Mounting media for FRET experiments

> Dear list
>  
> During a recent FRET experiment a question came up about what mounting media should be used on fixed samples during FRET experiments and whether any one media is better than other for this particular type of experiment.  From what’s published it seems that people use all kinds of different media.  Does anybody here have any idea about any specific media that would be best/give least interference with FRET results?
>  
> Thanks a lot to all of you in advance,
>  
> ---------------------------------------------------
> Yevgeniy Romin
>  
> Digital Microscopist
> Memorial Sloan-Kettering Cancer Center
> Molecular Cytology Core Facility
> 1275 York Ave. Box 333
> New York, NY 10065
> Tel.646-888-2186
> Fax. 646-422-0640
> ---------------------------------------------------
>  
>
>  
>      =====================================================================
>      
>      Please note that this e-mail and any files transmitted with it may be
>      privileged, confidential, and protected from disclosure under
>      applicable law. If the reader of this message is not the intended
>      recipient, or an employee or agent responsible for delivering this
>      message to the intended recipient, you are hereby notified that any
>      reading, dissemination, distribution, copying, or other use of this
>      communication or any of its attachments is strictly prohibited.  If
>      you have received this communication in error, please notify the
>      sender immediately by replying to this message and deleting this
>      message, any attachments, and all copies and backups from your
>      computer.
>
>

> Dear list
>
> During a recent FRET experiment a question came up about what mounting media should be used on fixed samples during FRET experiments and whether any one media is better than other for this particular type of experiment.  From what's published it seems that people use all kinds of different media.  Does anybody here have any idea about any specific media that would be best/give least interference with FRET results?
>
> Thanks a lot to all of you in advance,
>
> ---------------------------------------------------
> Yevgeniy Romin
>
> Digital Microscopist
> Memorial Sloan-Kettering Cancer Center
> Molecular Cytology Core Facility
> 1275 York Ave. Box 333
> New York, NY 10065
> Tel.646-888-2186
> Fax. 646-422-0640
> ---------------------------------------------------
>
>
>
>      =====================================================================
>
>      Please note that this e-mail and any files transmitted with it may be
>      privileged, confidential, and protected from disclosure under
>      applicable law. If the reader of this message is not the intended
>      recipient, or an employee or agent responsible for delivering this
>      message to the intended recipient, you are hereby notified that any
>      reading, dissemination, distribution, copying, or other use of this
>      communication or any of its attachments is strictly prohibited.  If
>      you have received this communication in error, please notify the
>      sender immediately by replying to this message and deleting this
>      message, any attachments, and all copies and backups from your
>      computer.
>
>

> Thank you very much John, I found the paper you recommended and it is already proving useful.  A question for you then - which media were you using for the live cells?  What I mean is whether it was something like PBS or some specific media?
>
> ---------------------------------------------------
> Yevgeniy Romin
>
> Digital Microscopist
> Memorial Sloan-Kettering Cancer Center
> Molecular Cytology Core Facility
> 1275 York Ave. Box 333
> New York, NY 10065
> Tel.646-888-2186
> Fax. 646-422-0640
> ---------------------------------------------------
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of John Oreopoulos
> Sent: Friday, April 16, 2010 11:30 AM
> To: [hidden email]
> Subject: Re: Mounting media for FRET experiments
>
> I have not used fixed specimens for FRET imaging (I have used the sensitized emission method on living cells), but I came across this paper a while ago which might be of interest to you:
>
> Rodighiero, S., et al., Fixation, mounting and sealing with nail polish of cell specimens lead to incorrect FRET measurements using acceptor photobleaching. Cellular Physiology and Biochemistry, 2008. 21(5-6): p. 489-498.
>
> John Oreopoulos
>
>
> On 2010-04-16, at 11:20 AM, Yevgeniy Romin wrote:
>
>> Dear list
>>
>> During a recent FRET experiment a question came up about what mounting media should be used on fixed samples during FRET experiments and whether any one media is better than other for this particular type of experiment.  From what's published it seems that people use all kinds of different media.  Does anybody here have any idea about any specific media that would be best/give least interference with FRET results?
>>
>> Thanks a lot to all of you in advance,
>>
>> ---------------------------------------------------
>> Yevgeniy Romin
>>
>> Digital Microscopist
>> Memorial Sloan-Kettering Cancer Center
>> Molecular Cytology Core Facility
>> 1275 York Ave. Box 333
>> New York, NY 10065
>> Tel.646-888-2186
>> Fax. 646-422-0640
>> ---------------------------------------------------
>>
>>
>>
>>     =====================================================================
>>
>>     Please note that this e-mail and any files transmitted with it may be
>>     privileged, confidential, and protected from disclosure under
>>     applicable law. If the reader of this message is not the intended
>>     recipient, or an employee or agent responsible for delivering this
>>     message to the intended recipient, you are hereby notified that any
>>     reading, dissemination, distribution, copying, or other use of this
>>     communication or any of its attachments is strictly prohibited.  If
>>     you have received this communication in error, please notify the
>>     sender immediately by replying to this message and deleting this
>>     message, any attachments, and all copies and backups from your
>>     computer.
>>
>>

> Dear John,
> Dear Yevgeniy,
>
> Yes, PBS or specialized low serum (1-2%) media is broadly used
> for live cell imaging under TIR illumination.
>
> I would like to bring your attention to two papers which are
> relevant to single molecule fluorscence and/or low light live
> cell imaging - I sent them separately to your e-mail addressess
> as the LISTSERVER rejected my message due to the attachments. I
> can also send the papers to anyone by request.
>
> 1. The Use of Protocatechuate Dioxygenase for Maintaining
> Anaerobic Conditions in Biochemical ExperimentsPravin V. Patil
> and David P. BallouDepartment of Biological Chemistry,
> University of Michigan, Ann Arbor, Michigan 48109-0606
> Analytical Biochemistry 286, 187–192 (2000)
> 2. An Oxygen Scavenging System for Improvement of Dye Stability
> in Single-Molecule Fluorescence ExperimentsColin Echeverrı´a
> Aitken,* R. Andrew Marshall,y and Joseph D. Puglisiz§
> Biophysical Journal Volume 94 March 2008 1826–1835
>  
> If you have any questions, please contact me offline or phone.
>
> Also, the accuracy of the FRET eff. measurements could vary or
> be affected by the mounting media used - live cell FRET seems to
> be the best approach.
>
> Have a nice weekend,
>
> Vitaly
> 301-515-7833
>
>
>
>
>
> ________________________________
> From: John Oreopoulos <[hidden email]>
> To: [hidden email]
> Sent: Fri, April 16, 2010 12:01:32 PM
> Subject: Re: Mounting media for FRET experiments
>
> Just regular PBS solution. I have never tried a rigorous
> comparison of different media.
>
> John
>
> On 2010-04-16, at 11:54 AM, Yevgeniy Romin wrote:
>
> > Thank you very much John, I found the paper you recommended
> and it is already proving useful.  A question for you then -
> which media were you using for the live cells?  What I mean is
> whether it was something like PBS or some specific media?
> >
> > ---------------------------------------------------
> > Yevgeniy Romin
> >
> > Digital Microscopist
> > Memorial Sloan-Kettering Cancer Center
> > Molecular Cytology Core Facility
> > 1275 York Ave. Box 333
> > New York, NY 10065
> > Tel.646-888-2186
> > Fax. 646-422-0640
> > ---------------------------------------------------
> >
> > -----Original Message-----
> > From: Confocal Microscopy List
> [mailto:[hidden email]] On Behalf Of John Oreopoulos
> > Sent: Friday, April 16, 2010 11:30 AM
> > To: [hidden email]
> > Subject: Re: Mounting media for FRET experiments
> >
> > I have not used fixed specimens for FRET imaging (I have used
> the sensitized emission method on living cells), but I came
> across this paper a while ago which might be of interest to you:
> >
> > Rodighiero, S., et al., Fixation, mounting and sealing with
> nail polish of cell specimens lead to incorrect FRET
> measurements using acceptor photobleaching. Cellular Physiology
> and Biochemistry, 2008. 21(5-6): p. 489-498.
> >
> > John Oreopoulos
> >
> >
> > On 2010-04-16, at 11:20 AM, Yevgeniy Romin wrote:
> >
> >> Dear list
> >>
> >> During a recent FRET experiment a question came up about what
> mounting media should be used on fixed samples during FRET
> experiments and whether any one media is better than other for
> this particular type of experiment.  From what's published it
> seems that people use all kinds of different media.  Does
> anybody here have any idea about any specific media that would
> be best/give least interference with FRET results?
> >>
> >> Thanks a lot to all of you in advance,
> >>
> >> ---------------------------------------------------
> >> Yevgeniy Romin
> >>
> >> Digital Microscopist
> >> Memorial Sloan-Kettering Cancer Center
> >> Molecular Cytology Core Facility
> >> 1275 York Ave. Box 333
> >> New York, NY 10065
> >> Tel.646-888-2186
> >> Fax. 646-422-0640
> >> ---------------------------------------------------
> >>
> >>
> >>
> >>   
> =====================================================================>>
> >>    Please note that this e-mail and any files transmitted
> with it may be
> >>    privileged, confidential, and protected from disclosure under
> >>    applicable law. If the reader of this message is not the
> intended>>    recipient, or an employee or agent responsible for
> delivering this
> >>    message to the intended recipient, you are hereby notified
> that any
> >>    reading, dissemination, distribution, copying, or other
> use of this
> >>    communication or any of its attachments is strictly
> prohibited.  If
> >>    you have received this communication in error, please
> notify the
> >>    sender immediately by replying to this message and
> deleting this
> >>    message, any attachments, and all copies and backups from your
> >>    computer.
> >>
> >>
>
>
>
>      

> Dear John,
> Dear Yevgeniy,
>
> Yes, PBS or specialized low serum (1-2%) media is broadly used
> for live cell imaging under TIR illumination.
>
> I would like to bring your attention to two papers which are
> relevant to single molecule fluorscence and/or low light live
> cell imaging - I sent them separately to your e-mail addressess
> as the LISTSERVER rejected my message due to the attachments. I
> can also send the papers to anyone by request.
>
> 1. The Use of Protocatechuate Dioxygenase for Maintaining
> Anaerobic Conditions in Biochemical ExperimentsPravin V. Patil
> and David P. BallouDepartment of Biological Chemistry,
> University of Michigan, Ann Arbor, Michigan 48109-0606
> Analytical Biochemistry 286, 187–192 (2000)
> 2. An Oxygen Scavenging System for Improvement of Dye Stability
> in Single-Molecule Fluorescence ExperimentsColin Echeverrı´a
> Aitken,* R. Andrew Marshall,y and Joseph D. Puglisiz§
> Biophysical Journal Volume 94 March 2008 1826–1835
>
> If you have any questions, please contact me offline or phone.
>
> Also, the accuracy of the FRET eff. measurements could vary or
> be affected by the mounting media used - live cell FRET seems to
> be the best approach.
>
> Have a nice weekend,
>
> Vitaly
> 301-515-7833
>
>
>
>
>
> ________________________________
> From: John Oreopoulos <[hidden email]>
> To: [hidden email]
> Sent: Fri, April 16, 2010 12:01:32 PM
> Subject: Re: Mounting media for FRET experiments
>
> Just regular PBS solution. I have never tried a rigorous
> comparison of different media.
>
> John
>
> On 2010-04-16, at 11:54 AM, Yevgeniy Romin wrote:
>
> > Thank you very much John, I found the paper you recommended
> and it is already proving useful.  A question for you then -
> which media were you using for the live cells?  What I mean is
> whether it was something like PBS or some specific media?
> >
> > ---------------------------------------------------
> > Yevgeniy Romin
> >
> > Digital Microscopist
> > Memorial Sloan-Kettering Cancer Center
> > Molecular Cytology Core Facility
> > 1275 York Ave. Box 333
> > New York, NY 10065
> > Tel.646-888-2186
> > Fax. 646-422-0640
> > ---------------------------------------------------
> >
> > -----Original Message-----
> > From: Confocal Microscopy List
> [mailto:[hidden email]] On Behalf Of John Oreopoulos
> > Sent: Friday, April 16, 2010 11:30 AM
> > To: [hidden email]
> > Subject: Re: Mounting media for FRET experiments
> >
> > I have not used fixed specimens for FRET imaging (I have used
> the sensitized emission method on living cells), but I came
> across this paper a while ago which might be of interest to you:
> >
> > Rodighiero, S., et al., Fixation, mounting and sealing with
> nail polish of cell specimens lead to incorrect FRET
> measurements using acceptor photobleaching. Cellular Physiology
> and Biochemistry, 2008. 21(5-6): p. 489-498.
> >
> > John Oreopoulos
> >
> >
> > On 2010-04-16, at 11:20 AM, Yevgeniy Romin wrote:
> >
> >> Dear list
> >>
> >> During a recent FRET experiment a question came up about what
> mounting media should be used on fixed samples during FRET
> experiments and whether any one media is better than other for
> this particular type of experiment.  From what's published it
> seems that people use all kinds of different media.  Does
> anybody here have any idea about any specific media that would
> be best/give least interference with FRET results?
> >>
> >> Thanks a lot to all of you in advance,
> >>
> >> ---------------------------------------------------
> >> Yevgeniy Romin
> >>
> >> Digital Microscopist
> >> Memorial Sloan-Kettering Cancer Center
> >> Molecular Cytology Core Facility
> >> 1275 York Ave. Box 333
> >> New York, NY 10065
> >> Tel.646-888-2186
> >> Fax. 646-422-0640
> >> ---------------------------------------------------
> >>
> >>
> >>
> >>
> =====================================================================>>
> >>    Please note that this e-mail and any files transmitted
> with it may be
> >>    privileged, confidential, and protected from disclosure under
> >>    applicable law. If the reader of this message is not the
> intended>>    recipient, or an employee or agent responsible for
> delivering this
> >>    message to the intended recipient, you are hereby notified
> that any
> >>    reading, dissemination, distribution, copying, or other
> use of this
> >>    communication or any of its attachments is strictly
> prohibited.  If
> >>    you have received this communication in error, please
> notify the
> >>    sender immediately by replying to this message and
> deleting this
> >>    message, any attachments, and all copies and backups from your
> >>    computer.
> >>
> >>
>
>
>
>

> Dear John,
> Dear Yevgeniy,
>
> Yes, PBS or specialized low serum (1-2%) media is broadly used
> for live cell imaging under TIR illumination.
>
> I would like to bring your attention to two papers which are
> relevant to single molecule fluorscence and/or low light live
> cell imaging - I sent them separately to your e-mail addressess
> as the LISTSERVER rejected my message due to the attachments. I
> can also send the papers to anyone by request.
>
> 1. The Use of Protocatechuate Dioxygenase for Maintaining
> Anaerobic Conditions in Biochemical ExperimentsPravin V. Patil
> and David P. BallouDepartment of Biological Chemistry,
> University of Michigan, Ann Arbor, Michigan 48109-0606
> Analytical Biochemistry 286, 187-192 (2000)
> 2. An Oxygen Scavenging System for Improvement of Dye Stability
> in Single-Molecule Fluorescence ExperimentsColin Echeverri´a
> Aitken,* R. Andrew Marshall,y and Joseph D. Puglisiz§
> Biophysical Journal Volume 94 March 2008 1826-1835
>
> If you have any questions, please contact me offline or phone.
>
> Also, the accuracy of the FRET eff. measurements could vary or
> be affected by the mounting media used - live cell FRET seems to
> be the best approach.
>
> Have a nice weekend,
>
> Vitaly
> 301-515-7833
>
>
>
>
>
> ________________________________
> From: John Oreopoulos <[hidden email]>
> To: [hidden email]
> Sent: Fri, April 16, 2010 12:01:32 PM
> Subject: Re: Mounting media for FRET experiments
>
> Just regular PBS solution. I have never tried a rigorous
> comparison of different media.
>
> John
>
> On 2010-04-16, at 11:54 AM, Yevgeniy Romin wrote:
>
> > Thank you very much John, I found the paper you recommended
> and it is already proving useful.  A question for you then -
> which media were you using for the live cells?  What I mean is
> whether it was something like PBS or some specific media?
> >
> > ---------------------------------------------------
> > Yevgeniy Romin
> >
> > Digital Microscopist
> > Memorial Sloan-Kettering Cancer Center
> > Molecular Cytology Core Facility
> > 1275 York Ave. Box 333
> > New York, NY 10065
> > Tel.646-888-2186
> > Fax. 646-422-0640
> > ---------------------------------------------------
> >
> > -----Original Message-----
> > From: Confocal Microscopy List
> [mailto:[hidden email]] On Behalf Of John Oreopoulos
> > Sent: Friday, April 16, 2010 11:30 AM
> > To: [hidden email]
> > Subject: Re: Mounting media for FRET experiments
> >
> > I have not used fixed specimens for FRET imaging (I have used
> the sensitized emission method on living cells), but I came
> across this paper a while ago which might be of interest to you:
> >
> > Rodighiero, S., et al., Fixation, mounting and sealing with
> nail polish of cell specimens lead to incorrect FRET
> measurements using acceptor photobleaching. Cellular Physiology
> and Biochemistry, 2008. 21(5-6): p. 489-498.
> >
> > John Oreopoulos
> >
> >
> > On 2010-04-16, at 11:20 AM, Yevgeniy Romin wrote:
> >
> >> Dear list
> >>
> >> During a recent FRET experiment a question came up about what
> mounting media should be used on fixed samples during FRET
> experiments and whether any one media is better than other for
> this particular type of experiment.  From what's published it
> seems that people use all kinds of different media.  Does
> anybody here have any idea about any specific media that would
> be best/give least interference with FRET results?
> >>
> >> Thanks a lot to all of you in advance,
> >>
> >> ---------------------------------------------------
> >> Yevgeniy Romin
> >>
> >> Digital Microscopist
> >> Memorial Sloan-Kettering Cancer Center
> >> Molecular Cytology Core Facility
> >> 1275 York Ave. Box 333
> >> New York, NY 10065
> >> Tel.646-888-2186
> >> Fax. 646-422-0640
> >> ---------------------------------------------------
> >>
> >>
> >>
> >>
> =====================================================================>>
> >>    Please note that this e-mail and any files transmitted
> with it may be
> >>    privileged, confidential, and protected from disclosure under
> >>    applicable law. If the reader of this message is not the
> intended>>    recipient, or an employee or agent responsible for
> delivering this
> >>    message to the intended recipient, you are hereby notified
> that any
> >>    reading, dissemination, distribution, copying, or other
> use of this
> >>    communication or any of its attachments is strictly
> prohibited.  If
> >>    you have received this communication in error, please
> notify the
> >>    sender immediately by replying to this message and
> deleting this
> >>    message, any attachments, and all copies and backups from your
> >>    computer.
> >>
> >>
>
>
>
>

> Dear John,
> Dear Yevgeniy,
>
> Yes, PBS or specialized low serum (1-2%) media is broadly used
> for live cell imaging under TIR illumination.
>
> I would like to bring your attention to two papers which are
> relevant to single molecule fluorscence and/or low light live
> cell imaging - I sent them separately to your e-mail addressess
> as the LISTSERVER rejected my message due to the attachments. I
> can also send the papers to anyone by request.
>
> 1. The Use of Protocatechuate Dioxygenase for Maintaining
> Anaerobic Conditions in Biochemical ExperimentsPravin V. Patil
> and David P. BallouDepartment of Biological Chemistry,
> University of Michigan, Ann Arbor, Michigan 48109-0606
> Analytical Biochemistry 286, 187-192 (2000)
> 2. An Oxygen Scavenging System for Improvement of Dye Stability
> in Single-Molecule Fluorescence ExperimentsColin Echeverri´a
> Aitken,* R. Andrew Marshall,y and Joseph D. Puglisiz§
> Biophysical Journal Volume 94 March 2008 1826-1835
>
> If you have any questions, please contact me offline or phone.
>
> Also, the accuracy of the FRET eff. measurements could vary or
> be affected by the mounting media used - live cell FRET seems to
> be the best approach.
>
> Have a nice weekend,
>
> Vitaly
> 301-515-7833
>
>
>
>
>
> ________________________________
> From: John Oreopoulos <[hidden email]>
> To: [hidden email]
> Sent: Fri, April 16, 2010 12:01:32 PM
> Subject: Re: Mounting media for FRET experiments
>
> Just regular PBS solution. I have never tried a rigorous
> comparison of different media.
>
> John
>
> On 2010-04-16, at 11:54 AM, Yevgeniy Romin wrote:
>
> > Thank you very much John, I found the paper you recommended
> and it is already proving useful.  A question for you then -
> which media were you using for the live cells?  What I mean is
> whether it was something like PBS or some specific media?
> >
> > ---------------------------------------------------
> > Yevgeniy Romin
> >
> > Digital Microscopist
> > Memorial Sloan-Kettering Cancer Center
> > Molecular Cytology Core Facility
> > 1275 York Ave. Box 333
> > New York, NY 10065
> > Tel.646-888-2186
> > Fax. 646-422-0640
> > ---------------------------------------------------
> >
> > -----Original Message-----
> > From: Confocal Microscopy List
> [mailto:[hidden email]] On Behalf Of John Oreopoulos
> > Sent: Friday, April 16, 2010 11:30 AM
> > To: [hidden email]
> > Subject: Re: Mounting media for FRET experiments
> >
> > I have not used fixed specimens for FRET imaging (I have used
> the sensitized emission method on living cells), but I came
> across this paper a while ago which might be of interest to you:
> >
> > Rodighiero, S., et al., Fixation, mounting and sealing with
> nail polish of cell specimens lead to incorrect FRET
> measurements using acceptor photobleaching. Cellular Physiology
> and Biochemistry, 2008. 21(5-6): p. 489-498.
> >
> > John Oreopoulos
> >
> >
> > On 2010-04-16, at 11:20 AM, Yevgeniy Romin wrote:
> >
> >> Dear list
> >>
> >> During a recent FRET experiment a question came up about what
> mounting media should be used on fixed samples during FRET
> experiments and whether any one media is better than other for
> this particular type of experiment.  From what's published it
> seems that people use all kinds of different media.  Does
> anybody here have any idea about any specific media that would
> be best/give least interference with FRET results?
> >>
> >> Thanks a lot to all of you in advance,
> >>
> >> ---------------------------------------------------
> >> Yevgeniy Romin
> >>
> >> Digital Microscopist
> >> Memorial Sloan-Kettering Cancer Center
> >> Molecular Cytology Core Facility
> >> 1275 York Ave. Box 333
> >> New York, NY 10065
> >> Tel.646-888-2186
> >> Fax. 646-422-0640
> >> ---------------------------------------------------
> >>
> >>
> >>
> >>
> =====================================================================>>
> >>    Please note that this e-mail and any files transmitted
> with it may be
> >>    privileged, confidential, and protected from disclosure under
> >>    applicable law. If the reader of this message is not the
> intended>>    recipient, or an employee or agent responsible for
> delivering this
> >>    message to the intended recipient, you are hereby notified
> that any
> >>    reading, dissemination, distribution, copying, or other
> use of this
> >>    communication or any of its attachments is strictly
> prohibited.  If
> >>    you have received this communication in error, please
> notify the
> >>    sender immediately by replying to this message and
> deleting this
> >>    message, any attachments, and all copies and backups from your
> >>    computer.
> >>
> >>
>
>
>
>

>
>
>Cheers
>
>
>Cam
>
>
>
>Cameron J. Nowell
>Microscpy Manager
>Central Resource for Advanced Microscopy
>Ludwig Insttue for Cancer Research
>PO Box 2008
>Royal Melbourne Hospital
>Victoria, 3050
>AUSTRALIA
>
>Office: +61 3 9341 3155
>Mobile: +61422882700
>Fax: +61 3 9341 3104
>
>http://www.ludwig.edu.au/branch/research/platform/microscopy.htm
>
>
>________________________________
>
>From: Confocal Microscopy List on behalf of Yevgeniy Romin
>Sent: Sun 18/04/2010 1:49 AM
>To: [hidden email]
>Subject: Re: Mounting media for FRET experiments
>
>
>
>Thank you very much to everyone replying both on and off the list.  Your

>The possible reasons for the changes in FRET efficiency are very many...
>I also do most of my FRET imaging in live samples.
>
>Daniel
>
>----- Original Message -----
>From: Vitaly Boyko <[hidden email]>
>Date: Friday, April 16, 2010 19:36
>Subject: Re: Mounting media for FRET experiments
>To: [hidden email]
>
>> Dear John,
>> Dear Yevgeniy,
>>
>> Yes, PBS or specialized low serum (1-2%) media is broadly used
>> for live cell imaging under TIR illumination.
>>
>> I would like to bring your attention to two papers which are
>> relevant to single molecule fluorscence and/or low light live
>> cell imaging - I sent them separately to your e-mail addressess
>> as the LISTSERVER rejected my message due to the attachments. I
>> can also send the papers to anyone by request.
>>
>> 1. The Use of Protocatechuate Dioxygenase for Maintaining
>> Anaerobic Conditions in Biochemical ExperimentsPravin V. Patil
>> and David P. BallouDepartment of Biological Chemistry,
>> University of Michigan, Ann Arbor, Michigan 48109-0606
>> Analytical Biochemistry 286, 187-192 (2000)
>> 2. An Oxygen Scavenging System for Improvement of Dye Stability
>> in Single-Molecule Fluorescence ExperimentsColin Echeverri´a
>> Aitken,* R. Andrew Marshall,y and Joseph D. Puglisiz§
>> Biophysical Journal Volume 94 March 2008 1826-1835
>>
>> If you have any questions, please contact me offline or phone.
>>
>> Also, the accuracy of the FRET eff. measurements could vary or
>> be affected by the mounting media used - live cell FRET seems to
>> be the best approach.
>>
>> Have a nice weekend,
>>
>> Vitaly
>> 301-515-7833
>>
>>
>>
>>
>>
>> ________________________________
>> From: John Oreopoulos <[hidden email]>
>> To: [hidden email]
>> Sent: Fri, April 16, 2010 12:01:32 PM
>> Subject: Re: Mounting media for FRET experiments
>>
>> Just regular PBS solution. I have never tried a rigorous
>> comparison of different media.
>>
>> John
>>
>> On 2010-04-16, at 11:54 AM, Yevgeniy Romin wrote:
>>
>> > Thank you very much John, I found the paper you recommended
>> and it is already proving useful.  A question for you then -
>> which media were you using for the live cells?  What I mean is
>> whether it was something like PBS or some specific media?
>> >
>> > ---------------------------------------------------
>> > Yevgeniy Romin
>> >
>> > Digital Microscopist
>> > Memorial Sloan-Kettering Cancer Center
>> > Molecular Cytology Core Facility
>> > 1275 York Ave. Box 333
>> > New York, NY 10065
>> > Tel.646-888-2186
>> > Fax. 646-422-0640
>> > ---------------------------------------------------
>> >
>> > -----Original Message-----
>> > From: Confocal Microscopy List
>> [mailto:[hidden email]] On Behalf Of John Oreopoulos
>> > Sent: Friday, April 16, 2010 11:30 AM
>> > To: [hidden email]
>> > Subject: Re: Mounting media for FRET experiments
>> >
>> > I have not used fixed specimens for FRET imaging (I have used
>> the sensitized emission method on living cells), but I came
>> across this paper a while ago which might be of interest to you:
>> >
>> > Rodighiero, S., et al., Fixation, mounting and sealing with
>> nail polish of cell specimens lead to incorrect FRET
>> measurements using acceptor photobleaching. Cellular Physiology
>> and Biochemistry, 2008. 21(5-6): p. 489-498.
>> >
>> > John Oreopoulos
>> >
>> >
>> > On 2010-04-16, at 11:20 AM, Yevgeniy Romin wrote:
>> >
>> >> Dear list
>> >>
>> >> During a recent FRET experiment a question came up about what
>> mounting media should be used on fixed samples during FRET
>> experiments and whether any one media is better than other for
>> this particular type of experiment.  From what's published it
>> seems that people use all kinds of different media.  Does
>> anybody here have any idea about any specific media that would
>> be best/give least interference with FRET results?
>> >>
>> >> Thanks a lot to all of you in advance,
>> >>
>> >> ---------------------------------------------------
>> >> Yevgeniy Romin
>> >>
>> >> Digital Microscopist
>> >> Memorial Sloan-Kettering Cancer Center
>> >> Molecular Cytology Core Facility
>> >> 1275 York Ave. Box 333
>> >> New York, NY 10065
>> >> Tel.646-888-2186
>> >> Fax. 646-422-0640
>> >> ---------------------------------------------------
>> >>
>> >>
>> >>
>> >>
>> =====================================================================>>
>> >>    Please note that this e-mail and any files transmitted
>> with it may be
>> >>    privileged, confidential, and protected from disclosure under
>> >>    applicable law. If the reader of this message is not the
>> intended>>    recipient, or an employee or agent responsible for
>> delivering this
>> >>    message to the intended recipient, you are hereby notified
>> that any
>> >>    reading, dissemination, distribution, copying, or other
>> use of this
>> >>    communication or any of its attachments is strictly
>> prohibited.  If
>> >>    you have received this communication in error, please
>> notify the
>> >>    sender immediately by replying to this message and
>> deleting this
>> >>    message, any attachments, and all copies and backups from your
>> >>    computer.
>> >>
>> >>
>>
>>
>>
>>
>
>Daniel Gitler, Ph.D.
>Department of Physiology and Neurobiology
>Faculty of Health Sciences
>Ben Gurion University of the Negev
>Beer-Sheva 84105
>Israel
>
>Tel:  +972-8-6477345
>Cell: +972-54-2110100
>Fax: + 972-8-6477628
>http://web2.bgu.ac.il/physiology/faculty-members/daniel-gitler/
>
>?

> I have done FRET on Candida cells (live cells, not fixed) which are also  
> round and small in size and refuse to attach onto the coverslip. I used  
> Poly Lysine coated coverslip to adhere them on to the surface of the  
> coverslip so that the movement is less. This you can do in your lab and  
> these are commercially provided also.
> After final washing with PBS, i mounted my cells with antifade reagent  
> provided commercially ( it has some percentage of glycerol ). This has  
> worked for me very well, although i can not say about WBC's.
> Best
> Charu
>
> CHARU TANWAR
> Imaging Specialist
> Advanced Instrumentation Research Facility
> Jawaharlal Nehru University
> New Delhi 110067
> India.
>
> --- On Sat, 17/4/10, Yevgeniy Romin <[hidden email]> wrote:
>
>
> From: Yevgeniy Romin <[hidden email]>
> Subject: Re: Mounting media for FRET experiments
> To: [hidden email]
> Date: Saturday, 17 April, 2010, 9:19 PM
>
>
> Thank you very much to everyone replying both on and off the list.  Your  
> advice and the papers that were referred to were very helpful.  FRET on  
> live samples would be the ideal choice, unfortunately in this case we  
> are doing FRET on white blood cells, which are very round and refuse to  
> attach and sit still, introducing motion artifacts into the FRET  
> analysis.  We are currently working on immobilizing them, but there is a  
> fear of matrigel or a more viscous media introducing FRET measurement  
> artifacts as well.  Does anyone have experience with doing FRET on cells  
> that do not attach or immobilizing them in a least invasive way?
> ________________________________________
> From: Confocal Microscopy List [[hidden email]] On  
> Behalf Of Daniel Gitler [[hidden email]]
> Sent: Saturday, April 17, 2010 5:22 AM
> To: [hidden email]
> Subject: Re: Mounting media for FRET experiments
>
> Dear John and Yevgeniy,
>
> My experience when measuring FRET from the same samples before and after  
> fixation is that fixation itself will very much change the FRET  
> efficiency value that you measure (Cerulean and Venus in HEK cells, PBS  
> for both). Efficiency in the fixed samples was significantly lower. This  
> should not come as any big surprise, since the cellular environment  
> around the fluorophores will be very different.
> The possible reasons for the changes in FRET efficiency are very many...
> I also do most of my FRET imaging in live samples.
>
> Daniel
>
> ----- Original Message -----
> From: Vitaly Boyko <[hidden email]>
> Date: Friday, April 16, 2010 19:36
> Subject: Re: Mounting media for FRET experiments
> To: [hidden email]
>
>> Dear John,
>> Dear Yevgeniy,
>>
>> Yes, PBS or specialized low serum (1-2%) media is broadly used
>> for live cell imaging under TIR illumination.
>>
>> I would like to bring your attention to two papers which are
>> relevant to single molecule fluorscence and/or low light live
>> cell imaging - I sent them separately to your e-mail addressess
>> as the LISTSERVER rejected my message due to the attachments. I
>> can also send the papers to anyone by request.
>>
>> 1. The Use of Protocatechuate Dioxygenase for Maintaining
>> Anaerobic Conditions in Biochemical ExperimentsPravin V. Patil
>> and David P. BallouDepartment of Biological Chemistry,
>> University of Michigan, Ann Arbor, Michigan 48109-0606
>> Analytical Biochemistry 286, 187–192 (2000)
>> 2. An Oxygen Scavenging System for Improvement of Dye Stability
>> in Single-Molecule Fluorescence ExperimentsColin Echeverrı´a
>> Aitken,* R. Andrew Marshall,y and Joseph D. Puglisiz§
>> Biophysical Journal Volume 94 March 2008 1826–1835
>>
>> If you have any questions, please contact me offline or phone.
>>
>> Also, the accuracy of the FRET eff. measurements could vary or
>> be affected by the mounting media used - live cell FRET seems to
>> be the best approach.
>>
>> Have a nice weekend,
>>
>> Vitaly
>> 301-515-7833
>>
>>
>>
>>
>>
>> ________________________________
>> From: John Oreopoulos <[hidden email]>
>> To: [hidden email]
>> Sent: Fri, April 16, 2010 12:01:32 PM
>> Subject: Re: Mounting media for FRET experiments
>>
>> Just regular PBS solution. I have never tried a rigorous
>> comparison of different media.
>>
>> John
>>
>> On 2010-04-16, at 11:54 AM, Yevgeniy Romin wrote:
>>
>> > Thank you very much John, I found the paper you recommended
>> and it is already proving useful.  A question for you then -
>> which media were you using for the live cells?  What I mean is
>> whether it was something like PBS or some specific media?
>> >
>> > ---------------------------------------------------
>> > Yevgeniy Romin
>> >
>> > Digital Microscopist
>> > Memorial Sloan-Kettering Cancer Center
>> > Molecular Cytology Core Facility
>> > 1275 York Ave. Box 333
>> > New York, NY 10065
>> > Tel.646-888-2186
>> > Fax. 646-422-0640
>> > ---------------------------------------------------
>> >
>> > -----Original Message-----
>> > From: Confocal Microscopy List
>> [mailto:[hidden email]] On Behalf Of John Oreopoulos
>> > Sent: Friday, April 16, 2010 11:30 AM
>> > To: [hidden email]
>> > Subject: Re: Mounting media for FRET experiments
>> >
>> > I have not used fixed specimens for FRET imaging (I have used
>> the sensitized emission method on living cells), but I came
>> across this paper a while ago which might be of interest to you:
>> >
>> > Rodighiero, S., et al., Fixation, mounting and sealing with
>> nail polish of cell specimens lead to incorrect FRET
>> measurements using acceptor photobleaching. Cellular Physiology
>> and Biochemistry, 2008. 21(5-6): p. 489-498.
>> >
>> > John Oreopoulos
>> >
>> >
>> > On 2010-04-16, at 11:20 AM, Yevgeniy Romin wrote:
>> >
>> >> Dear list
>> >>
>> >> During a recent FRET experiment a question came up about what
>> mounting media should be used on fixed samples during FRET
>> experiments and whether any one media is better than other for
>> this particular type of experiment.  From what's published it
>> seems that people use all kinds of different media.  Does
>> anybody here have any idea about any specific media that would
>> be best/give least interference with FRET results?
>> >>
>> >> Thanks a lot to all of you in advance,
>> >>
>> >> ---------------------------------------------------
>> >> Yevgeniy Romin
>> >>
>> >> Digital Microscopist
>> >> Memorial Sloan-Kettering Cancer Center
>> >> Molecular Cytology Core Facility
>> >> 1275 York Ave. Box 333
>> >> New York, NY 10065
>> >> Tel.646-888-2186
>> >> Fax. 646-422-0640
>> >> ---------------------------------------------------
>> >>
>> >>
>> >>
>> >>
>> =====================================================================>>
>> >>    Please note that this e-mail and any files transmitted
>> with it may be
>> >>    privileged, confidential, and protected from disclosure under
>> >>    applicable law. If the reader of this message is not the
>> intended>>    recipient, or an employee or agent responsible for
>> delivering this
>> >>    message to the intended recipient, you are hereby notified
>> that any
>> >>    reading, dissemination, distribution, copying, or other
>> use of this
>> >>    communication or any of its attachments is strictly
>> prohibited.  If
>> >>    you have received this communication in error, please
>> notify the
>> >>    sender immediately by replying to this message and
>> deleting this
>> >>    message, any attachments, and all copies and backups from your
>> >>    computer.
>> >>
>> >>
>>
>>
>>
>>
>
> Daniel Gitler, Ph.D.
> Department of Physiology and Neurobiology
> Faculty of Health Sciences
> Ben Gurion University of the Negev
> Beer-Sheva 84105
> Israel
>
> Tel:  +972-8-6477345
> Cell: +972-54-2110100
> Fax: + 972-8-6477628
> http://web2.bgu.ac.il/physiology/faculty-members/daniel-gitler/
>
> ‎
>
>