beads for localized stimulation of proteins

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> Hi,
>
> This isn't a confocal problem, but I have seen great suggestions for many
> imaging issues so I figured I'll post mine.
>
> I am trying to image the effects of a localized ligand stimulation on
> migrating cells (osteoblasts). To localize the ligand, I am using protein
> A/G coated magnetic beads (1um dia). However the beads are aggregating, and
> moving around too much when imaging. Also they are completely messing up
> the DIC image (not too important apart from knowing the location of the
> bead and the region of contact.)
>
> I was wondering if any of you have any suggestions to make this set up
> work. Ideally, the beads should be ~2-5 um diameter, have either some
> functional group which I can use to immobilize the protein and be heavy
> enough that it settles down in a culture and doesn't move about too much.
> Also, something that doesn't interfere too much with fluorescent imaging
> (438 nm and 515 nm currently) would be great.
>
> I apologize for the rather long post.
>
> Thanks
> Abhijit Deb Roy
> PhD Candidate
> Biomedical Sciences Program
> University of Connecticut Health Centre, Farmington
>

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> To join, leave or search the confocal microscopy listserv, go to:
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>
> Abhijith,
>
> Have you tried localizing beads with poly lysine. I do lot of fluorescence
> imaging of beads, poly lysine coated coverslips worked well for me. To
> avoid the aggregation try sonication or votexing.
>
> Hope it helps,
>
> Aleem
>
>
>
> On Tue, Jun 4, 2013 at 11:11 AM, abhijit debroy <[hidden email]>wrote:
>
>> *****
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>> *****
>>
>> Hi,
>>
>> This isn't a confocal problem, but I have seen great suggestions for many
>> imaging issues so I figured I'll post mine.
>>
>> I am trying to image the effects of a localized ligand stimulation on
>> migrating cells (osteoblasts). To localize the ligand, I am using protein
>> A/G coated magnetic beads (1um dia). However the beads are aggregating, and
>> moving around too much when imaging. Also they are completely messing up
>> the DIC image (not too important apart from knowing the location of the
>> bead and the region of contact.)
>>
>> I was wondering if any of you have any suggestions to make this set up
>> work. Ideally, the beads should be ~2-5 um diameter, have either some
>> functional group which I can use to immobilize the protein and be heavy
>> enough that it settles down in a culture and doesn't move about too much.
>> Also, something that doesn't interfere too much with fluorescent imaging
>> (438 nm and 515 nm currently) would be great.
>>
>> I apologize for the rather long post.
>>
>> Thanks
>> Abhijit Deb Roy
>> PhD Candidate
>> Biomedical Sciences Program
>> University of Connecticut Health Centre, Farmington
>
>
>
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> *Aleem Syed
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>
> I am afraid, I don't use any culture media on top of the beads. I use
> polymer beads as standards for fluorescence imaging. I do sonicate ligand
> coated quantum dots all the time and  never saw any ligand dissociation,
> Though you need to optimise the temperature for sonicatoin and
> concentration for your application, generally lower temperatures (ca. 10-18
> degree Celsius) work fine.
>
> Best,
> Aleem
>