spectral unmixing with Zeiss 510 meta

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>
> Dear List--
>
> I am trying to learn how to use the spectral unmixing function on the
> Zeiss 510.  I've loaded individual spectra of the three fluorophores that
> I'm using.  I then took an image of a region in which there's a lot of
> triple labeling and loaded the stored spectra to allow linear unmixing.
>  The program displays a resulting image.  However, the program appears not
> to display structures in which there are coexisting labels--only the few
> regions in which there is single-labeling.
>
> Am I missing something?  Or is this how the program is designed to work?
>
> Any suggestions welcome!
>
> Thanks--
>
> Martin Wessendorf
> --
> 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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> To join, leave or search the confocal microscopy listserv, go to:
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>
> It really depends on how the algorithm handles assignment.  For each pixel,
> the algorithm has to decide whether to false-color it (for example) red,
> blue, or green, depending on whether the algorithm decides that that pixel
> is mostly the flurophore assigned to red, or blue, or green.  Some
> algorithms can't make a proportional call, for instance they can't give you
> information that a pixel is 40% the blue-assigned flurophore and 60% the
> red-assigned fluorphore.  In this case it would show the pixel only as red,
> because the red-assigned fluorphore dominates that pixel.  I'm not familiar
> with the Zeiss spectral unmix algorithm, but unless there's just a setting
> somewhere I suspect this is what it is doing to you.  Our in-house software
> will actually 'dither' pixels by proportion of fluorophore present in each
> pixel to deal with this problem.  The Zeiss software may also be able to do
> this, but I'm not sure.
>
> Craig
>
>
> On Wed, May 23, 2012 at 9:32 AM, Martin Wessendorf <[hidden email]> wrote:
>
>> *****
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/**wa?A0=confocalmicroscopy<http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy>
>> *****
>>
>> Dear List--
>>
>> I am trying to learn how to use the spectral unmixing function on the
>> Zeiss 510.  I've loaded individual spectra of the three fluorophores that
>> I'm using.  I then took an image of a region in which there's a lot of
>> triple labeling and loaded the stored spectra to allow linear unmixing.
>>  The program displays a resulting image.  However, the program appears not
>> to display structures in which there are coexisting labels--only the few
>> regions in which there is single-labeling.
>>
>> Am I missing something?  Or is this how the program is designed to work?
>>
>> Any suggestions welcome!
>>
>> Thanks--
>>
>> Martin Wessendorf
>> --
>> 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]
>>

> On Wed, May 23, 2012 at 11:21 AM, Craig Brideau<[hidden email]>  wrote:
>> *****
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>> *****
>>
>> It really depends on how the algorithm handles assignment.  For each pixel,
>> the algorithm has to decide whether to false-color it (for example) red,
>> blue, or green, depending on whether the algorithm decides that that pixel
>> is mostly the flurophore assigned to red, or blue, or green.  Some
>> algorithms can't make a proportional call, for instance they can't give you
>> information that a pixel is 40% the blue-assigned flurophore and 60% the
>> red-assigned fluorphore.  In this case it would show the pixel only as red,
>> because the red-assigned fluorphore dominates that pixel.  I'm not familiar
>> with the Zeiss spectral unmix algorithm, but unless there's just a setting
>> somewhere I suspect this is what it is doing to you.  Our in-house software
>> will actually 'dither' pixels by proportion of fluorophore present in each
>> pixel to deal with this problem.  The Zeiss software may also be able to do
>> this, but I'm not sure.
>>
>> Craig
>>
>>
>> On Wed, May 23, 2012 at 9:32 AM, Martin Wessendorf<[hidden email]>  wrote:
>>
>>> *****
>>> To join, leave or search the confocal microscopy listserv, go to:
>>> http://lists.umn.edu/cgi-bin/**wa?A0=confocalmicroscopy<http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy>
>>> *****
>>>
>>> Dear List--
>>>
>>> I am trying to learn how to use the spectral unmixing function on the
>>> Zeiss 510.  I've loaded individual spectra of the three fluorophores that
>>> I'm using.  I then took an image of a region in which there's a lot of
>>> triple labeling and loaded the stored spectra to allow linear unmixing.
>>>   The program displays a resulting image.  However, the program appears not
>>> to display structures in which there are coexisting labels--only the few
>>> regions in which there is single-labeling.
>>>
>>> Am I missing something?  Or is this how the program is designed to work?
>>>
>>> Any suggestions welcome!
>>>
>>> Thanks--
>>>
>>> Martin Wessendorf
>>> --
>>> 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]
>>>