Re: Kasper at al ROXS reference link

> *****
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> Hi George,
>
> Can you send a link to the PDF of the Kasper paper,
> or the full reference, I dont find it ...
>
> cheers
>
> Dan
>
>
> On Sep 13, 2011, at 7:01 AM, CONFOCALMICROSCOPY automatic digest system
> wrote:
>
> > Bleaching during acquisition - check out the ROXS paper (Kasper et al
> > 2010, Small). This and similar reagents - including some for live cell
> > imaging - should improve STED, OMX (and the other 3D-SIM), and confocal,
> > and widefield imaging. Of course ultra-stable fluorophores would be
> > problematic for PALm/STORM/Monet (the user could always change solutions
> > for the latter modes).
>
> Dr. Daniel James White BSc. (Hons.) PhD
>
> Leader - Image Processing Facility,
> Senior Microscopist,
> Light Microscopy Facility.
>
> Max Planck Institute of Molecular Cell Biology and Genetics
> Pfotenhauerstrasse 108
> 01307 DRESDEN
> Germany
>
> +49 (0)15114966933 (German Mobile)
> +49 (0)351 210 2627 (Work phone at MPI-CBG)
> +49 (0)351 210 1078 (Fax MPI-CBG LMF)
> chalkie666                                      Skype
> http://www.bioimagexd.net       BioImageXD
> http://fiji.sc                                  Fiji -  is just ImageJ
> (Batteries Included)
> http://www.chalkie.org.uk               Dan's Homepages
> https://ifn.mpi-cbg.de                  Biopolis Dresden Imaging Platform
> (BioDIP)
> dan (at) chalkie.org.uk
> ( white (at) mpi-cbg.de )
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Try this link :
>
> http://www.mpibpc.mpg.de/groups/hell/publications/pdf/smll_6_13_1379-1384.pdf
>
> Cheers,
>
> Christophe
>
> On Tue, Sep 13, 2011 at 09:55, Daniel James White<[hidden email]>  wrote:
>
>    
>> *****
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>> *****
>>
>> Hi George,
>>
>> Can you send a link to the PDF of the Kasper paper,
>> or the full reference, I dont find it ...
>>
>> cheers
>>
>> Dan
>>
>>
>> On Sep 13, 2011, at 7:01 AM, CONFOCALMICROSCOPY automatic digest system
>> wrote:
>>
>>      
>>> Bleaching during acquisition - check out the ROXS paper (Kasper et al
>>> 2010, Small). This and similar reagents - including some for live cell
>>> imaging - should improve STED, OMX (and the other 3D-SIM), and confocal,
>>> and widefield imaging. Of course ultra-stable fluorophores would be
>>> problematic for PALm/STORM/Monet (the user could always change solutions
>>> for the latter modes).
>>>        
>> Dr. Daniel James White BSc. (Hons.) PhD
>>
>> Leader - Image Processing Facility,
>> Senior Microscopist,
>> Light Microscopy Facility.
>>
>> Max Planck Institute of Molecular Cell Biology and Genetics
>> Pfotenhauerstrasse 108
>> 01307 DRESDEN
>> Germany
>>
>> +49 (0)15114966933 (German Mobile)
>> +49 (0)351 210 2627 (Work phone at MPI-CBG)
>> +49 (0)351 210 1078 (Fax MPI-CBG LMF)
>> chalkie666                                      Skype
>> http://www.bioimagexd.net       BioImageXD
>> http://fiji.sc                                  Fiji -  is just ImageJ
>> (Batteries Included)
>> http://www.chalkie.org.uk               Dan's Homepages
>> https://ifn.mpi-cbg.de                  Biopolis Dresden Imaging Platform
>> (BioDIP)
>> dan (at) chalkie.org.uk
>> ( white (at) mpi-cbg.de )
>>
>>      
>