how to measure acidification in endosomes?

Dear colleagues,

to demonstrate a receptor has indeed been internalized (and he is not
just looking at a structure still continuous with the plasma membrane),
a user of our facilities wants to measure the acidification of the
endosome compartment (its co-localized with EEA1).

Which is a good protocol to do so?
Which alternative strategy would be applicable?

Any suggestion welcome,
Thanks, jens

---
dr. jens rietdorf
head microscopy
novartis research foundation
friedrich-miescher-institute, wro1066.2.16
maulbeerstr.66, 4058 basel, switzerland
couriel:rietdorf(at)fmi(dot)ch
fon: +41.61.69.75172
fax: +41.61.69.73976

Dear Dr Rietdorf and others,

indeed, also in our research we are very much interested in measuring endosomal pH.

One strategy, I was thinking, was using a pH sensitive dye, with a precise defined pKa value like Lysosensor green (LysoSensor™ Green DND-189  pKa 5.2; LysoSensor™ Green DND-153  pKA 7.5), or use SNARF-1, conjugated to a low MW dextran, in that way you get a pH shift when the endosome is acidifying (pKa 7,5). According to Mol Probes (http://probes.invitrogen.com/media/pis/mp01270.pdf) it should even be possible to calculate the pH after calibrating and solely measuring emission intensities at two different wavelenghts.. However, I didn't do this myself yet..

LysoSensor™ Green DND-189  pKa 5.2; LysoSensor™ Green DND-153  pKA 7.5

Another possibility is measuring fluorescence of simultaneously added FITC and TMR:
Sonawane, N. D., Szoka, F. C., and Verkman, A. S. (2003). Chloride accumulation and swelling in endosomes enhances DNA transfer by polyamine-DNA polyplexes. Journal of Biological Chemistry. 278: 44826-44831.

Anyone who has experience with this or other suggestions are all wellcome !

Kind regards,

Dries.




--
Dries Vercauteren, PhD student
Master of Bioscience Engineering: Cell and Gene Biotechnology

Ghent Research Group on Nanomedicines
www.ugent.be/fw/en/research/biofys
Faculty of pharmaceutical sciences, Ghent University
Harelbekestraat 72, 9000 Ghent
Belgium

Phone:  +329/264 80 49
Mobile: +32485/30 69 80
E-mail: [hidden email]
          [hidden email]

if it is a transformable system, I believe pHluorins may be where you want to go, check the original paper by Miesenboeck and Rohtman:

Miesenbock, G., De Angelis, D. A. & Rothman, J. E. Visualizing secretion and synaptic transmission
with pH-sensitive green fluorescent proteins. Nature 394, 192–195 (1998).

I believe you can get the construct directly from the Mount Sinai lab, with the endocytic receptor and a mammalian promotor, thus directly usable, in 3 different flavours according to your imaging system/application

Dries Vercauteren escreveu:

Dear Dr Rietdorf and others,

indeed, also in our research we are very much interested in measuring endosomal pH.

One strategy, I was thinking, was using a pH sensitive dye, with a precise defined pKa value like Lysosensor green (LysoSensor™ Green DND-189  pKa 5.2; LysoSensor™ Green DND-153  pKA 7.5), or use SNARF-1, conjugated to a low MW dextran, in that way you get a pH shift when the endosome is acidifying (pKa 7,5). According to Mol Probes (http://probes.invitrogen.com/media/pis/mp01270.pdf) it should even be possible to calculate the pH after calibrating and solely measuring emission intensities at two different wavelenghts.. However, I didn't do this myself yet..

LysoSensor™ Green DND-189  pKa 5.2; LysoSensor™ Green DND-153  pKA 7.5

Another possibility is measuring fluorescence of simultaneously added FITC and TMR:
Sonawane, N. D., Szoka, F. C., and Verkman, A. S. (2003). Chloride accumulation and swelling in endosomes enhances DNA transfer by polyamine-DNA polyplexes. Journal of Biological Chemistry. 278: 44826-44831.

Anyone who has experience with this or other suggestions are all wellcome !

Kind regards,

Dries.

2009/5/15 Rietdorf, Jens [hidden email]

Dear colleagues,

to demonstrate a receptor has indeed been internalized (and he is not
just looking at a structure still continuous with the plasma membrane),
a user of our facilities wants to measure the acidification of the
endosome compartment (its co-localized with EEA1).

Which is a good protocol to do so?
Which alternative strategy would be applicable?

Any suggestion welcome,
Thanks, jens

---
dr. jens rietdorf
head microscopy
novartis research foundation
friedrich-miescher-institute, wro1066.2.16
maulbeerstr.66, 4058 basel, switzerland
couriel:rietdorf(at)fmi(dot)ch
fon: +41.61.69.75172
fax: +41.61.69.73976

--
Dries Vercauteren, PhD student
Master of Bioscience Engineering: Cell and Gene Biotechnology

Ghent Research Group on Nanomedicines
www.ugent.be/fw/en/research/biofys
Faculty of pharmaceutical sciences, Ghent University
Harelbekestraat 72, 9000 Ghent
Belgium

Phone:  +329/264 80 49
Mobile: +32485/30 69 80
E-mail: [hidden email]
          [hidden email]

-- 


**********************************************************
Jose' A. Feijo', Prof.                    
----------------------------------------------------------         
Dep. Biologia Vegetal, Fac.Ciencias, Universidade Lisboa
PT-1749-016 Lisboa, PORTUGAL

tel. +351.21.750.00.47/00/24, fax  +351.21.750.00.48

and/ e

Inst.Gulbenkian Ciencia, PT-2780-156 Oeiras, PORTUGAL

tel. +351.21.440.79.41/00/19, fax +351.21.440.79.70
__________________________________________________________
e.mail: [hidden email]                          
URL: http://www.igc.gulbenkian.pt/code/research.php?lang=en&unit_id=38
**********************************************************

if it is a transformable system, I believe pHluorins may be where you want to go, check the original paper by Miesenboeck and Rohtman:

Miesenbock, G., De Angelis, D. A. & Rothman, J. E. Visualizing secretion and synaptic transmission
with pH-sensitive green fluorescent proteins. Nature 394, 192–195 (1998).

I believe you can get the construct directly from the Mount Sinai lab, with the endocytic receptor and a mammalian promotor, thus directly usable, in 3 different flavours according to your imaging system/application

Dries Vercauteren escreveu:

Dear Dr Rietdorf and others,

indeed, also in our research we are very much interested in measuring endosomal pH.

One strategy, I was thinking, was using a pH sensitive dye, with a precise defined pKa value like Lysosensor green (LysoSensor™ Green DND-189  pKa 5.2; LysoSensor™ Green DND-153  pKA 7.5), or use SNARF-1, conjugated to a low MW dextran, in that way you get a pH shift when the endosome is acidifying (pKa 7,5). According to Mol Probes (http://probes.invitrogen.com/media/pis/mp01270.pdf) it should even be possible to calculate the pH after calibrating and solely measuring emission intensities at two different wavelenghts.. However, I didn't do this myself yet..

LysoSensor™ Green DND-189  pKa 5.2; LysoSensor™ Green DND-153  pKA 7.5

Another possibility is measuring fluorescence of simultaneously added FITC and TMR:
Sonawane, N. D., Szoka, F. C., and Verkman, A. S. (2003). Chloride accumulation and swelling in endosomes enhances DNA transfer by polyamine-DNA polyplexes. Journal of Biological Chemistry. 278: 44826-44831.

Anyone who has experience with this or other suggestions are all wellcome !

Kind regards,

Dries.

2009/5/15 Rietdorf, Jens [hidden email]

Dear colleagues,

to demonstrate a receptor has indeed been internalized (and he is not
just looking at a structure still continuous with the plasma membrane),
a user of our facilities wants to measure the acidification of the
endosome compartment (its co-localized with EEA1).

Which is a good protocol to do so?
Which alternative strategy would be applicable?

Any suggestion welcome,
Thanks, jens

---
dr. jens rietdorf
head microscopy
novartis research foundation
friedrich-miescher-institute, wro1066.2.16
maulbeerstr.66, 4058 basel, switzerland
couriel:rietdorf(at)fmi(dot)ch
fon: +41.61.69.75172
fax: +41.61.69.73976

--
Dries Vercauteren, PhD student
Master of Bioscience Engineering: Cell and Gene Biotechnology

Ghent Research Group on Nanomedicines
www.ugent.be/fw/en/research/biofys
Faculty of pharmaceutical sciences, Ghent University
Harelbekestraat 72, 9000 Ghent
Belgium

Phone:  +329/264 80 49
Mobile: +32485/30 69 80
E-mail: [hidden email]
          [hidden email]

-- 


**********************************************************
Jose' A. Feijo', Prof.                    
----------------------------------------------------------         
Dep. Biologia Vegetal, Fac.Ciencias, Universidade Lisboa
PT-1749-016 Lisboa, PORTUGAL

tel. +351.21.750.00.47/00/24, fax  +351.21.750.00.48

and/ e

Inst.Gulbenkian Ciencia, PT-2780-156 Oeiras, PORTUGAL

tel. +351.21.440.79.41/00/19, fax +351.21.440.79.70
__________________________________________________________
e.mail: [hidden email]                          
URL: http://www.igc.gulbenkian.pt/code/research.php?lang=en&unit_id=38
**********************************************************

A simple way is to use acridine orange fluorescence, which is reduced at low pH, e.g. Gonzalez, A., Koren'kov, V. and Wagner, G.J. (1999) A comparison of Zn, Mn, Cd, and Ca transport mechanisms in oat root tonoplast vesicles. Physiol. Plant.  106, 203–209.  This is in synthetic vesicles made from the membrane of interest.
cheers,
Rosemray

Rosemary White
CSIRO Plant Industry
GPO Box 1600
Canberra, ACT 2601
Australia

ph 61 2 6246 5475
fx 61 2 6246 5334



On 15/05/09 11:14 PM, "José A. Feijó" <jfeijo@...> wrote:

if it is a transformable system, I believe pHluorins may be where you want to go, check the original paper by Miesenboeck and Rohtman:

Miesenbock, G., De Angelis, D. A. & Rothman, J. E. Visualizing secretion and synaptic transmission
with pH-sensitive green fluorescent proteins. Nature 394, 192–195 (1998).

I believe you can get the construct directly from the Mount Sinai lab, with the endocytic receptor and a mammalian promotor, thus directly usable, in 3 different flavours according to your imaging system/application

Dries Vercauteren escreveu:

Dear Dr Rietdorf and others,
 
indeed, also in our research we are very much interested in measuring endosomal pH.
 
One strategy, I was thinking, was using a pH sensitive dye, with a precise defined pKa value like Lysosensor green (LysoSensor™ Green DND-189  pKa 5.2; LysoSensor™ Green DND-153  pKA 7.5), or use SNARF-1, conjugated to a low MW dextran, in that way you get a pH shift when the endosome is acidifying (pKa 7,5). According to Mol Probes (http://probes.invitrogen.com/media/pis/mp01270.pdf) it should even be possible to calculate the pH after calibrating and solely measuring emission intensities at two different wavelenghts.. However, I didn't do this myself yet..
 
LysoSensor™ Green DND-189  pKa 5.2; LysoSensor™ Green DND-153  pKA 7.5
 
Another possibility is measuring fluorescence of simultaneously added FITC and TMR:
        Sonawane, N. D., Szoka, F. C., and Verkman, A. S. (2003). Chloride accumulation and swelling in endosomes enhances DNA transfer by polyamine-DNA polyplexes. Journal of Biological Chemistry. 278: 44826-44831.

Anyone who has experience with this or other suggestions are all wellcome !
 
Kind regards,
 
Dries.
 
 
2009/5/15 Rietdorf, Jens <jens.rietdorf@...> <[hidden email]>
 

Dear colleagues,
 
to demonstrate a receptor has indeed been internalized (and he is not
just looking at a structure still continuous with the plasma membrane),
a user of our facilities wants to measure the acidification of the
endosome compartment (its co-localized with EEA1).
 
Which is a good protocol to do so?
Which alternative strategy would be applicable?
 
Any suggestion welcome,
Thanks, jens
 
---
dr. jens rietdorf
head microscopy
novartis research foundation
friedrich-miescher-institute, wro1066.2.16
maulbeerstr.66, 4058 basel, switzerland
couriel:rietdorf(at)fmi(dot)ch
fon: +41.61.69.75172
fax: +41.61.69.73976
 

 
 
 

Dear List,

We need to use some pretty expensive coverslips for high NA
objectives(around 8 USD per piece). We might have to reuse them :(.
Any one has any established protocol for coverslip re-use for share?
Suggestions are welcomed too.

Thanks a lot...


Regards,
Edna

Edna-
We don't exactly re-use them, but we do clean them for hours (12 h) in 1 N HCl and then wash exhaustively in deionized water, followed by several rinses in 95% ethanol and air-drying.  This takes off everything left by the manufacturing process and leaves a molecularly clean glass surface.  If you actually grew cells on the coverslips, it might not be drastic enough to clean off the cell debris, though.
Carol Heckman
Center for Microscopy & Microanalysis
Bowling Green State University
________________________________________
From: Confocal Microscopy List [[hidden email]] On Behalf Of Hu Xian [[hidden email]]
Sent: Monday, May 18, 2009 2:54 AM
To: [hidden email]
Subject: Protocols for reusing coverslips

Dear List,

We need to use some pretty expensive coverslips for high NA
objectives(around 8 USD per piece). We might have to reuse them :(.
Any one has any established protocol for coverslip re-use for share?
Suggestions are welcomed too.

Thanks a lot...


Regards,
Edna

Likewise:

We remove the coverslip by soaking in 2X SSC [probably for no real reason,
but it helps preserve the specimen on the slide, and I suppose you could add
a drop of Tween 20 to the Coplin jar]. Recover and then rinse the coverslip
in deionised water, and finally wipe the coverslip carefully with ether or
petroleum spirit in the fume cupboard [gloves + KimTech Science 75512
tissues] to get it as clean as possible before the wash sequence below. We
use immersion oil for imaging [which doesn't dissolve so well in ethanol,
hence ether/petroleum spirit], and more importantly 'always liquid'
VectaShield + DAPI non-hardening mountant [naturally with no nail polish
gluing it on]. You can generally slowly soak off 'permanently' mounted
coverslips with things like Xylene/Toluene [check what the original mountant
was dissolved in, e.g. Histomount uses toluene]. After ether/petroleum
spirit cleaning, quickly visually inspect the cover-slips at an angle to the
reflected light to ensure they are smear free before the wash sequence
below.

[This wash sequence is also used for new 'pre-washed' glass slides from
boxes]: Soak the cleaned coverslips overnight in 5ml Teepol/RenClean in ~500
ml [try a slotted rack to hold the coverslips upright]. Wash off detergent
gently with tap water then de-ionised. Leave for 1h in ~500 ml de-ionised +
5ml conc HCL. Rinse with tap water then de-ionised, and put in 100% ethanol
for 1h. Replace with fresh 100% ethanol for another hour.  Remove Ethanol
and air dry in covered chamber. We generally save the last ethanol wash to
re-use as the next 'first' one. I always wipe the cover-slip again with 70%
ethanol and KimTech Science 75512 tissues [wet then dry side], and leave to
dry just before use or reuse.

Haven't need to do this for a while, but it used to work. It's expensive in
time and materials though, and you ideally need some sort of rack for the
washes [easy if you have an in-house workshop].

Keith
---------------------------------------------------------------------------
Dr Keith J. Morris,
Molecular Cytogenetics and Microscopy Core,
Laboratory 00/069 and 00/070,
The Wellcome Trust Centre for Human Genetics,
Roosevelt Drive,
Oxford  OX3 7BN,
United Kingdom.

Telephone:  +44 (0)1865 287568
Email:  [hidden email]
Web-pages: http://www.well.ox.ac.uk/cytogenetics/
 
-----Original Message-----
From: Confocal Microscopy List [mailto:[hidden email]] On
Behalf Of Hu Xian
Sent: 18 May 2009 07:55
To: [hidden email]
Subject: Protocols for reusing coverslips

Dear List,

We need to use some pretty expensive coverslips for high NA
objectives(around 8 USD per piece). We might have to reuse them :(.
Any one has any established protocol for coverslip re-use for share?
Suggestions are welcomed too.

Thanks a lot...


Regards,
Edna

Dear Keith and Carol,

Thanks for the kind advice.  And perhaps I should elaborate our
experiment conditions a bit more.

We are using two high NA lens from different vendors, both for TIRF
experiment.And to match the high NA of the lens, the coverslips need to
have high RI, hence are not made of normal glass( at least not
entirely).  One of the lens is not commercialized yet, neither does the
coverslips for the lens, so we don't know what's in there exactly. The
other one is the 1.65 NA lens from Olympus, and the coverslip should be
made of sapphire. As measured by micrometer, the thickness is around 0.17mm.

As for the sample preparation, we wash the coverslips as normal(10M
nitric acid, milli Q washing, air dry), coat them with fibronectin and
grow cells on them. They are used for TIRF imaging, hence no mounting
media but medium with matching RI with water(PBS/water) on top of them.
Hence removing mounting media is not really our concern, we are more
nervous about getting cells off as well as the fibronectin. Once these
are removed, we will probably use the old method again to clean the
coverslip.

Thanks for helping.

Regards,

Edna, HU Xian





Keith Morris wrote:

Hi Edna,

I though it might be TIRF coverslips [obviously not Sapphire ones from the
$10 cost].

Back in my inhalation fibre toxicity/bio-durability days I recovered the
inhaled glassfibres from the lung tissue using bleach. The lungs were always
digested in bleach for 1 to 4 hours, in a large centrifuge tube on a
motorised roller at 4oC in a cold room [probably in 50ml bleach]. You nipped
in every few hours and the lungs would gradually get smaller and smaller and
then disappear from view [fully digested]. Your cells adhered to coverslips
naturally won't need long. The bleach completely liquidises the lung tissue
such that the tissue digest fully passed through submicron pore size
Nucleopore filters, leaving just the recovered glass fibres on the filter
surface for viewing via SEM or optical microscope using standard filter
optical clearing techniques [making the filter transparent].

Well actually it was 14% hypochlorite solution we used latterly to digest
the tissues, although traditionally household bleach was used - always the
cheapest stuff, not the one with thickeners, and this would be a tad milder
and have detergents added.

Bleach didn't affect the glass fibres and from EDX SEM elemental analysis
measurements, chlorine was only found within very eroded glass fibres - MMVF
fibres tend to dissolve faster in the mildly alkaline lung surfactant
[glassfibres] or acidic alveolar macrophage phagolysosomes [Rockwool]
depending on fibre composition. Unlike other tissue digestion methods [e.g.
plasma ashing], bleach at 4oC was found to minimise fibre breakage during
recovery [eroded micron diameter glass fibres can be very very fragile after
months/years in the lung]. Thus bleach should be glass friendly, easily
washed off, and OK for use with your coverslips. I would think around 10 or
so minutes in bleach would be enough for cells on a coverslip, maybe longer
or less even at RT or say 37oC. I wouldn't have thought the fibronectin
would be a particular problem either - but try it and see.

Once the cells have been digested off the coverlips, you can try the rest of
the cleaning protocol I mentioned [including perhaps a detergent pre-wash
and then ether/petroleum spirit manually cleaning] after the 'digested'
slides have been washed off in de-ionised water. I see no reason why bleach
shouldn't be work well, although you'll have to adapt the digestion
agitation system and a rack would again be useful. The only proviso is that
you wouldn't want any chlorine remaining on the glass surface when
re-culturing [not something I've tried] - but we saw no evidence of that on
our intact [non-eroded] glassfibres' with SEM elemental analysis.

Others have used enzymes or even sodium hydroxide and plasma ashing to
recover fibres from lungs and 'digest'/remove the cellular material:
e.g. http://annhyg.oxfordjournals.org/cgi/reprint/41/6/721.pdf 
The alternative enzyme digestion might appeal, but I suppose enzymes might
stick to glass more than bleach and might be a bit specific rather than a
general digest [or they might not].

Regards

Keith

 


---------------------------------------------------------------------------
Dr Keith J. Morris,
Molecular Cytogenetics and Microscopy Core,
Laboratory 00/069 and 00/070,
The Wellcome Trust Centre for Human Genetics,
Roosevelt Drive,
Oxford  OX3 7BN,
United Kingdom.

Telephone:  +44 (0)1865 287568
Email:  [hidden email]
Web-pages: http://www.well.ox.ac.uk/cytogenetics/
 
-----Original Message-----
From: Confocal Microscopy List [mailto:[hidden email]] On
Behalf Of Hu Xian
Sent: 19 May 2009 05:07
To: [hidden email]
Subject: Re: Protocols for reusing coverslips

Dear Keith and Carol,

Thanks for the kind advice.  And perhaps I should elaborate our
experiment conditions a bit more.

We are using two high NA lens from different vendors, both for TIRF
experiment.And to match the high NA of the lens, the coverslips need to
have high RI, hence are not made of normal glass( at least not
entirely).  One of the lens is not commercialized yet, neither does the
coverslips for the lens, so we don't know what's in there exactly. The
other one is the 1.65 NA lens from Olympus, and the coverslip should be
made of sapphire. As measured by micrometer, the thickness is around 0.17mm.

As for the sample preparation, we wash the coverslips as normal(10M
nitric acid, milli Q washing, air dry), coat them with fibronectin and
grow cells on them. They are used for TIRF imaging, hence no mounting
media but medium with matching RI with water(PBS/water) on top of them.
Hence removing mounting media is not really our concern, we are more
nervous about getting cells off as well as the fibronectin. Once these
are removed, we will probably use the old method again to clean the
coverslip.

Thanks for helping.

Regards,

Edna, HU Xian





Keith Morris wrote:
> Likewise:
>
> We remove the coverslip by soaking in 2X SSC [probably for no real reason,
> but it helps preserve the specimen on the slide, and I suppose you could
add
> a drop of Tween 20 to the Coplin jar]. Recover and then rinse the
coverslip
> in deionised water, and finally wipe the coverslip carefully with ether or
> petroleum spirit in the fume cupboard [gloves + KimTech Science 75512
> tissues] to get it as clean as possible before the wash sequence below. We
> use immersion oil for imaging [which doesn't dissolve so well in ethanol,
> hence ether/petroleum spirit], and more importantly 'always liquid'
> VectaShield + DAPI non-hardening mountant [naturally with no nail polish
> gluing it on]. You can generally slowly soak off 'permanently' mounted
> coverslips with things like Xylene/Toluene [check what the original
mountant
> was dissolved in, e.g. Histomount uses toluene]. After ether/petroleum
> spirit cleaning, quickly visually inspect the cover-slips at an angle to
the
> reflected light to ensure they are smear free before the wash sequence
> below.
>
> [This wash sequence is also used for new 'pre-washed' glass slides from
> boxes]: Soak the cleaned coverslips overnight in 5ml Teepol/RenClean in
~500
> ml [try a slotted rack to hold the coverslips upright]. Wash off detergent
> gently with tap water then de-ionised. Leave for 1h in ~500 ml de-ionised
+
> 5ml conc HCL. Rinse with tap water then de-ionised, and put in 100%
ethanol
> for 1h. Replace with fresh 100% ethanol for another hour.  Remove Ethanol
> and air dry in covered chamber. We generally save the last ethanol wash to
> re-use as the next 'first' one. I always wipe the cover-slip again with
70%
> ethanol and KimTech Science 75512 tissues [wet then dry side], and leave
to
> dry just before use or reuse.
>
> Haven't need to do this for a while, but it used to work. It's expensive
in
> time and materials though, and you ideally need some sort of rack for the
> washes [easy if you have an in-house workshop].
>
> Keith
>
--------------------------------------------------------------------------- On

We have the same cover glass for TIRF, even thoough we have not tried  
this on these slips we clean all our lithographic glass substrates  
with piranha at a 4:1 ratio.
http://en.wikipedia.org/wiki/Piranha_solution
  It eats off almost every organic material- leave it in for 10min  
and rinse a bunch with DI water. We do this is a hood and waste it in  
a special container with a vented cap. It is very nasty and  
exothermic so only make a small amount in a beaker.
Try one Si slip in this and see what happens- actually let me know. I  
am not sure the chemistry of the shaphire is exactly the same as  
glass but it should not be that different for short term exposures.

best
Julia
Sheetz lab


On May 19, 2009, at 12:07 AM, Hu Xian wrote:

Yep it's basically hydrogen peroxide and a strong acid. Chemicals of these
sort have been used for lung tissue digestion* for many decades [perhaps
most are not made quite as aggressive as 'Piranha solution' though].

Tissue digestion protocols are typically based on strong acids
[hydrochloric, glacial acetic], hydrogen peroxide, bleach [5% sodium
hypochlorite], formamide, plasma ashing and proteolytic enzymes - all to
typically to digest away lung tissue and to recover inhaled particulate
matter**. Sometimes it's a combination of these chemicals/procedures.

The method used is solely selected in order to minimise damage to the
delicate material that you want to recover, e.g. inhaled coal particles,
glassfibres, asbestos, talc, mineral dust, paramid fibres, diatoms** etc....
If the inhaled material was say bleach sensitive, then an enzymatic
digestion would be used.

Provided your cover-slip is completely resistant to these chemicals, the use
of any of the above should provide a successful digest and removal of the
cells and fibronectin. Piranha solution sounds a pretty aggressive tissue
digestant though, 'making the glass hydrophilic by hydroxylating the
surface' - and for disposal we could just pour our bleach down the drain.

Keith

*unlike lung, fatty tissues are far harder to digest.
** Sometimes to check for sea drowning, you look for the presence of diatoms
in the lung

---------------------------------------------------------------------------
Dr Keith J. Morris,
Molecular Cytogenetics and Microscopy Core,
Laboratory 00/069 and 00/070,
The Wellcome Trust Centre for Human Genetics,
Roosevelt Drive,
Oxford  OX3 7BN,
United Kingdom.

Telephone:  +44 (0)1865 287568
Email:  [hidden email]
Web-pages: http://www.well.ox.ac.uk/cytogenetics/
 

-----Original Message-----
From: Confocal Microscopy List [mailto:[hidden email]] On
Behalf Of js1719
Sent: 20 May 2009 03:03
To: [hidden email]
Subject: Re: Protocols for reusing coverslips

We have the same cover glass for TIRF, even thoough we have not tried  
this on these slips we clean all our lithographic glass substrates  
with piranha at a 4:1 ratio.
http://en.wikipedia.org/wiki/Piranha_solution
  It eats off almost every organic material- leave it in for 10min  
and rinse a bunch with DI water. We do this is a hood and waste it in  
a special container with a vented cap. It is very nasty and  
exothermic so only make a small amount in a beaker.
Try one Si slip in this and see what happens- actually let me know. I  
am not sure the chemistry of the shaphire is exactly the same as  
glass but it should not be that different for short term exposures.

best
Julia
Sheetz lab


On May 19, 2009, at 12:07 AM, Hu Xian wrote: