I thought I could allow the solution to dry to the slide, then pass it through a flame? Thanks |
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** Shane, Might be the polylysine. How are you applying that? We have found much better results if we put our slide or coverslip (whatever we plan to polylysine coat) into a plasma for a minute. Immediately add water and let evaporate to dryness, and then add the polylysine and again let evaporate. This seems to make the coat really sticky. Of course to try this you need a handy plasma generator -- but these are often around in materials science labs or EM labs because they are used to clean surfaces. Hope this helps, Tobias On 5/27/14, 6:21 AM, Shane van Breda wrote: > ***** > To join, leave or search the confocal microscopy listserv, go to: > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy > Post images on http://www.imgur.com and include the link in your posting. > ***** > > Dear Members, > > I am having problems with my method of fixation. I am attempting to fix my bacteria to > poly - l - lysine slides. My cells are grown in 98 microtiter plates (used for antimicrobial > investigations) and one well contains ~ 200 ul of 1 x 10^5 CFU/ml in media. I have > attempted centrifuging to obtain a pellet, but no luck. So my last attempt was to remove > the 200 ul of cells in the media and place them in fixative (2.5 % v/v FA and GA for AFM > and 4 % v/v FA for confocal in 1 x PBS). I place ~ 50 - 100 ul of the sample on a slide and > allow to fix to for ~ 30 min at room temperature. I then rinse with 1 x PBS and dH2O. > > Almost no cells are being fixed to slide and I can't understand why? > > If there are any suggestions, that would be great. > > Would it be better to avoid this method of fixation and rather use heat? I thought I could > allow the solution to dry to the slide, then pass it through a flame? > > Thanks > -- __ ___ ^ ___ ___ Tobias I. Baskin / \ / / \ / \ Professor / / / / \ \ \ Biology Department / __/ /__ /___ \ \ \__ 611 N. Pleasant St. / / / \ \ \ University of Massachusetts / / / \ \ \ Amherst, MA, 01003 USA / /___ / \ \___/ \_____ 413 - 545 - 1533 www.bio.umass.edu/biology/baskin |
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** We kept E coli in nutrient broth over glass coverslips for 3 hours and they became attached. Other methods: Chemical pretreatment of glass: Vadillo-RodrÃguez, V., Busscher, H.J., Norde, W., De Vries, J., Dijkstra, R.J., Stokroos, I., Van Der Mei, H.C., 2004. Comparison of atomic force microscopy interaction forces between bacteria and silicon nitride substrata for three commonly used immobilization methods. Appl. Environ. Microbiol. 70, 5441-5446. Cytocentrifugation: Shanholtzer, C.J., Schaper, P.J., Peterson, L.R., 1982. Concentrated gram stain smears prepared with a cytospin centrifuge. J. Clin. Microbiol. 16, 1052-1056 Treatment with azide: Sjoblad, R.D., Doetsch, R.N., 1982. Adsorption of polarlyflagellated bacteria to surfaces. Curr. Microbiol. 7, 191-194. --------------------------------------- -----Original Message----- From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Shane van Breda Sent: Tuesday, May 27, 2014 6:22 AM To: [hidden email] Subject: Bacterial fixation issue ***** To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** Dear Members, I am having problems with my method of fixation. I am attempting to fix my bacteria to poly - l - lysine slides. My cells are grown in 98 microtiter plates (used for antimicrobial investigations) and one well contains ~ 200 ul of 1 x 10^5 CFU/ml in media. I have attempted centrifuging to obtain a pellet, but no luck. So my last attempt was to remove the 200 ul of cells in the media and place them in fixative (2.5 % v/v FA and GA for AFM and 4 % v/v FA for confocal in 1 x PBS). I place ~ 50 - 100 ul of the sample on a slide and allow to fix to for ~ 30 min at room temperature. I then rinse with 1 x PBS and dH2O. Almost no cells are being fixed to slide and I can't understand why? If there are any suggestions, that would be great. Would it be better to avoid this method of fixation and rather use heat? I thought I could allow the solution to dry to the slide, then pass it through a flame? Thanks |
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