FPs - mPlum - spectral separation

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> Hello -
>
> I was wondering what people's experience is with the far red FP variants - mPlum
> or mRasberry
> Roger Tsien's Nat. Methods paper from 2005 says mPlum is better. Have people
> successfully been using this FP?
> Would be great to hear recommendations/things to consider.
> And if one would also want to image eGFP and another FP in between, what would
> people recommend for the optimal combination of spectral separation but also
> fluor brightness/stability?
>
> I have a core user who is aiming to express all three - I realize this is a
> difficult task, just for cell health and transfection, but was hoping for FP
> choice recommendations.
>
> Thank you for any feedback -
> Feel free to contact me off list.
> Lisa
>
>
> ---------------------------------------
> Lisa Cameron, Ph.D.
> Director of Confocal and Light Microscopy Core
> Dana Farber Cancer Institute
> Boston, MA 02215
> [hidden email]
>
>
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>
> We have a couple folks who have successfully used iFP1.4 in the far
> red (Cy5) channel on our scopes.  On our four line spinning disk
> confocal (405/491/561/640) we have successfully done 4-color imaging
> in mammalian cells using mTagBFP / EGFP / mCherry / iFP1.4.  Probably
> there are better combinations out there (iRFP is supposed to be better
> than iFP1.4) but this one works well.
>
> Kurt
>
> On 11/2/2011 3:10 PM, Cameron, Lisa wrote:
>> *****
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>> *****
>>
>> Hello -
>>
>> I was wondering what people's experience is with the far red FP
>> variants - mPlum
>> or mRasberry
>> Roger Tsien's Nat. Methods paper from 2005 says mPlum is better. Have
>> people
>> successfully been using this FP?
>> Would be great to hear recommendations/things to consider.
>> And if one would also want to image eGFP and another FP in between,
>> what would
>> people recommend for the optimal combination of spectral separation
>> but also
>> fluor brightness/stability?
>>
>> I have a core user who is aiming to express all three - I realize
>> this is a
>> difficult task, just for cell health and transfection, but was hoping
>> for FP
>> choice recommendations.
>>
>> Thank you for any feedback -
>> Feel free to contact me off list.
>> Lisa
>>
>>
>> ---------------------------------------
>> Lisa Cameron, Ph.D.
>> Director of Confocal and Light Microscopy Core
>> Dana Farber Cancer Institute
>> Boston, MA 02215
>> [hidden email]
>>
>>
>> The information in this e-mail is intended only for the person to
>> whom it is
>> addressed. If you believe this e-mail was sent to you in error and
>> the e-mail
>> contains patient information, please contact the Partners Compliance
>> HelpLine at
>> http://www.partners.org/complianceline . If the e-mail was sent to
>> you in error
>> but does not contain patient information, please contact the sender
>> and properly
>> dispose of the e-mail.
>>