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Hello all,
In order to do my experiment,I need to embed some fluorescent beads(.2 micron) inside my sample(which is Arabidopsis leaf).I was thinking of a simple way,just injecting the solution to the stem of the leaf(using a microlitre syringe and a 33 G needle).I am wondering if any one has any other suggestion to do that more efficiently?
Thanks
Sarah
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Search the CONFOCAL archive at
http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal Sarah You might simply cut the petiole with razor blade and immerse the cut end in the bead suspension contained in a microfuge tube. I load compounds into leaves using this technique all the time. Russ Russell N. Spear Sr. Research Specialist Dept. of Plant Pathology Univ. of Wisconsin 1630 Linden Dr. Madison WI 53706 voice 608.263.2093 fax 608.263.2626 >>> Sarah Kefayati <[hidden email]> 11/08/07 11:20 AM >>> Search the CONFOCAL archive at http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal Hello all, In order to do my experiment,I need to embed some fluorescent beads(.2 micron) inside my sample(which is Arabidopsis leaf).I was thinking of a simple way,just injecting the solution to the stem of the leaf(using a microlitre syringe and a 33 G needle).I am wondering if any one has any other suggestion to do that more efficiently? Thanks Sarah |
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In reply to this post by Sarah Kefayati
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This depends on exactly what you mean by “embedding beads” in the leaf. If you just want to see the beads in the xylem, you can let the cut petiole take them up from solution as Russell suggests. However, they won’t get out of the xylem into other tissues – 200 nm is probably too big for that. I say “probably”, because the xylem parenchyma can take up 3kD dextrans from xylem vessels under the right conditions, presumably by endocytosis. However, cell wall porosity is usually limited to under 8 nm, so 200 nm probably won’t get through the xylem walls, even at the porous pits. cheers, Rosemary Rosemary White [hidden email] CSIRO Plant Industry ph. 61 (0)2-6246 5475 GPO Box 1600 fax. 61 (0)2-6246 5334 Canberra, ACT 2601 Australia On 9/11/07 4:20 AM, "Sarah Kefayati" <[hidden email]> wrote: Search the CONFOCAL archive at http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal |
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Search the CONFOCAL archive at
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Dear Rosemary:
Thanks for the great information,
actually I was thinking of this problem too,but I just tried the injection way once and I could tell it somehow worked,I mean I could see some of the beads when I imaged my sample by the two-photon microscopy,but the solution was too diluted,this time I was thinking of using more concentrated solution(5 microlitre bead solution and 5 microlitre water),I just have one more question:if we assume that xylem can take up the beads ,if I see them this means that I am looking at the beads in which part?
thanks
Sarah
On Nov 8, 2007 5:35 PM, Rosemary White <[hidden email]> wrote:
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What are you trying to label with these beads? What’s the experiment? Depending on how long you let the leaves take up the solution, you’ll see them throughout the xylem. You really need to shine a bright light on the leaves while their petioles are in solution, then they’ll take it up faster and to a greater extent. So, you’ll see the beads in the xylem. cheers, Rosemary On 9/11/07 12:18 PM, "Sarah Kefayati" <[hidden email]> wrote: Search the CONFOCAL archive at http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal |
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