Alternative immersion media for a water immersion lens

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> Hello all,
> Is anyone aware of a suitable alternative immersion media for a water
> immersion lens? This lab is doing experiments at room temperature and the
> scope is not enclosed therefore no humidity control.
> Thanks very much all.
>
> Farid Jalali
>
>    

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>Hello all,
>Is anyone aware of a suitable alternative immersion media for a water
>immersion lens? This lab is doing experiments at room temperature and the
>scope is not enclosed therefore no humidity control.
>Thanks very much all.
>
>Farid Jalali

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> Hello All. Thank you very much to everyone for your replies and insightful
> suggestions. It never ceases to amaze me what a wonderful community this
> is.
> Have a great day all.
> Cheers
> Farid
>
> On Thu, Jul 21, 2011 at 9:42 PM, Farid Jalali <[hidden email]>
> wrote:
>
> > Hello all,
> > Is anyone aware of a suitable alternative immersion media for a water
> > immersion lens? This lab is doing experiments at room temperature and the
> > scope is not enclosed therefore no humidity control.
> > Thanks very much all.
> >
> > Farid Jalali
> >
>

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> Hi there,
>
> I have used 1:5 ultrasound gel too in the past. The Ri is not identical to water but close enough for many applications. Just make sure you use water for dilution. With NaCl solution, somehow the gel structure breaks down and you get an aqueous liquid with a precipitate, at least with our ultrasound gel.
>
> I don't know though what the 1:5 dilution in water does to exposed tissues in terms of physiology, as opposed to superfusion with buffer. Did anybody investigate?
>
> Steffen
>
>
> On 22.07.2011 09:08, Cameron Nowell wrote:
>>
>> Hi Farid,
>>
>> For small volumes we use the Zeiss Immersol W. But for large scale stuff
>> like using the large 20x water objective on our multiphoton system we
>> use a 1:5 dilution of ultrasound gel (make sure you use the clear one,
>> not the blue tinted stuff).
>>
>
>
> --
> ------------------------------------------------------------
> Steffen Dietzel, PD Dr. rer. nat
> Ludwig-Maximilians-Universität München
> Walter-Brendel-Zentrum für experimentelle Medizin (WBex)
> Head of light microscopy
>
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> Marchioninistr. 15, D-81377 München
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> Date: Sat, 23 Jul 2011 08:25:40 +1000
> From: [hidden email]
> Subject: Re: Alternative immersion media for a water immersion lens
> To: [hidden email]
>
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>
> The other way to do it is a continual water source.
> We have the Leica 63x with computer controlled water pump (no commercial
> interest), but also use a lab-made system using a pipette, reservoir and
> pump (designed by Steve Cody).
>
> We also use the Zeiss immersol and Cargille water RI oils but find they dry
> over time and the quality of the image deteriorates. The water pump also
> allow imaging multipoint experiments where there is considerable movement of
> the objective.
> Cheers,
> Stephen
>
> On 23 July 2011 03:19, Farid Jalali <[hidden email]> wrote:
>
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > *****
> >
> > Hello All. Thank you very much to everyone for your replies and insightful
> > suggestions. It never ceases to amaze me what a wonderful community this
> > is.
> > Have a great day all.
> > Cheers
> > Farid
> >
> > On Thu, Jul 21, 2011 at 9:42 PM, Farid Jalali <[hidden email]>
> > wrote:
> >
> > > Hello all,
> > > Is anyone aware of a suitable alternative immersion media for a water
> > > immersion lens? This lab is doing experiments at room temperature and the
> > > scope is not enclosed therefore no humidity control.
> > > Thanks very much all.
> > >
> > > Farid Jalali
> > >
> >
>
>
>
> --
> Stephen Firth
> Manager of Advanced Optical Microscopy
> Monash Micro Imaging
> Monash University
> Room G58 Building 75
> Phone 990 55612
> Mob 0400 695 425

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>
> Hi Leoncio,
> While I can't suggest a solution, I am interested in your comments on the dyes you have tried for your live cell imaging, specifically, the UV/violet excited dyes Hoechst and DAPI.
>
> My experience has been that Hoechst 33342 will stain nuclei in living cells and has not proved toxic over 24 hours of imaging, albeit using very low laser powers and only infrequent imaging. Were you using Hoechst 33342 or Hoechst 33258 (or the slightly longer wavelength excited Hoechst 34580)? Also, what concentration were you using? Frigault et al (J Cell Sci, 122, 753-767, 2009) suggest that to avoid toxicity effects in live cell imaging, these dyes may need to be used at 10-100x more dilute concentrations than usually recommended.
>
> Also you mentioned using DAPI for nuclear staining. This probe is relatively live cell membrane impermeant and usually requires quite high concentrations to get significant nuclear labelling in living cells. At high concentrations DAPI is also toxic so I am not surprised you had problems with this dye.
>
> As an aside, has anyone seen inhibition of cell division when using these

> Some people suggest that cell division is inhibited, but others have not reported any problems. What is the concensus?
>
> Regards
> Paul
>
> Assoc. Prof. Paul Rigby
> Centre for Microscopy, Characterisation&  Analysis (M510)
> The University of Western Australia
> 35 Stirling Highway
> Crawley  WA  6007
> Australia
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Vergara, Leoncio A.
> Sent: Tuesday, 26 July 2011 5:20 AM
> To: [hidden email]
> Subject: Long term Nuclear labeling in live cells
>
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>
> I was wondering if there is any non toxic alternative help in segmentation of nucleus and cytosol compartments to measure protein translocation dynamics in 12-24 hrs time lapse experiments in live cultured cells.
>
> We are working with cell lines stably expressing both GFP and Strawberry fluorescent protein constructs. We want to follow the single cell translocation process and correlate the two signals over a period of 12-24 hrs. We are looking for a tool to aid in segmentation between both compartments for automated image analysis. The problem is that all the DNA binding dyes we have tried are cytotoxic. We have tried DRAQ5, DAPI, HOESCHT and several SITO dyes from molecular probes. We have not tried the Vybrant(r) DyeCycle stains from Invitrogen, violet and Ruby could be compatible with GFP and Strawberry, but a call to their technical support was not very encouraging.
>
> I am wondering if there are any long term live cell tracking dyes that can label the cytosol and give a "negative" image of the nucleus, be non toxic and be compatible with GFP and Strawberry.
>
> Invitrogen also has the CellLight reagents but they are base either on GFP or RFP so won't be a solution either since we are using those channels. I guess we could develop a far-red construct for triple FP labeling, but I was hoping for an easier solution... :)
>
> For additional reference: the microscope we are using is a Prairie Technologies Swept Field Confocal, we have 4 channels available (typical DAPI/FITC/TRITC/Cy5) to work. This is not an spectral imaging system.
>
> Thanks in advance, any suggestion would be greatly appreciated
>
> Leoncio Vergara
> Technical Director
> Optical Microscopy Core
> Galveston
> Texas
>
>    

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>
> Hi Leoncio
>
> Dapi is probably not good because you use UV light for imaging, and cells
> do
> dye under UVs.
>
> I have imaged cells for 24h (time points every 3 min) labeled with
> GFP-Histone 2B. If you can get histone 2B with a in fusion with a
> fluorescent protein that goes to the CY5 channel it should work.
>
> You could also try Histone GFP and do a bright field /DIC image where you
> can clearly see the nucleus and the cytoplasm. Or DIC alone merged with the
> other 2 florescent channels images that you have can also help you to
> distinguish between the nucleus and the cytoplasm.
>
> Good luck
>
> Claudia.
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]]
> On
> Behalf Of Vergara, Leoncio A.
> Sent: segunda-feira, 25 de Julho de 2011 22:20
> To: [hidden email]
> Subject: Long term Nuclear labeling in live cells
>
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> I was wondering if there is any non toxic alternative help in segmentation
> of nucleus and cytosol compartments to measure protein translocation
> dynamics in 12-24 hrs time lapse experiments in live cultured cells.
>
> We are working with cell lines stably expressing both GFP and Strawberry
> fluorescent protein constructs. We want to follow the single cell
> translocation process and correlate the two signals over a period of 12-24
> hrs. We are looking for a tool to aid in segmentation between both
> compartments for automated image analysis. The problem is that all the DNA
> binding dyes we have tried are cytotoxic. We have tried DRAQ5, DAPI,
> HOESCHT
> and several SITO dyes from molecular probes. We have not tried the
> Vybrant(r) DyeCycle stains from Invitrogen, violet and Ruby could be
> compatible with GFP and Strawberry, but a call to their technical support
> was not very encouraging.
>
> I am wondering if there are any long term live cell tracking dyes that can
> label the cytosol and give a "negative" image of the nucleus, be non toxic
> and be compatible with GFP and Strawberry.
>
> Invitrogen also has the CellLight reagents but they are base either on GFP
> or RFP so won't be a solution either since we are using those channels. I
> guess we could develop a far-red construct for triple FP labeling, but I
> was
> hoping for an easier solution... :)
>
> For additional reference: the microscope we are using is a Prairie
> Technologies Swept Field Confocal, we have 4 channels available (typical
> DAPI/FITC/TRITC/Cy5) to work. This is not an spectral imaging system.
>
> Thanks in advance, any suggestion would be greatly appreciated
>
> Leoncio Vergara
> Technical Director
> Optical Microscopy Core
> Galveston
> Texas
>
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> To join, leave or search the confocal microscopy listserv, go to:
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>
> Hi Paul,
>
> I have used Hoechst 33342 in the past for live imaging both primary and
> cultured cells. After about 24 hours they will dye (usually quite
> spectacularly). But i have managed to image cells divinging with
> Hoechst, but the best is only ever one round of division.
>
> Cheers
>
> Cam
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]]
> On Behalf Of Paul Rigby
> Sent: Tuesday, 26 July 2011 11:46 AM
> To: [hidden email]
> Subject: Re: Long term Nuclear labeling in live cells
>
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Hi Leoncio,
> While I can't suggest a solution, I am interested in your comments on
> the dyes you have tried for your live cell imaging, specifically, the
> UV/violet excited dyes Hoechst and DAPI.
>
> My experience has been that Hoechst 33342 will stain nuclei in living
> cells and has not proved toxic over 24 hours of imaging, albeit using
> very low laser powers and only infrequent imaging. Were you using
> Hoechst 33342 or Hoechst 33258 (or the slightly longer wavelength
> excited Hoechst 34580)? Also, what concentration were you using?
> Frigault et al (J Cell Sci, 122, 753-767, 2009) suggest that to avoid
> toxicity effects in live cell imaging, these dyes may need to be used at
> 10-100x more dilute concentrations than usually recommended.
>
> Also you mentioned using DAPI for nuclear staining. This probe is
> relatively live cell membrane impermeant and usually requires quite high
> concentrations to get significant nuclear labelling in living cells. At
> high concentrations DAPI is also toxic so I am not surprised you had
> problems with this dye.
>
> As an aside, has anyone seen inhibition of cell division when using
> these DNA intercalating dyes? Some people suggest that cell division is
> inhibited, but others have not reported any problems. What is the
> concensus?
>
> Regards
> Paul
>
> Assoc. Prof. Paul Rigby
> Centre for Microscopy, Characterisation & Analysis (M510)
> The University of Western Australia
> 35 Stirling Highway
> Crawley  WA  6007
> Australia
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]]
> On Behalf Of Vergara, Leoncio A.
> Sent: Tuesday, 26 July 2011 5:20 AM
> To: [hidden email]
> Subject: Long term Nuclear labeling in live cells
>
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> I was wondering if there is any non toxic alternative help in
> segmentation of nucleus and cytosol compartments to measure protein
> translocation dynamics in 12-24 hrs time lapse experiments in live
> cultured cells.
>
> We are working with cell lines stably expressing both GFP and Strawberry
> fluorescent protein constructs. We want to follow the single cell
> translocation process and correlate the two signals over a period of
> 12-24 hrs. We are looking for a tool to aid in segmentation between both
> compartments for automated image analysis. The problem is that all the
> DNA binding dyes we have tried are cytotoxic. We have tried DRAQ5, DAPI,
> HOESCHT and several SITO dyes from molecular probes. We have not tried
> the Vybrant(r) DyeCycle stains from Invitrogen, violet and Ruby could be
> compatible with GFP and Strawberry, but a call to their technical
> support was not very encouraging.
>
> I am wondering if there are any long term live cell tracking dyes that
> can label the cytosol and give a "negative" image of the nucleus, be non
> toxic and be compatible with GFP and Strawberry.
>
> Invitrogen also has the CellLight reagents but they are base either on
> GFP or RFP so won't be a solution either since we are using those
> channels. I guess we could develop a far-red construct for triple FP
> labeling, but I was hoping for an easier solution... :)
>
> For additional reference: the microscope we are using is a Prairie
> Technologies Swept Field Confocal, we have 4 channels available (typical
> DAPI/FITC/TRITC/Cy5) to work. This is not an spectral imaging system.  
>
> Thanks in advance, any suggestion would be greatly appreciated
>
> Leoncio Vergara
> Technical Director
> Optical Microscopy Core
> Galveston
> Texas
>
>
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