Posted by Stewart, Angela on
URL: http://confocal-microscopy-list.275.s1.nabble.com/Frap-analysis-tp591758p591762.html

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Thank you,

Angie Stewart
PerkinElmer Life and Analytical Sciences
Life Science Instrument Sales
Mobile: 561-309-1013
Office: 561-745-9177
Email: [hidden email]
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-----Original Message-----
From: Confocal Microscopy List [mailto:[hidden email]] On
Behalf Of Anchall ............
Sent: Friday, January 25, 2008 4:38 AM
To: [hidden email]
Subject: Re: Frap analysis

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Dear Kevin,
         Thanks a lot for replying.I work with different RAS proteins
which are mostly localised in plasma membrane and some intracellular
organelles like golgi and ER.All these proteins have c terminal post
translational modifications .Now what I want to see is if different
post translational mutants of these proteins have similar or different
kinetics inside living cells.I am using MDCK cells for these expt.I
want to frap the mutants and the wt and see if there is any difference
in the diffusion kinetics and to find out if these modifications have
any role to play in defining localisation and kinetics of these
proteins.I will like to quantify the data once I get these frap
mesurements. Regarding which frap model I should use I am bit
confused.I dont know which model I should use to fit my data.
Also I didnt understand how sample geometry can help me select the
frap method .You also mentioned about checking some reference
solutions first. Can you guide me what kind of samples I should use
for reference.
Hope you will reply soon
Regards
Anchal

On Jan 25, 2008 7:47 AM, Kevin Braeckmans <[hidden email]>
wrote:
> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> Dear Anchal,
>
> It would be helpful if you could give some more details - what are you
> trying to measure, what kind of sample are you using, do you want to
obtain
> quantitative data and if so, which FRAP method would you like to use
etc.
>
> Very generally, the difficulty is not the image processing, which
usually is
> just averaging the fluorescence intensity in some ROI and normalizing
that
> to a reference area and the fluorescence before bleaching. If you want
to
> obtain quantitative data, the real challenge is to perform the
experiment
> according to the limits implied in the FRAP model (which are not
always
> clearly discussed in articles). Only then one can expect to obtain
> reasonable values from a best fit of the model to the recovery curve
> (obtaining a value does not necessarily mean it is a correct one).
>
> If you are starting from scratch, I would advise the following:
> 1. Define your experiment, the sample geometry being the most
important
> factor (3D extended sample, sample with limited thickness, sample of
limited
> volume)
> 2. Choose a FRAP method which is suitable for your experiment and
which can
> be performed by your instrument.
> 3. Practice on some reference solutions of known diffusion coefficient
to
> see if the method works correctly (each FRAP method has some limits
which
> are implied in the mathematical derivation - make sure to perform your
> experiment accordingly)
> 4. Apply the method to your actual samples.
>
> You also might want to check out the archives since this topic has
been if
> > someone can tell me step by step procedure to analyse frap data .I
use
> > leica
> > sp5 for collecting frap data.
> > Hope to hear from you all soon
> > Thanks
> > Anchal
>