Oil objective maximum area/distance for long-term timelapse imaging

> Hi Ken
>
>
>
> My experience: imaging 2 cells 1.7mm apart (thickness of the well wall in
> the MW plates we were using then) every 10 min for 12h with a 60x oil
> objective and a hardware autofocus at 37 deg resulted in a high risk (about
> 25% of the cases?) of losing focus. There go years of sweat and tears…
>
>
>
> We were lucky to get to test a super device manufactured by EMBLEM, the
> commercial side of EMBL. You send your objective. They custom make a cap
> and send you a kit containing cap, tubes, pump and instructions. It is a
> bit clumsy because you need to remove all other objectives and you need to
> be careful not to put oil all over the place but it works a charm. I have
> imaged 10 positions in each well over 15 wells every 10 min for 15 h with
> this device without losing focus. :) You could contact them<
> http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offers>
> to ask if they commercialize it.
>
>
>
> Med vänlig hälsning / Best regards
>
>
>
> Sylvie
>
>
>
> @@@@@@@@@@@@@@@@@@@@@@@@
>
> Sylvie Le Guyader, PhD
>
> Live Cell Imaging Facility Manager
>
> Karolinska Institutet- Bionut Dpt
>
> Hälsovägen 7,
>
> Novum, G lift, floor 6
>
> 14157 Huddinge
>
> Sweden
>
> mobile: +46 (0) 73 733 5008
>
> office: +46 (0) 08-524 811 72 New number!
>
> LCI website
>
>
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]]
> On Behalf Of Kenneth Chen
> Sent: den 2 mars 2016 13:22
> To: [hidden email]
> Subject: Oil objective maximum area/distance for long-term timelapse
> imaging
>
>
>
> *****
>
> To join, leave or search the confocal microscopy listserv, go to:
>
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>
> Post images on http://www.imgur.com and include the link in your posting.
>
> *****
>
>
>
> Hi all,
>
>
>
> We're in the process of designing microfluidic devices for multi-day
> time-lapse imaging. In the past we've had some trouble with image quality
> for very large devices deteriorating due to the loss/thinness of the
> immersion oil layer between sample and objective when very large areas are
> scanned. We have only used traditional oil objectives (no water or
>
> glycerol) Does anyone have any strategies to mitigate this or rules of
> thumb about "safe" maximum sampling areas or distances to travel?
>
>
>
> Thanks,
>
> Ken Chen
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com and include the link in your posting.
> *****
>
> We regularly image the 4 center wells (about 50 total points) of a Labtek 8
> well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
>
> First we put the plate on, one drop of oil on the 60X or 100X objective,
> and drive to all four wells.
>
> Then we take the plate off, and add one more drop of oil, and we're good to
> go.
>
> We also slow the stage speed way down so PFS can follow the glass.
>
> Hope this helps.
>
> Gary
>
> On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader <[hidden email]
> >
> wrote:
>
> > Hi Ken
> >
> >
> >
> > My experience: imaging 2 cells 1.7mm apart (thickness of the well wall in
> > the MW plates we were using then) every 10 min for 12h with a 60x oil
> > objective and a hardware autofocus at 37 deg resulted in a high risk
> (about
> > 25% of the cases?) of losing focus. There go years of sweat and tears…
> >
> >
> >
> > We were lucky to get to test a super device manufactured by EMBLEM, the
> > commercial side of EMBL. You send your objective. They custom make a cap
> > and send you a kit containing cap, tubes, pump and instructions. It is a
> > bit clumsy because you need to remove all other objectives and you need
> to
> > be careful not to put oil all over the place but it works a charm. I have
> > imaged 10 positions in each well over 15 wells every 10 min for 15 h with
> > this device without losing focus. :) You could contact them<
> > http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offers>
> > to ask if they commercialize it.
> >
> >
> >
> > Med vänlig hälsning / Best regards
> >
> >
> >
> > Sylvie
> >
> >
> >
> > @@@@@@@@@@@@@@@@@@@@@@@@
> >
> > Sylvie Le Guyader, PhD
> >
> > Live Cell Imaging Facility Manager
> >
> > Karolinska Institutet- Bionut Dpt
> >
> > Hälsovägen 7,
> >
> > Novum, G lift, floor 6
> >
> > 14157 Huddinge
> >
> > Sweden
> >
> > mobile: +46 (0) 73 733 5008
> >
> > office: +46 (0) 08-524 811 72 New number!
> >
> > LCI website
> >
> >
> >
> >
> >
> > -----Original Message-----
> > From: Confocal Microscopy List [mailto:[hidden email]]
> > On Behalf Of Kenneth Chen
> > Sent: den 2 mars 2016 13:22
> > To: [hidden email]
> > Subject: Oil objective maximum area/distance for long-term timelapse
> > imaging
> >
> >
> >
> > *****
> >
> > To join, leave or search the confocal microscopy listserv, go to:
> >
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> >
> > Post images on http://www.imgur.com and include the link in your
> posting.
> >
> > *****
> >
> >
> >
> > Hi all,
> >
> >
> >
> > We're in the process of designing microfluidic devices for multi-day
> > time-lapse imaging. In the past we've had some trouble with image quality
> > for very large devices deteriorating due to the loss/thinness of the
> > immersion oil layer between sample and objective when very large areas
> are
> > scanned. We have only used traditional oil objectives (no water or
> >
> > glycerol) Does anyone have any strategies to mitigate this or rules of
> > thumb about "safe" maximum sampling areas or distances to travel?
> >
> >
> >
> > Thanks,
> >
> > Ken Chen
> >
>
>
>
> --
> Best,
>
> Gary Laevsky, Ph.D.
> Confocal Imaging Facility Manager
> Dept. of Molecular Biology
> Washington Rd.
> Princeton University
> Princeton, New Jersey, 08544-1014
> (O) 609 258 5432
> (C) 508 507 1310
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com and include the link in your posting.
> *****
>
> We regularly image the 4 center wells (about 50 total points) of a Labtek 8
> well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
>
> First we put the plate on, one drop of oil on the 60X or 100X objective,
> and drive to all four wells.
>
> Then we take the plate off, and add one more drop of oil, and we're good to
> go.
>
> We also slow the stage speed way down so PFS can follow the glass.
>
> Hope this helps.
>
> Gary
>
> On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader <[hidden email]
> >
> wrote:
>
> > Hi Ken
> >
> >
> >
> > My experience: imaging 2 cells 1.7mm apart (thickness of the well wall in
> > the MW plates we were using then) every 10 min for 12h with a 60x oil
> > objective and a hardware autofocus at 37 deg resulted in a high risk
> (about
> > 25% of the cases?) of losing focus. There go years of sweat and tears…
> >
> >
> >
> > We were lucky to get to test a super device manufactured by EMBLEM, the
> > commercial side of EMBL. You send your objective. They custom make a cap
> > and send you a kit containing cap, tubes, pump and instructions. It is a
> > bit clumsy because you need to remove all other objectives and you need
> to
> > be careful not to put oil all over the place but it works a charm. I have
> > imaged 10 positions in each well over 15 wells every 10 min for 15 h with
> > this device without losing focus. :) You could contact them<
> > http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offers>
> > to ask if they commercialize it.
> >
> >
> >
> > Med vänlig hälsning / Best regards
> >
> >
> >
> > Sylvie
> >
> >
> >
> > @@@@@@@@@@@@@@@@@@@@@@@@
> >
> > Sylvie Le Guyader, PhD
> >
> > Live Cell Imaging Facility Manager
> >
> > Karolinska Institutet- Bionut Dpt
> >
> > Hälsovägen 7,
> >
> > Novum, G lift, floor 6
> >
> > 14157 Huddinge
> >
> > Sweden
> >
> > mobile: +46 (0) 73 733 5008
> >
> > office: +46 (0) 08-524 811 72 New number!
> >
> > LCI website
> >
> >
> >
> >
> >
> > -----Original Message-----
> > From: Confocal Microscopy List [mailto:[hidden email]]
> > On Behalf Of Kenneth Chen
> > Sent: den 2 mars 2016 13:22
> > To: [hidden email]
> > Subject: Oil objective maximum area/distance for long-term timelapse
> > imaging
> >
> >
> >
> > *****
> >
> > To join, leave or search the confocal microscopy listserv, go to:
> >
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> >
> > Post images on http://www.imgur.com and include the link in your
> posting.
> >
> > *****
> >
> >
> >
> > Hi all,
> >
> >
> >
> > We're in the process of designing microfluidic devices for multi-day
> > time-lapse imaging. In the past we've had some trouble with image quality
> > for very large devices deteriorating due to the loss/thinness of the
> > immersion oil layer between sample and objective when very large areas
> are
> > scanned. We have only used traditional oil objectives (no water or
> >
> > glycerol) Does anyone have any strategies to mitigate this or rules of
> > thumb about "safe" maximum sampling areas or distances to travel?
> >
> >
> >
> > Thanks,
> >
> > Ken Chen
> >
>
>
>
> --
> Best,
>
> Gary Laevsky, Ph.D.
> Confocal Imaging Facility Manager
> Dept. of Molecular Biology
> Washington Rd.
> Princeton University
> Princeton, New Jersey, 08544-1014
> (O) 609 258 5432
> (C) 508 507 1310
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com and include the link in your posting.
> *****
>
> We regularly image the 4 center wells (about 50 total points) of a
> Labtek 8 well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
>
> First we put the plate on, one drop of oil on the 60X or 100X
> objective, and drive to all four wells.
>
> Then we take the plate off, and add one more drop of oil, and we're
> good to go.
>
> We also slow the stage speed way down so PFS can follow the glass.
>
> Hope this helps.
>
> Gary
>
> On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader
> <[hidden email]
> >
> wrote:
>
> > Hi Ken
> >
> >
> >
> > My experience: imaging 2 cells 1.7mm apart (thickness of the well
> > wall in the MW plates we were using then) every 10 min for 12h with
> > a 60x oil objective and a hardware autofocus at 37 deg resulted in a
> > high risk
> (about
> > 25% of the cases?) of losing focus. There go years of sweat and
> > tears.
> >
> >
> >
> > We were lucky to get to test a super device manufactured by EMBLEM,
> > the commercial side of EMBL. You send your objective. They custom
> > make a cap and send you a kit containing cap, tubes, pump and
> > instructions. It is a bit clumsy because you need to remove all
> > other objectives and you need
> to
> > be careful not to put oil all over the place but it works a charm. I
> > have imaged 10 positions in each well over 15 wells every 10 min for
> > 15 h with this device without losing focus. :) You could contact
> > them<
> > http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offe
> > rs>
> > to ask if they commercialize it.
> >
> >
> >
> > Med vänlig hälsning / Best regards
> >
> >
> >
> > Sylvie
> >
> >
> >
> > @@@@@@@@@@@@@@@@@@@@@@@@
> >
> > Sylvie Le Guyader, PhD
> >
> > Live Cell Imaging Facility Manager
> >
> > Karolinska Institutet- Bionut Dpt
> >
> > Hälsovägen 7,
> >
> > Novum, G lift, floor 6
> >
> > 14157 Huddinge
> >
> > Sweden
> >
> > mobile: +46 (0) 73 733 5008
> >
> > office: +46 (0) 08-524 811 72 New number!
> >
> > LCI website
> >
> >
> >
> >
> >
> > -----Original Message-----
> > From: Confocal Microscopy List
> > [mailto:[hidden email]]
> > On Behalf Of Kenneth Chen
> > Sent: den 2 mars 2016 13:22
> > To: [hidden email]
> > Subject: Oil objective maximum area/distance for long-term timelapse
> > imaging
> >
> >
> >
> > *****
> >
> > To join, leave or search the confocal microscopy listserv, go to:
> >
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> >
> > Post images on http://www.imgur.com and include the link in your
> posting.
> >
> > *****
> >
> >
> >
> > Hi all,
> >
> >
> >
> > We're in the process of designing microfluidic devices for multi-day
> > time-lapse imaging. In the past we've had some trouble with image
> > quality for very large devices deteriorating due to the
> > loss/thinness of the immersion oil layer between sample and
> > objective when very large areas
> are
> > scanned. We have only used traditional oil objectives (no water or
> >
> > glycerol) Does anyone have any strategies to mitigate this or rules
> > of thumb about "safe" maximum sampling areas or distances to travel?
> >
> >
> >
> > Thanks,
> >
> > Ken Chen
> >
>
>
>
> --
> Best,
>
> Gary Laevsky, Ph.D.
> Confocal Imaging Facility Manager
> Dept. of Molecular Biology
> Washington Rd.
> Princeton University
> Princeton, New Jersey, 08544-1014
> (O) 609 258 5432
> (C) 508 507 1310
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com and include the link in your posting.
> *****
>
> We regularly image the 4 center wells (about 50 total points) of a Labtek 8
> well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
>
> First we put the plate on, one drop of oil on the 60X or 100X objective,
> and drive to all four wells.
>
> Then we take the plate off, and add one more drop of oil, and we're good to
> go.
>
> We also slow the stage speed way down so PFS can follow the glass.
>
> Hope this helps.
>
> Gary
>
> On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader <[hidden email]
> >
> wrote:
>
> > Hi Ken
> >
> >
> >
> > My experience: imaging 2 cells 1.7mm apart (thickness of the well wall in
> > the MW plates we were using then) every 10 min for 12h with a 60x oil
> > objective and a hardware autofocus at 37 deg resulted in a high risk
> (about
> > 25% of the cases?) of losing focus. There go years of sweat and tears…
> >
> >
> >
> > We were lucky to get to test a super device manufactured by EMBLEM, the
> > commercial side of EMBL. You send your objective. They custom make a cap
> > and send you a kit containing cap, tubes, pump and instructions. It is a
> > bit clumsy because you need to remove all other objectives and you need
> to
> > be careful not to put oil all over the place but it works a charm. I have
> > imaged 10 positions in each well over 15 wells every 10 min for 15 h with
> > this device without losing focus. :) You could contact them<
> > http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offers>
> > to ask if they commercialize it.
> >
> >
> >
> > Med vänlig hälsning / Best regards
> >
> >
> >
> > Sylvie
> >
> >
> >
> > @@@@@@@@@@@@@@@@@@@@@@@@
> >
> > Sylvie Le Guyader, PhD
> >
> > Live Cell Imaging Facility Manager
> >
> > Karolinska Institutet- Bionut Dpt
> >
> > Hälsovägen 7,
> >
> > Novum, G lift, floor 6
> >
> > 14157 Huddinge
> >
> > Sweden
> >
> > mobile: +46 (0) 73 733 5008
> >
> > office: +46 (0) 08-524 811 72 New number!
> >
> > LCI website
> >
> >
> >
> >
> >
> > -----Original Message-----
> > From: Confocal Microscopy List [mailto:[hidden email]]
> > On Behalf Of Kenneth Chen
> > Sent: den 2 mars 2016 13:22
> > To: [hidden email]
> > Subject: Oil objective maximum area/distance for long-term timelapse
> > imaging
> >
> >
> >
> > *****
> >
> > To join, leave or search the confocal microscopy listserv, go to:
> >
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> >
> > Post images on http://www.imgur.com and include the link in your
> posting.
> >
> > *****
> >
> >
> >
> > Hi all,
> >
> >
> >
> > We're in the process of designing microfluidic devices for multi-day
> > time-lapse imaging. In the past we've had some trouble with image quality
> > for very large devices deteriorating due to the loss/thinness of the
> > immersion oil layer between sample and objective when very large areas
> are
> > scanned. We have only used traditional oil objectives (no water or
> >
> > glycerol) Does anyone have any strategies to mitigate this or rules of
> > thumb about "safe" maximum sampling areas or distances to travel?
> >
> >
> >
> > Thanks,
> >
> > Ken Chen
> >
>
>
>
> --
> Best,
>
> Gary Laevsky, Ph.D.
> Confocal Imaging Facility Manager
> Dept. of Molecular Biology
> Washington Rd.
> Princeton University
> Princeton, New Jersey, 08544-1014
> (O) 609 258 5432
> (C) 508 507 1310
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com<http://www.imgur.com/> and include the link in your posting.
> *****
>
> I forgot to write that what the magic oil device does is that it refills
> the immersion oil on the objectuf lense. :-)
>
> I agree that reducing the stage speed helps but we never got to a fully
> reliable system. Might take magic hands... Sigh!
>
> Ann. What do you mean by 'it did not keep'? Did it bleach? The GattaQuant
> website specifically says that it virtually doesn't bleach! :-(
>
> Med vänlig hälsning / Best regards
>
> Sylvie
>
> @@@@@@@@@@@@@@@@@@@@@@@@
>
> Sylvie Le Guyader, PhD
> Live Cell Imaging Unit Manager
> Karolinska Institutet- Bionut Dpt
> Hälsovägen 7,
> Novum, G lift, floor 6
> 14157 Huddinge
> Sweden
> mobile: +46 (0) 73 733 5008<tel:%2B46%20%280%29%2073%20733%205008>
> office: +46 (0) 8 5248 1107<tel:%2B46%20%280%29%208%205248%201107>
> LCI website
>
>
> ---- Smith, Benjamin E. wrote ----
>
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com<http://www.imgur.com/> and include the link in your posting.
> *****
>
> I can also testify to the benefit of greatly reducing the stage velocity
> during long-term live imaging.  We have done imaging of up to 48-hours,
> and having the stage crawl along allows the immersion fluid to stay wetted
> to the objective, and also eliminates any sample motion.
>
> One other consideration we've done is to setup the run early in the
> morning so you can check up on it throughout the day.  That way, you can
> also add immersion fluid as needed.  Normally, you will find that towards
> the beginning of the run you may need to add a little more to the
> objective, but after about 3-4 hours everything stabilizes, and the system
> is good to go.
>
> I also make sure that there is a sufficient pause between scans so that I
> have enough time to adjust things and still start the next scan at exactly
> the next time interval.
>
> Good luck,
>    Ben Smith
>
> ________________________________________
> From: Confocal Microscopy List <[hidden email]<mailto:[hidden email]>> on
> behalf of Emmanuel Levy <[hidden email]<mailto:[hidden email]>>
> Sent: Wednesday, March 2, 2016 8:46 AM
> To: [hidden email]<mailto:[hidden email]>
> Subject: Re: Oil objective maximum area/distance for long-term timelapse
> imaging
>
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com<http://www.imgur.com/> and include the link in your posting.
> *****
>
> It may also help to use oil with high viscosity index so it remains spread
> on the glass.
> All the best,
> Emmanuel
>
>
> On 2 March 2016 at 16:18, Gary Laevsky <[hidden email]<mailto:[hidden email]>> wrote:
>
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on http://www.imgur.com<http://www.imgur.com/> and include the link in your
> posting.
> > *****
> >
> > We regularly image the 4 center wells (about 50 total points) of a
> Labtek 8
> > well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
> >
> > First we put the plate on, one drop of oil on the 60X or 100X objective,
> > and drive to all four wells.
> >
> > Then we take the plate off, and add one more drop of oil, and we're good
> to
> > go.
> >
> > We also slow the stage speed way down so PFS can follow the glass.
> >
> > Hope this helps.
> >
> > Gary
> >
> > On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader
> <[hidden email]<mailto:[hidden email]>
> > >
> > wrote:
> >
> > > Hi Ken
> > >
> > >
> > >
> > > My experience: imaging 2 cells 1.7mm apart (thickness of the well wall
> in
> > > the MW plates we were using then) every 10 min for 12h with a 60x oil
> > > objective and a hardware autofocus at 37 deg resulted in a high risk
> > (about
> > > 25% of the cases?) of losing focus. There go years of sweat and tears...
> > >
> > >
> > >
> > > We were lucky to get to test a super device manufactured by EMBLEM,
> the
> > > commercial side of EMBL. You send your objective. They custom make a
> cap
> > > and send you a kit containing cap, tubes, pump and instructions. It is
> a
> > > bit clumsy because you need to remove all other objectives and you
> need
> > to
> > > be careful not to put oil all over the place but it works a charm. I
> have
> > > imaged 10 positions in each well over 15 wells every 10 min for 15 h
> with
> > > this device without losing focus. :) You could contact them<
> > >
> http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offers>
> > > to ask if they commercialize it.
> > >
> > >
> > >
> > > Med vänlig hälsning / Best regards
> > >
> > >
> > >
> > > Sylvie
> > >
> > >
> > >
> > > @@@@@@@@@@@@@@@@@@@@@@@@
> > >
> > > Sylvie Le Guyader, PhD
> > >
> > > Live Cell Imaging Facility Manager
> > >
> > > Karolinska Institutet- Bionut Dpt
> > >
> > > Hälsovägen 7,
> > >
> > > Novum, G lift, floor 6
> > >
> > > 14157 Huddinge
> > >
> > > Sweden
> > >
> > > mobile: +46 (0) 73 733 5008<tel:%2B46%20%280%29%2073%20733%205008>
> > >
> > > office: +46 (0) 08-524 811 72 New number!
> > >
> > > LCI website
> > >
> > >
> > >
> > >
> > >
> > > -----Original Message-----
> > > From: Confocal Microscopy List
> [mailto:[hidden email]<mailto:[hidden email]>]
> > > On Behalf Of Kenneth Chen
> > > Sent: den 2 mars 2016 13:22
> > > To: [hidden email]<mailto:[hidden email]>
> > > Subject: Oil objective maximum area/distance for long-term timelapse
> > > imaging
> > >
> > >
> > >
> > > *****
> > >
> > > To join, leave or search the confocal microscopy listserv, go to:
> > >
> > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > >
> > > Post images on http://www.imgur.com<http://www.imgur.com/> and include the link in your
> > posting.
> > >
> > > *****
> > >
> > >
> > >
> > > Hi all,
> > >
> > >
> > >
> > > We're in the process of designing microfluidic devices for multi-day
> > > time-lapse imaging. In the past we've had some trouble with image
> quality
> > > for very large devices deteriorating due to the loss/thinness of the
> > > immersion oil layer between sample and objective when very large areas
> > are
> > > scanned. We have only used traditional oil objectives (no water or
> > >
> > > glycerol) Does anyone have any strategies to mitigate this or rules of
> > > thumb about "safe" maximum sampling areas or distances to travel?
> > >
> > >
> > >
> > > Thanks,
> > >
> > > Ken Chen
> > >
> >
> >
> >
> > --
> > Best,
> >
> > Gary Laevsky, Ph.D.
> > Confocal Imaging Facility Manager
> > Dept. of Molecular Biology
> > Washington Rd.
> > Princeton University
> > Princeton, New Jersey, 08544-1014
> > (O) 609 258 5432<tel:609%20258%205432>
> > (C) 508 507 1310<tel:508%20507%201310>
> >
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com and include the link in your posting.
> *****
>
> We tried to solve this problem by using water instead of oil, acknowledging
> that we lost the increased NA. We were using an inverted setup, and similar
> to Sylvie, we machined a cap that goes around the objective with a drip
> setup - so water drips into this cap, which encases the objective, and
> keeps water in the cap at all times. You have to empirically test what drip
> rate you need to counter evaporation. We found that the viscous water
> substitutes (e.g. ultrasound gel, gonisol, etc.) did not have enough
> capillary action to stay sealed between the objective and the bottom of the
> plate. But water did. This also allows for very fast imaging - you don't
> have to slow down the speed with which the stage travels between wells or
> within wells at all.
>
> Regards-
> Jason
>
> -------
>
> Jason Miller, MD, PhD
>
> University of Michigan Kellogg Eye Center
>
>
> Home address:
>
> 117 Worden Ave
>
> Ann Arbor, MI 48103
>
> Cell: (415) 225-2134<tel:%28415%29%20225-2134>
>
> E-mail: *[hidden email]<mailto:
> [hidden email]> <[hidden email]<mailto:
> [hidden email]>>*
>
>
> "Forgiveness does not change the past, but it does enlarge the future." -
> Paul Boese
>
> On Wed, Mar 2, 2016 at 12:05 PM, Sylvie Le Guyader <
> [hidden email]<mailto:[hidden email]>>
> wrote:
>
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on http://www.imgur.com<http://www.imgur.com/> and include
> the link in your posting.
> > *****
> >
> > I forgot to write that what the magic oil device does is that it refills
> > the immersion oil on the objectuf lense. :-)
> >
> > I agree that reducing the stage speed helps but we never got to a fully
> > reliable system. Might take magic hands... Sigh!
> >
> > Ann. What do you mean by 'it did not keep'? Did it bleach? The GattaQuant
> > website specifically says that it virtually doesn't bleach! :-(
> >
> > Med vänlig hälsning / Best regards
> >
> > Sylvie
> >
> > @@@@@@@@@@@@@@@@@@@@@@@@
> >
> > Sylvie Le Guyader, PhD
> > Live Cell Imaging Unit Manager
> > Karolinska Institutet- Bionut Dpt
> > Hälsovägen 7,
> > Novum, G lift, floor 6
> > 14157 Huddinge
> > Sweden
> > mobile: +46 (0) 73 733 5008<tel:%2B46%20%280%29%2073%20733%205008>
> > office: +46 (0) 8 5248 1107<tel:%2B46%20%280%29%208%205248%201107>
> > LCI website
> >
> >
> > ---- Smith, Benjamin E. wrote ----
> >
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on http://www.imgur.com<http://www.imgur.com/> and include
> the link in your posting.
> > *****
> >
> > I can also testify to the benefit of greatly reducing the stage velocity
> > during long-term live imaging.  We have done imaging of up to 48-hours,
> > and having the stage crawl along allows the immersion fluid to stay
> wetted
> > to the objective, and also eliminates any sample motion.
> >
> > One other consideration we've done is to setup the run early in the
> > morning so you can check up on it throughout the day.  That way, you can
> > also add immersion fluid as needed.  Normally, you will find that towards
> > the beginning of the run you may need to add a little more to the
> > objective, but after about 3-4 hours everything stabilizes, and the
> system
> > is good to go.
> >
> > I also make sure that there is a sufficient pause between scans so that I
> > have enough time to adjust things and still start the next scan at
> exactly
> > the next time interval.
> >
> > Good luck,
> >    Ben Smith
> >
> > ________________________________________
> > From: Confocal Microscopy List <[hidden email]<mailto:
> [hidden email]>> on
> > behalf of Emmanuel Levy <[hidden email]<mailto:
> [hidden email]>>
> > Sent: Wednesday, March 2, 2016 8:46 AM
> > To: [hidden email]<mailto:
> [hidden email]>
> > Subject: Re: Oil objective maximum area/distance for long-term timelapse
> > imaging
> >
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on http://www.imgur.com<http://www.imgur.com/> and include
> the link in your posting.
> > *****
> >
> > It may also help to use oil with high viscosity index so it remains
> spread
> > on the glass.
> > All the best,
> > Emmanuel
> >
> >
> > On 2 March 2016 at 16:18, Gary Laevsky <[hidden email]<mailto:
> [hidden email]>> wrote:
> >
> > > *****
> > > To join, leave or search the confocal microscopy listserv, go to:
> > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > Post images on http://www.imgur.com<http://www.imgur.com/> and
> include the link in your
> > posting.
> > > *****
> > >
> > > We regularly image the 4 center wells (about 50 total points) of a
> > Labtek 8
> > > well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
> > >
> > > First we put the plate on, one drop of oil on the 60X or 100X
> objective,
> > > and drive to all four wells.
> > >
> > > Then we take the plate off, and add one more drop of oil, and we're
> good
> > to
> > > go.
> > >
> > > We also slow the stage speed way down so PFS can follow the glass.
> > >
> > > Hope this helps.
> > >
> > > Gary
> > >
> > > On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader
> > <[hidden email]<mailto:[hidden email]>
> > > >
> > > wrote:
> > >
> > > > Hi Ken
> > > >
> > > >
> > > >
> > > > My experience: imaging 2 cells 1.7mm apart (thickness of the well
> wall
> > in
> > > > the MW plates we were using then) every 10 min for 12h with a 60x oil
> > > > objective and a hardware autofocus at 37 deg resulted in a high risk
> > > (about
> > > > 25% of the cases?) of losing focus. There go years of sweat and
> tears...
> > > >
> > > >
> > > >
> > > > We were lucky to get to test a super device manufactured by EMBLEM,
> > the
> > > > commercial side of EMBL. You send your objective. They custom make a
> > cap
> > > > and send you a kit containing cap, tubes, pump and instructions. It
> is
> > a
> > > > bit clumsy because you need to remove all other objectives and you
> > need
> > > to
> > > > be careful not to put oil all over the place but it works a charm. I
> > have
> > > > imaged 10 positions in each well over 15 wells every 10 min for 15 h
> > with
> > > > this device without losing focus. :) You could contact them<
> > > >
> > http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offers>
> > > > to ask if they commercialize it.
> > > >
> > > >
> > > >
> > > > Med vänlig hälsning / Best regards
> > > >
> > > >
> > > >
> > > > Sylvie
> > > >
> > > >
> > > >
> > > > @@@@@@@@@@@@@@@@@@@@@@@@
> > > >
> > > > Sylvie Le Guyader, PhD
> > > >
> > > > Live Cell Imaging Facility Manager
> > > >
> > > > Karolinska Institutet- Bionut Dpt
> > > >
> > > > Hälsovägen 7,
> > > >
> > > > Novum, G lift, floor 6
> > > >
> > > > 14157 Huddinge
> > > >
> > > > Sweden
> > > >
> > > > mobile: +46 (0) 73 733 5008<tel:%2B46%20%280%29%2073%20733%205008>
> > > >
> > > > office: +46 (0) 08-524 811 72 New number!
> > > >
> > > > LCI website
> > > >
> > > >
> > > >
> > > >
> > > >
> > > > -----Original Message-----
> > > > From: Confocal Microscopy List
> > [mailto:[hidden email]<mailto:
> [hidden email]>]
> > > > On Behalf Of Kenneth Chen
> > > > Sent: den 2 mars 2016 13:22
> > > > To: [hidden email]<mailto:
> [hidden email]>
> > > > Subject: Oil objective maximum area/distance for long-term timelapse
> > > > imaging
> > > >
> > > >
> > > >
> > > > *****
> > > >
> > > > To join, leave or search the confocal microscopy listserv, go to:
> > > >
> > > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > >
> > > > Post images on http://www.imgur.com<http://www.imgur.com/> and
> include the link in your
> > > posting.
> > > >
> > > > *****
> > > >
> > > >
> > > >
> > > > Hi all,
> > > >
> > > >
> > > >
> > > > We're in the process of designing microfluidic devices for multi-day
> > > > time-lapse imaging. In the past we've had some trouble with image
> > quality
> > > > for very large devices deteriorating due to the loss/thinness of the
> > > > immersion oil layer between sample and objective when very large
> areas
> > > are
> > > > scanned. We have only used traditional oil objectives (no water or
> > > >
> > > > glycerol) Does anyone have any strategies to mitigate this or rules
> of
> > > > thumb about "safe" maximum sampling areas or distances to travel?
> > > >
> > > >
> > > >
> > > > Thanks,
> > > >
> > > > Ken Chen
> > > >
> > >
> > >
> > >
> > > --
> > > Best,
> > >
> > > Gary Laevsky, Ph.D.
> > > Confocal Imaging Facility Manager
> > > Dept. of Molecular Biology
> > > Washington Rd.
> > > Princeton University
> > > Princeton, New Jersey, 08544-1014
> > > (O) 609 258 5432<tel:609%20258%205432>
> > > (C) 508 507 1310<tel:508%20507%201310>
> > >
> >
> **********************************************************
> Electronic Mail is not secure, may not be read every day, and should not
> be used for urgent or sensitive issues
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com<http://www.imgur.com/> and include the link in your posting.
> *****
>
> We tried to solve this problem by using water instead of oil,
> acknowledging
> that we lost the increased NA. We were using an inverted setup, and
> similar
> to Sylvie, we machined a cap that goes around the objective with a drip
> setup - so water drips into this cap, which encases the objective, and
> keeps water in the cap at all times. You have to empirically test what
> drip
> rate you need to counter evaporation. We found that the viscous water
> substitutes (e.g. ultrasound gel, gonisol, etc.) did not have enough
> capillary action to stay sealed between the objective and the bottom of
> the
> plate. But water did. This also allows for very fast imaging - you don't
> have to slow down the speed with which the stage travels between wells or
> within wells at all.
>
> Regards-
> Jason
>
> -------
>
> Jason Miller, MD, PhD
>
> University of Michigan Kellogg Eye Center
>
>
> Home address:
>
> 117 Worden Ave
>
> Ann Arbor, MI 48103
>
> Cell: (415) 225-2134<tel:%28415%29%20225-2134><tel:%28415%29%20225-2134>
>
> E-mail: *[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>> <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>>*
>
>
> "Forgiveness does not change the past, but it does enlarge the future." -
> Paul Boese
>
> On Wed, Mar 2, 2016 at 12:05 PM, Sylvie Le Guyader <
> [hidden email]<mailto:[hidden email]><mailto:[hidden email]<mailto:[hidden email]>>>
> wrote:
>
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/> and include
> the link in your posting.
> > *****
> >
> > I forgot to write that what the magic oil device does is that it refills
> > the immersion oil on the objectuf lense. :-)
> >
> > I agree that reducing the stage speed helps but we never got to a fully
> > reliable system. Might take magic hands... Sigh!
> >
> > Ann. What do you mean by 'it did not keep'? Did it bleach? The
> > GattaQuant
> > website specifically says that it virtually doesn't bleach! :-(
> >
> > Med vänlig hälsning / Best regards
> >
> > Sylvie
> >
> > @@@@@@@@@@@@@@@@@@@@@@@@
> >
> > Sylvie Le Guyader, PhD
> > Live Cell Imaging Unit Manager
> > Karolinska Institutet- Bionut Dpt
> > Hälsovägen 7,
> > Novum, G lift, floor 6
> > 14157 Huddinge
> > Sweden
> > mobile: +46 (0) 73 733 5008<tel:%2B46%20%280%29%2073%20733%205008><tel:%2B46%20%280%29%2073%20733%205008>
> > office: +46 (0) 8 5248 1107<tel:%2B46%20%280%29%208%205248%201107>
> > LCI website
> >
> >
> > ---- Smith, Benjamin E. wrote ----
> >
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/> and include
> the link in your posting.
> > *****
> >
> > I can also testify to the benefit of greatly reducing the stage velocity
> > during long-term live imaging.  We have done imaging of up to 48-hours,
> > and having the stage crawl along allows the immersion fluid to stay
> wetted
> > to the objective, and also eliminates any sample motion.
> >
> > One other consideration we've done is to setup the run early in the
> > morning so you can check up on it throughout the day.  That way, you can
> > also add immersion fluid as needed.  Normally, you will find that
> > towards
> > the beginning of the run you may need to add a little more to the
> > objective, but after about 3-4 hours everything stabilizes, and the
> system
> > is good to go.
> >
> > I also make sure that there is a sufficient pause between scans so that
> > I
> > have enough time to adjust things and still start the next scan at
> exactly
> > the next time interval.
> >
> > Good luck,
> >    Ben Smith
> >
> > ________________________________________
> > From: Confocal Microscopy List <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>> on
> > behalf of Emmanuel Levy <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>>
> > Sent: Wednesday, March 2, 2016 8:46 AM
> > To: [hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>
> > Subject: Re: Oil objective maximum area/distance for long-term timelapse
> > imaging
> >
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/> and include
> the link in your posting.
> > *****
> >
> > It may also help to use oil with high viscosity index so it remains
> spread
> > on the glass.
> > All the best,
> > Emmanuel
> >
> >
> > On 2 March 2016 at 16:18, Gary Laevsky <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>> wrote:
> >
> > > *****
> > > To join, leave or search the confocal microscopy listserv, go to:
> > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > Post images on http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/> and
> include the link in your
> > posting.
> > > *****
> > >
> > > We regularly image the 4 center wells (about 50 total points) of a
> > Labtek 8
> > > well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
> > >
> > > First we put the plate on, one drop of oil on the 60X or 100X
> objective,
> > > and drive to all four wells.
> > >
> > > Then we take the plate off, and add one more drop of oil, and we're
> good
> > to
> > > go.
> > >
> > > We also slow the stage speed way down so PFS can follow the glass.
> > >
> > > Hope this helps.
> > >
> > > Gary
> > >
> > > On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader
> > <[hidden email]<mailto:[hidden email]><mailto:[hidden email]<mailto:[hidden email]>>
> > > >
> > > wrote:
> > >
> > > > Hi Ken
> > > >
> > > >
> > > >
> > > > My experience: imaging 2 cells 1.7mm apart (thickness of the well
> wall
> > in
> > > > the MW plates we were using then) every 10 min for 12h with a 60x
> > > > oil
> > > > objective and a hardware autofocus at 37 deg resulted in a high risk
> > > (about
> > > > 25% of the cases?) of losing focus. There go years of sweat and
> tears...
> > > >
> > > >
> > > >
> > > > We were lucky to get to test a super device manufactured by EMBLEM,
> > the
> > > > commercial side of EMBL. You send your objective. They custom make a
> > cap
> > > > and send you a kit containing cap, tubes, pump and instructions. It
> is
> > a
> > > > bit clumsy because you need to remove all other objectives and you
> > need
> > > to
> > > > be careful not to put oil all over the place but it works a charm. I
> > have
> > > > imaged 10 positions in each well over 15 wells every 10 min for 15 h
> > with
> > > > this device without losing focus. :) You could contact them<
> > > >
> > http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offers>
> > > > to ask if they commercialize it.
> > > >
> > > >
> > > >
> > > > Med vänlig hälsning / Best regards
> > > >
> > > >
> > > >
> > > > Sylvie
> > > >
> > > >
> > > >
> > > > @@@@@@@@@@@@@@@@@@@@@@@@
> > > >
> > > > Sylvie Le Guyader, PhD
> > > >
> > > > Live Cell Imaging Facility Manager
> > > >
> > > > Karolinska Institutet- Bionut Dpt
> > > >
> > > > Hälsovägen 7,
> > > >
> > > > Novum, G lift, floor 6
> > > >
> > > > 14157 Huddinge
> > > >
> > > > Sweden
> > > >
> > > > mobile: +46 (0) 73 733 5008<tel:%2B46%20%280%29%2073%20733%205008><tel:%2B46%20%280%29%2073%20733%205008>
> > > >
> > > > office: +46 (0) 08-524 811 72 New number!
> > > >
> > > > LCI website
> > > >
> > > >
> > > >
> > > >
> > > >
> > > > -----Original Message-----
> > > > From: Confocal Microscopy List
> > [mailto:[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>]
> > > > On Behalf Of Kenneth Chen
> > > > Sent: den 2 mars 2016 13:22
> > > > To: [hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>
> > > > Subject: Oil objective maximum area/distance for long-term timelapse
> > > > imaging
> > > >
> > > >
> > > >
> > > > *****
> > > >
> > > > To join, leave or search the confocal microscopy listserv, go to:
> > > >
> > > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > >
> > > > Post images on http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/> and
> include the link in your
> > > posting.
> > > >
> > > > *****
> > > >
> > > >
> > > >
> > > > Hi all,
> > > >
> > > >
> > > >
> > > > We're in the process of designing microfluidic devices for multi-day
> > > > time-lapse imaging. In the past we've had some trouble with image
> > quality
> > > > for very large devices deteriorating due to the loss/thinness of the
> > > > immersion oil layer between sample and objective when very large
> areas
> > > are
> > > > scanned. We have only used traditional oil objectives (no water or
> > > >
> > > > glycerol) Does anyone have any strategies to mitigate this or rules
> of
> > > > thumb about "safe" maximum sampling areas or distances to travel?
> > > >
> > > >
> > > >
> > > > Thanks,
> > > >
> > > > Ken Chen
> > > >
> > >
> > >
> > >
> > > --
> > > Best,
> > >
> > > Gary Laevsky, Ph.D.
> > > Confocal Imaging Facility Manager
> > > Dept. of Molecular Biology
> > > Washington Rd.
> > > Princeton University
> > > Princeton, New Jersey, 08544-1014
> > > (O) 609 258 5432<tel:609%20258%205432><tel:609%20258%205432>
> > > (C) 508 507 1310<tel:508%20507%201310><tel:508%20507%201310>
> > >
> >
> **********************************************************
> Electronic Mail is not secure, may not be read every day, and should not
> be used for urgent or sensitive issues
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com and include the link in your posting.
> *****
>
> Hi Emmanuel-
>
> I thought I was the only one who had noticed this problem! I've not seen
> it discussed on the listserve, and when I contacted Nikon, they hadn't
> heard of the problem. But it soon became clear to me that the issue you
> bring up is exactly what's going on. Here's what I've noticed about the
> phenomenon and some things I've done to avoid the problem. We use the Nikon
> PFS system, which as you know, relies on an IR beam reflecting off a
> refractive index mismatched surface. We see the problem manifest as a
> "jitter" as PFS rapidly jumps between planes (the objective water-glass
> interface, and then the glass surface-cell interface).
>
>
> a)     If you have confluent cells, especially if they are densely packed,
> that decreases the problem since the RI of the cells is different than pure
> water.
>
> b)    The higher the NA objective, the worse the problem. Although to be
> honest, I haven't distinguished whether it's higher objective magnification
> or higher NA specifically.
>
> c)     The thinner the glass, the worse the problem. If you are using an
> objective with a correction collar, that means you can try for glass that
> is thicker and adjust by adjusting the correction collar.
>
> Our main solution for automated imaging involved writing a micromanager
> script. What we found out was that if perfect focus starts to jitter at a
> spot (jumping between the top and bottom of the glass), we let PFS go for a
> few seconds and take the average Z position of where it is during the
> jitter (get Z position every x ms, and average that position over the few
> seconds we let PFS go). Then we turn PFS off, have the stage move to this Z
> position (the average Z depth), and turn PFS back on. 95% of the time,
> that's all we need. Occasionally, that doesn't work. If it doesn't, we try
> one more time. And then if that doesn't work, we assume we are instead out
> of PFS range, and we have the script automatically move X um up, then X um
> down from the original Z focus spot and reattempt PFS focus there. The X um
> is determined empirically, but once you determine it, it's remarkably
> reproducible. We've been able to do runs over entire plates for 40+ hours,
> imaging every 20 minutes to 1 hour, using this type of setup.
>
> -Jason
>
>
> On 2 March 2016 at 19:19, Miller, Jason <[hidden email]<mailto:
> [hidden email]>> wrote:
>
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on http://www.imgur.com<http://www.imgur.com/> and include
> the link in your posting.
> > *****
> >
> > We tried to solve this problem by using water instead of oil,
> > acknowledging
> > that we lost the increased NA. We were using an inverted setup, and
> > similar
> > to Sylvie, we machined a cap that goes around the objective with a drip
> > setup - so water drips into this cap, which encases the objective, and
> > keeps water in the cap at all times. You have to empirically test what
> > drip
> > rate you need to counter evaporation. We found that the viscous water
> > substitutes (e.g. ultrasound gel, gonisol, etc.) did not have enough
> > capillary action to stay sealed between the objective and the bottom of
> > the
> > plate. But water did. This also allows for very fast imaging - you don't
> > have to slow down the speed with which the stage travels between wells or
> > within wells at all.
> >
> > Regards-
> > Jason
> >
> > -------
> >
> > Jason Miller, MD, PhD
> >
> > University of Michigan Kellogg Eye Center
> >
> >
> > Home address:
> >
> > 117 Worden Ave
> >
> > Ann Arbor, MI 48103
> >
> > Cell: (415) 225-2134<tel:%28415%29%20225-2134><tel:%28415%29%20225-2134>
> >
> > E-mail: *[hidden email]<mailto:
> [hidden email]><mailto:
> > [hidden email]<mailto:[hidden email]>>
> <[hidden email]<mailto:[hidden email]
> ><mailto:
> > [hidden email]<mailto:[hidden email]
> >>>*
> >
> >
> > "Forgiveness does not change the past, but it does enlarge the future." -
> > Paul Boese
> >
> > On Wed, Mar 2, 2016 at 12:05 PM, Sylvie Le Guyader <
> > [hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>>
> > wrote:
> >
> > > *****
> > > To join, leave or search the confocal microscopy listserv, go to:
> > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > Post images on http://www.imgur.com<http://www.imgur.com/><
> http://www.imgur.com/> and include
> > the link in your posting.
> > > *****
> > >
> > > I forgot to write that what the magic oil device does is that it
> refills
> > > the immersion oil on the objectuf lense. :-)
> > >
> > > I agree that reducing the stage speed helps but we never got to a fully
> > > reliable system. Might take magic hands... Sigh!
> > >
> > > Ann. What do you mean by 'it did not keep'? Did it bleach? The
> > > GattaQuant
> > > website specifically says that it virtually doesn't bleach! :-(
> > >
> > > Med vänlig hälsning / Best regards
> > >
> > > Sylvie
> > >
> > > @@@@@@@@@@@@@@@@@@@@@@@@
> > >
> > > Sylvie Le Guyader, PhD
> > > Live Cell Imaging Unit Manager
> > > Karolinska Institutet- Bionut Dpt
> > > Hälsovägen 7,
> > > Novum, G lift, floor 6
> > > 14157 Huddinge
> > > Sweden
> > > mobile: +46 (0) 73 733 5008
> <tel:%2B46%20%280%29%2073%20733%205008><tel:%2B46%20%280%29%2073%20733%205008>
> > > office: +46 (0) 8 5248 1107<tel:%2B46%20%280%29%208%205248%201107>
> > > LCI website
> > >
> > >
> > > ---- Smith, Benjamin E. wrote ----
> > >
> > > *****
> > > To join, leave or search the confocal microscopy listserv, go to:
> > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > Post images on http://www.imgur.com<http://www.imgur.com/><
> http://www.imgur.com/> and include
> > the link in your posting.
> > > *****
> > >
> > > I can also testify to the benefit of greatly reducing the stage
> velocity
> > > during long-term live imaging.  We have done imaging of up to 48-hours,
> > > and having the stage crawl along allows the immersion fluid to stay
> > wetted
> > > to the objective, and also eliminates any sample motion.
> > >
> > > One other consideration we've done is to setup the run early in the
> > > morning so you can check up on it throughout the day.  That way, you
> can
> > > also add immersion fluid as needed.  Normally, you will find that
> > > towards
> > > the beginning of the run you may need to add a little more to the
> > > objective, but after about 3-4 hours everything stabilizes, and the
> > system
> > > is good to go.
> > >
> > > I also make sure that there is a sufficient pause between scans so that
> > > I
> > > have enough time to adjust things and still start the next scan at
> > exactly
> > > the next time interval.
> > >
> > > Good luck,
> > >    Ben Smith
> > >
> > > ________________________________________
> > > From: Confocal Microscopy List <[hidden email]
> <mailto:[hidden email]><mailto:
> > [hidden email]<mailto:[hidden email]>>>
> on
> > > behalf of Emmanuel Levy <[hidden email]<mailto:
> [hidden email]><mailto:
> > [hidden email]<mailto:[hidden email]>>>
> > > Sent: Wednesday, March 2, 2016 8:46 AM
> > > To: [hidden email]<mailto:
> [hidden email]><mailto:
> > [hidden email]<mailto:[hidden email]
> >>
> > > Subject: Re: Oil objective maximum area/distance for long-term
> timelapse
> > > imaging
> > >
> > > *****
> > > To join, leave or search the confocal microscopy listserv, go to:
> > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > Post images on http://www.imgur.com<http://www.imgur.com/><
> http://www.imgur.com/> and include
> > the link in your posting.
> > > *****
> > >
> > > It may also help to use oil with high viscosity index so it remains
> > spread
> > > on the glass.
> > > All the best,
> > > Emmanuel
> > >
> > >
> > > On 2 March 2016 at 16:18, Gary Laevsky <[hidden email]
> <mailto:[hidden email]><mailto:
> > [hidden email]<mailto:[hidden email]>>> wrote:
> > >
> > > > *****
> > > > To join, leave or search the confocal microscopy listserv, go to:
> > > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > > Post images on http://www.imgur.com<http://www.imgur.com/><
> http://www.imgur.com/> and
> > include the link in your
> > > posting.
> > > > *****
> > > >
> > > > We regularly image the 4 center wells (about 50 total points) of a
> > > Labtek 8
> > > > well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
> > > >
> > > > First we put the plate on, one drop of oil on the 60X or 100X
> > objective,
> > > > and drive to all four wells.
> > > >
> > > > Then we take the plate off, and add one more drop of oil, and we're
> > good
> > > to
> > > > go.
> > > >
> > > > We also slow the stage speed way down so PFS can follow the glass.
> > > >
> > > > Hope this helps.
> > > >
> > > > Gary
> > > >
> > > > On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader
> > > <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>
> > > > >
> > > > wrote:
> > > >
> > > > > Hi Ken
> > > > >
> > > > >
> > > > >
> > > > > My experience: imaging 2 cells 1.7mm apart (thickness of the well
> > wall
> > > in
> > > > > the MW plates we were using then) every 10 min for 12h with a 60x
> > > > > oil
> > > > > objective and a hardware autofocus at 37 deg resulted in a high
> risk
> > > > (about
> > > > > 25% of the cases?) of losing focus. There go years of sweat and
> > tears...
> > > > >
> > > > >
> > > > >
> > > > > We were lucky to get to test a super device manufactured by EMBLEM,
> > > the
> > > > > commercial side of EMBL. You send your objective. They custom make
> a
> > > cap
> > > > > and send you a kit containing cap, tubes, pump and instructions. It
> > is
> > > a
> > > > > bit clumsy because you need to remove all other objectives and you
> > > need
> > > > to
> > > > > be careful not to put oil all over the place but it works a charm.
> I
> > > have
> > > > > imaged 10 positions in each well over 15 wells every 10 min for 15
> h
> > > with
> > > > > this device without losing focus. :) You could contact them<
> > > > >
> > > http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offers
> >
> > > > > to ask if they commercialize it.
> > > > >
> > > > >
> > > > >
> > > > > Med vänlig hälsning / Best regards
> > > > >
> > > > >
> > > > >
> > > > > Sylvie
> > > > >
> > > > >
> > > > >
> > > > > @@@@@@@@@@@@@@@@@@@@@@@@
> > > > >
> > > > > Sylvie Le Guyader, PhD
> > > > >
> > > > > Live Cell Imaging Facility Manager
> > > > >
> > > > > Karolinska Institutet- Bionut Dpt
> > > > >
> > > > > Hälsovägen 7,
> > > > >
> > > > > Novum, G lift, floor 6
> > > > >
> > > > > 14157 Huddinge
> > > > >
> > > > > Sweden
> > > > >
> > > > > mobile: +46 (0) 73 733 5008
> <tel:%2B46%20%280%29%2073%20733%205008><tel:%2B46%20%280%29%2073%20733%205008>
> > > > >
> > > > > office: +46 (0) 08-524 811 72 New number!
> > > > >
> > > > > LCI website
> > > > >
> > > > >
> > > > >
> > > > >
> > > > >
> > > > > -----Original Message-----
> > > > > From: Confocal Microscopy List
> > > [mailto:[hidden email]<mailto:
> [hidden email]><mailto:
> > [hidden email]<mailto:[hidden email]
> >>]
> > > > > On Behalf Of Kenneth Chen
> > > > > Sent: den 2 mars 2016 13:22
> > > > > To: [hidden email]<mailto:
> [hidden email]><mailto:
> > [hidden email]<mailto:[hidden email]
> >>
> > > > > Subject: Oil objective maximum area/distance for long-term
> timelapse
> > > > > imaging
> > > > >
> > > > >
> > > > >
> > > > > *****
> > > > >
> > > > > To join, leave or search the confocal microscopy listserv, go to:
> > > > >
> > > > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > > >
> > > > > Post images on http://www.imgur.com<http://www.imgur.com/><
> http://www.imgur.com/> and
> > include the link in your
> > > > posting.
> > > > >
> > > > > *****
> > > > >
> > > > >
> > > > >
> > > > > Hi all,
> > > > >
> > > > >
> > > > >
> > > > > We're in the process of designing microfluidic devices for
> multi-day
> > > > > time-lapse imaging. In the past we've had some trouble with image
> > > quality
> > > > > for very large devices deteriorating due to the loss/thinness of
> the
> > > > > immersion oil layer between sample and objective when very large
> > areas
> > > > are
> > > > > scanned. We have only used traditional oil objectives (no water or
> > > > >
> > > > > glycerol) Does anyone have any strategies to mitigate this or rules
> > of
> > > > > thumb about "safe" maximum sampling areas or distances to travel?
> > > > >
> > > > >
> > > > >
> > > > > Thanks,
> > > > >
> > > > > Ken Chen
> > > > >
> > > >
> > > >
> > > >
> > > > --
> > > > Best,
> > > >
> > > > Gary Laevsky, Ph.D.
> > > > Confocal Imaging Facility Manager
> > > > Dept. of Molecular Biology
> > > > Washington Rd.
> > > > Princeton University
> > > > Princeton, New Jersey, 08544-1014
> > > > (O) 609 258 5432<tel:609%20258%205432><tel:609%20258%205432>
> > > > (C) 508 507 1310<tel:508%20507%201310><tel:508%20507%201310>
> > > >
> > >
> > **********************************************************
> > Electronic Mail is not secure, may not be read every day, and should not
> > be used for urgent or sensitive issues
> >
> **********************************************************
> Electronic Mail is not secure, may not be read every day, and should not
> be used for urgent or sensitive issues
>

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> Post images on http://www.imgur.com<http://www.imgur.com/> and include the link in your posting.
> *****
>
> We tried to solve this problem by using water instead of oil,
> acknowledging that we lost the increased NA. We were using an inverted
> setup, and similar to Sylvie, we machined a cap that goes around the
> objective with a drip setup - so water drips into this cap, which
> encases the objective, and keeps water in the cap at all times. You
> have to empirically test what drip rate you need to counter
> evaporation. We found that the viscous water substitutes (e.g.
> ultrasound gel, gonisol, etc.) did not have enough capillary action to
> stay sealed between the objective and the bottom of the plate. But
> water did. This also allows for very fast imaging - you don't have to
> slow down the speed with which the stage travels between wells or
> within wells at all.
>
> Regards-
> Jason
>
> -------
>
> Jason Miller, MD, PhD
>
> University of Michigan Kellogg Eye Center
>
>
> Home address:
>
> 117 Worden Ave
>
> Ann Arbor, MI 48103
>
> Cell: (415)
> 225-2134<tel:%28415%29%20225-2134><tel:%28415%29%20225-2134>
>
> E-mail: *[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>> <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]
> >>>*
>
>
> "Forgiveness does not change the past, but it does enlarge the
> future." - Paul Boese
>
> On Wed, Mar 2, 2016 at 12:05 PM, Sylvie Le Guyader <
> [hidden email]<mailto:[hidden email]><mailto:Sylvie.
> [hidden email]<mailto:[hidden email]>>>
> wrote:
>
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on
> > http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/>
> > and include
> the link in your posting.
> > *****
> >
> > I forgot to write that what the magic oil device does is that it
> > refills the immersion oil on the objectuf lense. :-)
> >
> > I agree that reducing the stage speed helps but we never got to a
> > fully reliable system. Might take magic hands... Sigh!
> >
> > Ann. What do you mean by 'it did not keep'? Did it bleach? The
> > GattaQuant website specifically says that it virtually doesn't
> > bleach! :-(
> >
> > Med vänlig hälsning / Best regards
> >
> > Sylvie
> >
> > @@@@@@@@@@@@@@@@@@@@@@@@
> >
> > Sylvie Le Guyader, PhD
> > Live Cell Imaging Unit Manager
> > Karolinska Institutet- Bionut Dpt
> > Hälsovägen 7,
> > Novum, G lift, floor 6
> > 14157 Huddinge
> > Sweden
> > mobile: +46 (0) 73 733
> > 5008<tel:%2B46%20%280%29%2073%20733%205008><tel:%2B46%20%280%29%2073
> > %20733%205008>
> > office: +46 (0) 8 5248 1107<tel:%2B46%20%280%29%208%205248%201107>
> > LCI website
> >
> >
> > ---- Smith, Benjamin E. wrote ----
> >
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on
> > http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/>
> > and include
> the link in your posting.
> > *****
> >
> > I can also testify to the benefit of greatly reducing the stage
> > velocity during long-term live imaging.  We have done imaging of up
> > to 48-hours, and having the stage crawl along allows the immersion
> > fluid to stay
> wetted
> > to the objective, and also eliminates any sample motion.
> >
> > One other consideration we've done is to setup the run early in the
> > morning so you can check up on it throughout the day.  That way, you
> > can also add immersion fluid as needed.  Normally, you will find
> > that towards the beginning of the run you may need to add a little
> > more to the objective, but after about 3-4 hours everything
> > stabilizes, and the
> system
> > is good to go.
> >
> > I also make sure that there is a sufficient pause between scans so
> > that I have enough time to adjust things and still start the next
> > scan at
> exactly
> > the next time interval.
> >
> > Good luck,
> >    Ben Smith
> >
> > ________________________________________
> > From: Confocal Microscopy List <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]
> DU>>> on
> > behalf of Emmanuel Levy <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>>
> > Sent: Wednesday, March 2, 2016 8:46 AM
> > To: [hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]
> DU>>
> > Subject: Re: Oil objective maximum area/distance for long-term
> > timelapse imaging
> >
> > *****
> > To join, leave or search the confocal microscopy listserv, go to:
> > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > Post images on
> > http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/>
> > and include
> the link in your posting.
> > *****
> >
> > It may also help to use oil with high viscosity index so it remains
> spread
> > on the glass.
> > All the best,
> > Emmanuel
> >
> >
> > On 2 March 2016 at 16:18, Gary Laevsky <[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]>>> wrote:
> >
> > > *****
> > > To join, leave or search the confocal microscopy listserv, go to:
> > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > Post images on
> > > http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com/>
> > > and
> include the link in your
> > posting.
> > > *****
> > >
> > > We regularly image the 4 center wells (about 50 total points) of a
> > Labtek 8
> > > well chambered coverslip for 8-16 hours at 37c using PFS on a TiE.
> > >
> > > First we put the plate on, one drop of oil on the 60X or 100X
> objective,
> > > and drive to all four wells.
> > >
> > > Then we take the plate off, and add one more drop of oil, and
> > > we're
> good
> > to
> > > go.
> > >
> > > We also slow the stage speed way down so PFS can follow the glass.
> > >
> > > Hope this helps.
> > >
> > > Gary
> > >
> > > On Wed, Mar 2, 2016 at 7:49 AM, Sylvie Le Guyader
> > <[hidden email]<mailto:[hidden email]><mailto:Sylv
> > [hidden email]<mailto:[hidden email]>>
> > > >
> > > wrote:
> > >
> > > > Hi Ken
> > > >
> > > >
> > > >
> > > > My experience: imaging 2 cells 1.7mm apart (thickness of the
> > > > well
> wall
> > in
> > > > the MW plates we were using then) every 10 min for 12h with a
> > > > 60x oil objective and a hardware autofocus at 37 deg resulted in
> > > > a high risk
> > > (about
> > > > 25% of the cases?) of losing focus. There go years of sweat and
> tears...
> > > >
> > > >
> > > >
> > > > We were lucky to get to test a super device manufactured by
> > > > EMBLEM,
> > the
> > > > commercial side of EMBL. You send your objective. They custom
> > > > make a
> > cap
> > > > and send you a kit containing cap, tubes, pump and instructions.
> > > > It
> is
> > a
> > > > bit clumsy because you need to remove all other objectives and
> > > > you
> > need
> > > to
> > > > be careful not to put oil all over the place but it works a
> > > > charm. I
> > have
> > > > imaged 10 positions in each well over 15 wells every 10 min for
> > > > 15 h
> > with
> > > > this device without losing focus. :) You could contact them<
> > > >
> > http://www.embl-em.de/articles.php?lang=de&hid=4&Cat=Technology_Offe
> > rs>
> > > > to ask if they commercialize it.
> > > >
> > > >
> > > >
> > > > Med vänlig hälsning / Best regards
> > > >
> > > >
> > > >
> > > > Sylvie
> > > >
> > > >
> > > >
> > > > @@@@@@@@@@@@@@@@@@@@@@@@
> > > >
> > > > Sylvie Le Guyader, PhD
> > > >
> > > > Live Cell Imaging Facility Manager
> > > >
> > > > Karolinska Institutet- Bionut Dpt
> > > >
> > > > Hälsovägen 7,
> > > >
> > > > Novum, G lift, floor 6
> > > >
> > > > 14157 Huddinge
> > > >
> > > > Sweden
> > > >
> > > > mobile: +46 (0) 73 733
> > > > 5008<tel:%2B46%20%280%29%2073%20733%205008><tel:%2B46%20%280%29%
> > > > 2073%20733%205008>
> > > >
> > > > office: +46 (0) 08-524 811 72 New number!
> > > >
> > > > LCI website
> > > >
> > > >
> > > >
> > > >
> > > >
> > > > -----Original Message-----
> > > > From: Confocal Microscopy List
> > [mailto:[hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]
> DU>>]
> > > > On Behalf Of Kenneth Chen
> > > > Sent: den 2 mars 2016 13:22
> > > > To: [hidden email]<mailto:[hidden email]><mailto:
> [hidden email]<mailto:[hidden email]
> DU>>
> > > > Subject: Oil objective maximum area/distance for long-term
> > > > timelapse imaging
> > > >
> > > >
> > > >
> > > > *****
> > > >
> > > > To join, leave or search the confocal microscopy listserv, go to:
> > > >
> > > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> > > >
> > > > Post images on
> > > > http://www.imgur.com<http://www.imgur.com/><http://www.imgur.com
> > > > /> and
> include the link in your
> > > posting.
> > > >
> > > > *****
> > > >
> > > >
> > > >
> > > > Hi all,
> > > >
> > > >
> > > >
> > > > We're in the process of designing microfluidic devices for
> > > > multi-day time-lapse imaging. In the past we've had some trouble
> > > > with image
> > quality
> > > > for very large devices deteriorating due to the loss/thinness of
> > > > the immersion oil layer between sample and objective when very
> > > > large
> areas
> > > are
> > > > scanned. We have only used traditional oil objectives (no water
> > > > or
> > > >
> > > > glycerol) Does anyone have any strategies to mitigate this or
> > > > rules
> of
> > > > thumb about "safe" maximum sampling areas or distances to travel?
> > > >
> > > >
> > > >
> > > > Thanks,
> > > >
> > > > Ken Chen
> > > >
> > >
> > >
> > >
> > > --
> > > Best,
> > >
> > > Gary Laevsky, Ph.D.
> > > Confocal Imaging Facility Manager
> > > Dept. of Molecular Biology
> > > Washington Rd.
> > > Princeton University
> > > Princeton, New Jersey, 08544-1014
> > > (O) 609 258 5432<tel:609%20258%205432><tel:609%20258%205432>
> > > (C) 508 507 1310<tel:508%20507%201310><tel:508%20507%201310>
> > >
> >
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