> You won't be able to separate GFP and YFP reliably without a spectral
> system; the emission wavelengths aren't separated by enough to do this
> with conventional filters.
>
> There are other fluorescent protein combinations you could consider
> which might be better behaved, such as one of the new BFPs or a
> UV-excited GFP like Sapphire which would let you do 4 proteins with
> better separation between channels.  I think you can also multiplex CFP,
> GFP, mkOrange, and a far red FP like TagFP635 or tHcRed.  You could
> probably add BFP or Sapphire to that mix to do 5 proteins, although you
> will probably start getting some crosstalk you need to deal with.
>
> Kurt
>
> Christian wrote:
>>
>> Recently a new faculty member has introduced new constructs of both
>> YFP and CFP for localization in plant cells, mostly tobacco and
>> arabidopsis.  Our current system, a FluoView 500 is not set up for
>> this work, so I've been asked to investigate new avenues.
>>
>> In any case, I think we've all seen a spectral system separate GFP,
>> Sytox Green and FITC in the same cell, but for CFP, YFP, GFP, RFP
>> colocalization in plant cells would a spectral system offer more
>> utility than a system with better filter sets and laser lines?
>>
>> Obviously there is a cost question in relation to utility here.  Also,
>> here in Midwest of the US, we have primarily Zeiss, Olympus and Nikon
>> systems.  If anyone would like comment on those in particular, that'd
>> be great.
>>
>> I also have a more specific question, with several groups targeting
>> chloroplasts, I should probably just lean towards a spectral system?
>> Finally, do YFP and GFP overlap too greatly in plants (pH
>> difference?!?) to be separated by either system?
>>
>> If any has some negative feedback, or suggestions, please feel free to
>> email me privately.  I find folks are awfully nice on the list, but
>> when we're talking several hundred thousand dollars, I need brutal
>> honesty.
>>
>> Thank you.
>>
>> Christian
>>
>