Alexa488 staining question

> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> It sounds like using Prolong Gold from Molecular Probes  
> (Invitrogen) would make the most sense in your situation.  If used  
> correctly, it would certainly help with the Alexa 488 signal and  
> provides a RI that should be matched to your immersion oil.
>
> No commercial affiliation.
>
> --
> Samuel A. Connell
> Director, Light Microscopy
> Cell & Tissue Imaging Center
> St. Jude Children's Research Hospital
> 332 North Lauderdale St., E7061
> Memphis, TN 38105-2794
> (901) 495-2536
> [hidden email]
>
>
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List on behalf of Farid Jalali
> Sent: Sat 10/20/2007 10:22 AM
> To: [hidden email]
> Subject: Alexa488 staining question.    .
>
> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> Hello All,
> This is a question about using Molecualr Probes Alexa 488 Donkey  
> Anti-Mouse
> secondary antibodies.
> I am using this antidody to detect a number of different targets  
> and have
> noticed that the signal intensity fades over the course of 7-10 days.
> I am using it for indirect immunofluorescent detection of targets  
> that form
> intra-nuclear foci ranging in size from ~300nm to 2um. Compared to
> the distinct, punctate, bright
> foci I image within 1-2 days after staining, 7-10 days later they are
> smaller, more diffuse and not bright at all. Using the same  
> exposure times
> and gain setting does not yeild the same quality of images.
> This is an obvious problem as I am trying to be consistent with my  
> settings
> from sample to sample for quantitation.
>
> Has anyone come across a problem like this previously? I am  
> mounting my
> coverslips with Vectashield. Has anyone come across an antifade  
> mountant
> that has an RI closer to that of immersion oil?
>
> Thanks to all.
> Cheers
> Farid
>
> --
> Farid Jalali MSc
> Senior Research Technician/ Lab Manager
> Dr. Robert Bristow Lab
> Applied Molecular Oncology
> Princess Margaret Hospital
> Toronto, Canada
> 416-946-4501 X4351 (Princess Margaret Hospital)
> 416-581-7754 STTARR at MaRS Building
> 416-581-7791 STTARR Microscopy Suite

>Search the CONFOCAL archive at
>http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>Hello All,
>This is a question about using Molecualr Probes Alexa 488 Donkey
>Anti-Mouse secondary antibodies.
>I am using this antidody to detect a number of different targets and
>have noticed that the signal intensity fades over the course of 7-10 days.
>I am using it for indirect immunofluorescent detection of targets
>that form intra-nuclear foci ranging in size from ~300nm to 2um.
>Compared to the distinct, punctate, bright
>foci I image within 1-2 days after staining, 7-10 days later they
>are smaller, more diffuse and not bright at all. Using the same
>exposure times and gain setting does not yeild the same quality of images.
>This is an obvious problem as I am trying to be consistent with my
>settings from sample to sample for quantitation.
>
>Has anyone come across a problem like this previously? I am mounting
>my coverslips with Vectashield. Has anyone come across an antifade
>mountant that has an RI closer to that of immersion oil?
>
>Thanks to all.
>Cheers
>Farid
>
>--
>Farid Jalali MSc
>Senior Research Technician/ Lab Manager
>Dr. Robert Bristow Lab
>Applied Molecular Oncology
>Princess Margaret Hospital
>Toronto, Canada
>416-946-4501 X4351 (Princess Margaret Hospital)
>416-581-7754 STTARR at MaRS Building
>416-581-7791 STTARR Microscopy Suite

> This is a question about using Molecualr Probes Alexa 488 Donkey
> Anti-Mouse secondary antibodies.
> I am using this antidody to detect a number of different targets and
> have noticed that the signal intensity fades over the course of 7-10 days.
> I am using it for indirect immunofluorescent detection of targets that
> form intra-nuclear foci ranging in size from ~300nm to 2um. Compared to
> the distinct, punctate, bright
> foci I image within 1-2 days after staining, 7-10 days later they are
> smaller, more diffuse and not bright at all. Using the same exposure
> times and gain setting does not yeild the same quality of images.
> This is an obvious problem as I am trying to be consistent with my
> settings from sample to sample for quantitation.
>  
> Has anyone come across a problem like this previously? I am mounting my
> coverslips with Vectashield. Has anyone come across an antifade mountant
> that has an RI closer to that of immersion oil?

> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> It sounds like using Prolong Gold from Molecular Probes  
> (Invitrogen) would make the most sense in your situation.  If used  
> correctly, it would certainly help with the Alexa 488 signal and  
> provides a RI that should be matched to your immersion oil.
>
> No commercial affiliation.
>
> --
> Samuel A. Connell
> Director, Light Microscopy
> Cell & Tissue Imaging Center
> St. Jude Children's Research Hospital
> 332 North Lauderdale St., E7061
> Memphis, TN 38105-2794
> (901) 495-2536
> [hidden email]
>
>
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List on behalf of Farid Jalali
> Sent: Sat 10/20/2007 10:22 AM
> To: [hidden email]
> Subject: Alexa488 staining question.    .
>
> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> Hello All,
> This is a question about using Molecualr Probes Alexa 488 Donkey  
> Anti-Mouse
> secondary antibodies.
> I am using this antidody to detect a number of different targets  
> and have
> noticed that the signal intensity fades over the course of 7-10 days.
> I am using it for indirect immunofluorescent detection of targets  
> that form
> intra-nuclear foci ranging in size from ~300nm to 2um. Compared to
> the distinct, punctate, bright
> foci I image within 1-2 days after staining, 7-10 days later they are
> smaller, more diffuse and not bright at all. Using the same  
> exposure times
> and gain setting does not yeild the same quality of images.
> This is an obvious problem as I am trying to be consistent with my  
> settings
> from sample to sample for quantitation.
>
> Has anyone come across a problem like this previously? I am  
> mounting my
> coverslips with Vectashield. Has anyone come across an antifade  
> mountant
> that has an RI closer to that of immersion oil?
>
> Thanks to all.
> Cheers
> Farid
>
> --
> Farid Jalali MSc
> Senior Research Technician/ Lab Manager
> Dr. Robert Bristow Lab
> Applied Molecular Oncology
> Princess Margaret Hospital
> Toronto, Canada
> 416-946-4501 X4351 (Princess Margaret Hospital)
> 416-581-7754 STTARR at MaRS Building
> 416-581-7791 STTARR Microscopy Suite

> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> Dear All,
>
> Just a quick question about Prolong Gold (with DAPI) and Alexa488.
>
> I know Prolong Gold is meant to be very good but I was helping a couple
> of researchers today imaging their cells, (on coverslips mounted on
> slides), which had an Alexa488 secondary and they seemed to be bleaching
> rather rapidly even though they were mounted in Prolong Gold.
>
> The samples were actually a couple of weeks old but I have had this
> experience once before. There also seemed to be a bit of a background
> problem (in the green channel) aside from any reflection which I was
> thinking might be something to do with having the DAPI in the mounting
> medium. The red fluorophore was fine.
>
> I thought the Alexa488 bleaching might be caused by having too much
> residual buffer left on the coverslip prior to mounting which then
> dilutes down the Prolong Gold?
>
> Has anyone else had this experience?
>
> Kind regards,
>
> Jacqui
>
> Jacqueline Ross
> Biomedical Imaging Research Unit
> School of Medical Sciences
> Faculty of Medical & Health Sciences
> The University of Auckland
> Private Bag 92019
> Auckland, NEW ZEALAND
>
> Tel: 64 9 373 7599 Ext 87438
> Fax: 64 9 373 7484
>
> http://www.health.auckland.ac.nz/biru/
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]] On
> Behalf Of Michael Schell
> Sent: 21 October 2007 05:51
> To: [hidden email]
> Subject: Re: Alexa488 staining question. .
>
> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> I agree.  Lose the Vectashield.  Switching to Prolong Gold will allow
> you to preserve your signal for months.  None of the mounting medias
> for fluorescence will completely solve your RI mismatch.  Prolong,
> for example, goes from 1.39 to 1.45 as it dries (see the Invitrogen
> spec sheet), but you will never reach 1.518 (oil).  Mowiol is a bit
> closer (1.49), and Pawley says that 84% sucrose is the same as oil.
> Has anybody successfully implemented 84% sucrose as a fluorescent
> mounting medium?
>
> No commercial affiliation.
>
> Michael J. Schell,
> Assist. Professor
> Dept. of Pharmacology
> Uniformed Services University
> 4301 Jones Bridge Rd.
> Bethesda, MD  20814-3220
> tel:  (301) 295-3249
> [hidden email]
>
> On Oct 20, 2007, at 12:26 PM, Connell, Samuel wrote:
>
>> Search the CONFOCAL archive at
>> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>>
>> It sounds like using Prolong Gold from Molecular Probes
>> (Invitrogen) would make the most sense in your situation.  If used
>> correctly, it would certainly help with the Alexa 488 signal and
>> provides a RI that should be matched to your immersion oil.
>>
>> No commercial affiliation.
>>
>> --
>> Samuel A. Connell
>> Director, Light Microscopy
>> Cell & Tissue Imaging Center
>> St. Jude Children's Research Hospital
>> 332 North Lauderdale St., E7061
>> Memphis, TN 38105-2794
>> (901) 495-2536
>> [hidden email]
>>
>>
>>
>>
>>
>> -----Original Message-----
>> From: Confocal Microscopy List on behalf of Farid Jalali
>> Sent: Sat 10/20/2007 10:22 AM
>> To: [hidden email]
>> Subject: Alexa488 staining question.    .
>>
>> Search the CONFOCAL archive at
>> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>>
>> Hello All,
>> This is a question about using Molecualr Probes Alexa 488 Donkey
>> Anti-Mouse
>> secondary antibodies.
>> I am using this antidody to detect a number of different targets
>> and have
>> noticed that the signal intensity fades over the course of 7-10 days.
>> I am using it for indirect immunofluorescent detection of targets
>> that form
>> intra-nuclear foci ranging in size from ~300nm to 2um. Compared to
>> the distinct, punctate, bright
>> foci I image within 1-2 days after staining, 7-10 days later they are
>> smaller, more diffuse and not bright at all. Using the same
>> exposure times
>> and gain setting does not yeild the same quality of images.
>> This is an obvious problem as I am trying to be consistent with my
>> settings
>> from sample to sample for quantitation.
>>
>> Has anyone come across a problem like this previously? I am
>> mounting my
>> coverslips with Vectashield. Has anyone come across an antifade
>> mountant
>> that has an RI closer to that of immersion oil?
>>
>> Thanks to all.
>> Cheers
>> Farid
>>
>> --
>> Farid Jalali MSc
>> Senior Research Technician/ Lab Manager
>> Dr. Robert Bristow Lab
>> Applied Molecular Oncology
>> Princess Margaret Hospital
>> Toronto, Canada
>> 416-946-4501 X4351 (Princess Margaret Hospital)
>> 416-581-7754 STTARR at MaRS Building
>> 416-581-7791 STTARR Microscopy Suite
>

> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> Is sample shrinkage a general problem with mounting media which harden? I am
> not a fan of the PBS+glycerol+antifade combo because it's so messy - difficult
> to remove immersion oil, broken bits of nailpolish all over the stage and the
> lenses . . . . .
>
> Judy
>
> Judy Trogadis
> Bio-Imaging Coordinator
> St. Michael's Hospital, 7Queen
> 30 Bond St.
> Toronto, ON M5B 1W8, Canada
> ph:  416-864-6060  x6337
> pager: 416-685-9219
> fax: 416-864-6043
> [hidden email]
>
>
>>>> Sarah Aubut <[hidden email]> 10/23/07 8:56 AM >>>
> Search the CONFOCAL archive at
> http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal
>
> I recently attended a short course on Basic confocal at the Microscopy
> meeting in Fort Lauderdale, and the instructors advised against using
> Prolong and all other mountants that contain polyvinyl alcohol as this
> causes shrinkage up to 50% in your sample.
> What they suggested was something that matched the RI of the sample. One
> specific was PBS + glycerol (30%) with 0.25% p-phenylenediamine. DABCO was
> also mentioned as an alternative.
> I don't know if this information helps at all, but I thought I should
> contribute the little that I know!
>
>
> Sarah Aubut
> Lab Technician, Microscopy Suite
> Canadian Forestry Service
> Sault Ste Marie, ON
> Canada
>
> [hidden email]