Re: Leica SP8 confocal Windows 10 upgrade

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Dear confocalmicroscopy-list,
please allow me to reactivate this old thread because the problem persists: How to update the operating systems of Leica SP8 from Windows7 (end of life) to Windows10.  
The (only) solution, which was recently offered to us by Leica, is to purchase a new workstation for ~9KEuro. And our team is not alone with this problem as I know at least 6 other microscopes with this issue.

Did this group find an alternative solution to this problem? Did anybody successfully upgrade the OS on the existing hardware - without breaking the system?

Any input on this is highly appreciated.
cheers, aRnim

--
Dr. Arnim Jenett
Imaging and Data Management
TEFOR Paris-Saclay,
CNRS UMS2010 / INRAE UMS1451,
Université Paris-Saclay

Bat 32, 1 Avenue de la Terrasse
91190 Gif-sur-Yvette, France
https://tps.tefor.net

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Hi Arnim,

first, I'm *not* a happy owner of SP8.

Second, with most (if not all) of our microscopes we're happier with
Windows 7. It is unsupported, but it works; why break it then? When IT
folks are complaining, my philosophy is, if a smart refrigerator, chinese
watch, or a phone with Android 4 can connect to the institution's WiFi, why
not a Win 7 PC?

Third, if you don't get a more assuring answer from other listers, you can
just "give it a shot":
1) Get a new harddrive (assuming your PC does not support NVMe I'd suggest
a SATA SSD with good TBW specs, e.g. ADATA SU800, or, even better, Samsung
860 PRO (not EVO)).
2) now you have two options - upgrade the OS (higher chances of success?)
or start from scratch (cleaner system?)
2a) To upgrade, clone your old disk to the SSD (it's a bit tricky if your
old disk is bigger than the SSD).
3a) Boot from the SSD and do an in-place upgrade to Windows 10 (some
versions are tricky to upgrade, e.g. Win 7 Enterprise).
4a) Test and report!
or
2b) To start from scratch, install clean Windows 10 on the SSD (I remember
some LAS versions could only run from the D drive, so if that's your case,
and you want LAS to run from the same SSD, just partition it accordingly).
3b) Install the same LAS software you used under Windows 7 (the LAS may
want to rewrite the firmware of the SP8, so if you use the same version of
LAS, you'll be able to go back to your old OS later, if needed).
4b) Test and report!

Good luck!

zdenek

On Wed, Oct 21, 2020 at 5:50 AM Arnim Jenett <[hidden email]> wrote:


--
--
Zdenek Svindrych, Ph.D.
Research Scientist - Microscopy Imaging Specialist
Department of Biochemistry and Cell Biology
Geisel School of Medicine at Dartmouth

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Our IT department created a "walled off" section of our network for our
Win7 microscopes. We can connect our microscope computers to our local
server for data transfer, but they are cut off from everything else and
will reject outside connections. It's not a perfect solution, but our IT
department deemed it "good enough" given our needs and inability to upgrade
them to Win10.

Craig

On Wed, Oct 21, 2020 at 7:27 AM Zdenek Svindrych <[hidden email]> wrote:

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Bonjour Arnim;
        We have a very clunky but inexpensive work-around, but it works. This is to address our IT department encouraging elimination of Win 7 computers for network security.
        We found a second low-end computer and installed Win 10 Pro. Then we connected this directly to our Win 7 computer with a StarTech.com USB 3.0 to Gigabit Ethernet NIC Network Adapter.
        Our users have to transfer their acquired data from the Win 7 computer to the Win 10 computer at the end of their session (easy drag-and-drop). The Win 10 computer is accessible for remote data transfer.

        Best;
Kathy



-----Original Message-----
From: Confocal Microscopy List <[hidden email]> On Behalf Of Arnim Jenett
Sent: Wednesday, October 21, 2020 2:39 AM
To: [hidden email]
Subject: Re: Leica SP8 confocal Windows 10 upgrade

*****
To join, leave or search the confocal microscopy listserv, go to:
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Dear confocalmicroscopy-list,
please allow me to reactivate this old thread because the problem persists: How to update the operating systems of Leica SP8 from Windows7 (end of life) to Windows10.  
The (only) solution, which was recently offered to us by Leica, is to purchase a new workstation for ~9KEuro. And our team is not alone with this problem as I know at least 6 other microscopes with this issue.

Did this group find an alternative solution to this problem? Did anybody successfully upgrade the OS on the existing hardware - without breaking the system?

Any input on this is highly appreciated.
cheers, aRnim

--
Dr. Arnim Jenett
Imaging and Data Management
TEFOR Paris-Saclay,
CNRS UMS2010 / INRAE UMS1451,
Université Paris-Saclay

Bat 32, 1 Avenue de la Terrasse
91190 Gif-sur-Yvette, France
https://tps.tefor.net

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To join, leave or search the confocal microscopy listserv, go to:
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Hi Armin,
Our IT Dept opted for a Win 7 "Extended Security Updates (ESU)" from
Microsoft inc through 2023. So far we had no problem and the cost is very
reasonable. For more information on how to obtain the ESU, please check out
this blog: "
https://techcommunity.microsoft.com/t5/windows-it-pro-blog/obtaining-extended-security-updates-for-eligible-windows-devices/ba-p/1167091
)".
I hope this helps.

Best,
Blaise

Blaise Ndjamen, PhD

Director,

Histology and Light Microscopy Core Facility,

Gladstone Institutes,

1650 Owens St, San Francisco, CA 94158

Tel. 415-734-2566

https://labs.gladstone.org/histology/index.html


On Wed, Oct 21, 2020 at 2:50 AM Arnim Jenett <[hidden email]> wrote:

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Dear Arnim,

Steffen Dietzel for example was one of the people who bravely did the upgrade by themselves and he published the procedure which addresses Leica SP8:

https://www.bioimaging.bmc.med.uni-muenchen.de/manuals-protocols/maintenance_protocolls/win7towin10/index.html
From Win7 to Win 10 LTSC - Core Facility Bioimaging - LMU Munich<https://www.bioimaging.bmc.med.uni-muenchen.de/manuals-protocols/maintenance_protocolls/win7towin10/index.html>
SP8 with compact supply unit with a HP Z640 ().SP8 MP plus compact supply unit and Camera DFC365FX with a HP Z640, LASX 3.5.0.18371 ().SP8 WLL with a HP Z640, LASX 3.5.5.19976 ().
www.bioimaging.bmc.med.uni-muenchen.de

It's a bit of hacking around. My former colleague followed the procedure and got stuck. Luckily, the Leica representatives there are quite flexible (not a Leica subsidiary but a third party company) and their engineer helped with the upgrade, so it ended successfully.

Best wishes,
Radek


Radek MACHAN, Ph.D. (Senior Research Fellow)
SCELSE Advanced Biofilm Imaging Facility<http://www.scelse.sg/Page/imaging-facility> Manager
Nanyang Technological University
#B2, 60 Nanyang Drive, SBS-01N-27
Singapore 637551
________________________________
From: Confocal Microscopy List <[hidden email]> on behalf of Arnim Jenett <[hidden email]>
Sent: Wednesday, October 21, 2020 17:39
To: [hidden email] <[hidden email]>
Subject: Re: Leica SP8 confocal Windows 10 upgrade

*****
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.
*****

Dear confocalmicroscopy-list,
please allow me to reactivate this old thread because the problem persists: How to update the operating systems of Leica SP8 from Windows7 (end of life) to Windows10.
The (only) solution, which was recently offered to us by Leica, is to purchase a new workstation for ~9KEuro. And our team is not alone with this problem as I know at least 6 other microscopes with this issue.

Did this group find an alternative solution to this problem? Did anybody successfully upgrade the OS on the existing hardware - without breaking the system?

Any input on this is highly appreciated.
cheers, aRnim

--
Dr. Arnim Jenett
Imaging and Data Management
TEFOR Paris-Saclay,
CNRS UMS2010 / INRAE UMS1451,
Université Paris-Saclay

Bat 32, 1 Avenue de la Terrasse
91190 Gif-sur-Yvette, France
https://tps.tefor.net
________________________________

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Dear All,
thank you very much for the multitude of good ideas/solutions.
When I find some time we will dive into the approach of the LMU -
integrating the dd (and avoiding the frimware update) as suggested by
Zdenek.
The short-term solution - at least for our systems - however, will be
based on Kathy's suggestion: as our Microscopes already are directly
connected to a Linux file server which is pulling the data automatically
from the microscopes, we will simply take the SP8s offline and access
the files exclusively through the server. Thank you for opening my eyes,
there!
I'll report back on the progress/success (much later) so others can
profit from our experiences as I will from these of/at the LMU.
Gratefully, aRnim
PS: we are already running the ESU on these machines. Good point.


-------- Forwarded Message --------
Subject: Re: Leica SP8 confocal Windows 10 upgrade
Date: Wed, 21 Oct 2020 04:39:26 -0500
From: Arnim Jenett <[hidden email]>
To: [hidden email]
CC: Arnim Jenett <[hidden email]>



Dear confocalmicroscopy-list, please allow me to reactivate this old
thread because the problem persists: How to update the operating systems
of Leica SP8 from Windows7 (end of life) to Windows10. The (only)
solution, which was recently offered to us by Leica, is to purchase a
new workstation for ~9KEuro. And our team is not alone with this problem
as I know at least 6 other microscopes with this issue.
Did this group find an alternative solution to this problem? Did anybody
successfully upgrade the OS on the existing hardware - without breaking
the system?

Any input on this is highly appreciated. cheers, aRnim

--
Dr. Arnim Jenett
Imaging and Data Management
TEFOR Paris-Saclay,
CNRS UMS2010 / INRAE UMS1451,
Université Paris-Saclay

Bat 32, 1 Avenue de la Terrasse
91190 Gif-sur-Yvette, France
https://tps.tefor.net

*****
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.
*****

Dear list,

I’m looking for a software to align two 3D volumes. Basically, I am scanning volumes bi-directionally and there is a hysteresis between the up and downward motion. Now I’m looking for a software/ImageJ plug-in to correct this hysteresis.

So far we have tested:

https://imagej.net/Descriptor-based_registration_(2d/3d) <https://imagej.net/Descriptor-based_registration_(2d/3d)>

and

https://imagej.net/Fijiyama <https://imagej.net/Fijiyama>

However, we haven’t had the results we anticipated. The former only worked for 2D images for us.

Anyone has experience with this and can recommend us a good software? Perhaps even with a tutorial Video (e.g. the first plug in above has a nice tutorial: https://www.youtube.com/watch?v=SKW1xwhsxdo <https://www.youtube.com/watch?v=SKW1xwhsxdo>).

Thank you!
Nino Karpf



__________________________________
Prof. Dr. Sebastian 'Nino' Karpf
Juniorprofessor
 

University of Lübeck
Institute for Biomedical Optics (BMO)
 
Tel +49 451 3101 3240
E-Mail [hidden email] <mailto:[hidden email]>
www.bmo.uni-luebeck.de <http://www.bmo.uni-luebeck.de/>
 
Peter-Monnik-Weg 4
23562 Lübeck
Germany

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Hi Nino,
Alignment of 3D volumes can be done in FIJI, but is a little tricky since FIJI can only represent 3D data as stacks of slices. So if your volumes have to be aligned in XYZ and have shear/mag issues, FIJI will require a lot of trial and error and could still result in slice to slice variation. Is this something you have to perform regularly or a one-off issue?

If you want really effective N-D alignment I would recommend either going the hard route and coding it in Matlab or Python, or using a purchased software package like Imaris.

If you want to keep to free software, BigWarp in FIJI can do a great job but is mainly main for 2D images. FIJIyama or the other built-in registration plugins are probably your best options.

Cheers,
John


____________________________________________________________________________
John M. Heddleston  |  Director  |  Microscopy Facility
Cleveland Clinic  |  Florida Research & Innovation Center
Email: [hidden email]
Desk: 772.345.8117




From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Sebastian 'Nino' Karpf
Sent: Thursday, October 22, 2020 6:11 AM
To: [hidden email]
Subject: [BULK][EXT] Software Recommendation for 3D volume registration/alignment

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To join, leave or search the confocal microscopy listserv, go to:
http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy<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.
*****

Dear list,

I’m looking for a software to align two 3D volumes. Basically, I am scanning volumes bi-directionally and there is a hysteresis between the up and downward motion. Now I’m looking for a software/ImageJ plug-in to correct this hysteresis.

So far we have tested:

https://imagej.net/Descriptor-based_registration_(2d/3d)<https://imagej.net/Descriptor-based_registration_(2d/3d)> <https://imagej.net/Descriptor-based_registration_(2d/3d)<https://imagej.net/Descriptor-based_registration_(2d/3d)>>

and

https://imagej.net/Fijiyama<https://imagej.net/Fijiyama> <https://imagej.net/Fijiyama<https://imagej.net/Fijiyama>>

However, we haven’t had the results we anticipated. The former only worked for 2D images for us.

Anyone has experience with this and can recommend us a good software? Perhaps even with a tutorial Video (e.g. the first plug in above has a nice tutorial: https://www.youtube.com/watch?v=SKW1xwhsxdo<https://www.youtube.com/watch?v=SKW1xwhsxdo> <https://www.youtube.com/watch?v=SKW1xwhsxdo<https://www.youtube.com/watch?v=SKW1xwhsxdo>>).

Thank you!
Nino Karpf



__________________________________
Prof. Dr. Sebastian 'Nino' Karpf
Juniorprofessor


University of Lübeck
Institute for Biomedical Optics (BMO)

Tel +49 451 3101 3240
E-Mail [hidden email]<mailto:[hidden email]> <mailto:[hidden email]>
www.bmo.uni-luebeck.de<http://www.bmo.uni-luebeck.de> <http://www.bmo.uni-luebeck.de/<http://www.bmo.uni-luebeck.de>>

Peter-Monnik-Weg 4
23562 Lübeck
Germany


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I asked my colleague, Rob Clements. He replied: Fiji has a bunch of registration plugins built in that I have used .  You basically set coincidence points between the images and it warps them.
Turboreg i beleive is one but its been a while since ive done it.  I have also used a program called VIAS way back when.  Volume integration and alignment system, may be difficult to locate since its older.

-----Original Message-----
From: Confocal Microscopy List <[hidden email]> On Behalf Of Sebastian 'Nino' Karpf
Sent: Thursday, October 22, 2020 6:11 AM
To: [hidden email]
Subject: Software Recommendation for 3D volume registration/alignment

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Dear list,

I’m looking for a software to align two 3D volumes. Basically, I am scanning volumes bi-directionally and there is a hysteresis between the up and downward motion. Now I’m looking for a software/ImageJ plug-in to correct this hysteresis.

So far we have tested:

https://nam03.safelinks.protection.outlook.com/?url=https%3A%2F%2Fimagej.net%2FDescriptor-based_registration_&amp;data=04%7C01%7Cmmodel%40KENT.EDU%7C04a87804f41142af488808d876742e4e%7Ce5a06f4a1ec44d018f73e7dd15f26134%7C1%7C0%7C637389588655076957%7CUnknown%7CTWFpbGZsb3d8eyJWIjoiMC4wLjAwMDAiLCJQIjoiV2luMzIiLCJBTiI6Ik1haWwiLCJXVCI6Mn0%3D%7C1000&amp;sdata=gR0hQRhc6p2eMZwGuxLb%2FHgrdKP335jZ%2BBUw%2BrHnBco%3D&amp;reserved=0(2d/3d) <https://nam03.safelinks.protection.outlook.com/?url=https%3A%2F%2Fimagej.net%2FDescriptor-based_registration_&amp;data=04%7C01%7Cmmodel%40KENT.EDU%7C04a87804f41142af488808d876742e4e%7Ce5a06f4a1ec44d018f73e7dd15f26134%7C1%7C0%7C637389588655076957%7CUnknown%7CTWFpbGZsb3d8eyJWIjoiMC4wLjAwMDAiLCJQIjoiV2luMzIiLCJBTiI6Ik1haWwiLCJXVCI6Mn0%3D%7C1000&amp;sdata=gR0hQRhc6p2eMZwGuxLb%2FHgrdKP335jZ%2BBUw%2BrHnBco%3D&amp;reserved=0(2d/3d)>

and

https://nam03.safelinks.protection.outlook.com/?url=https%3A%2F%2Fimagej.net%2FFijiyama&amp;data=04%7C01%7Cmmodel%40KENT.EDU%7C04a87804f41142af488808d876742e4e%7Ce5a06f4a1ec44d018f73e7dd15f26134%7C1%7C0%7C637389588655076957%7CUnknown%7CTWFpbGZsb3d8eyJWIjoiMC4wLjAwMDAiLCJQIjoiV2luMzIiLCJBTiI6Ik1haWwiLCJXVCI6Mn0%3D%7C1000&amp;sdata=iA3i5r0r42CHR8lmYOkrhokFZjcr0nN345Bz4NlGNEM%3D&amp;reserved=0 <https://nam03.safelinks.protection.outlook.com/?url=https%3A%2F%2Fimagej.net%2FFijiyama&amp;data=04%7C01%7Cmmodel%40KENT.EDU%7C04a87804f41142af488808d876742e4e%7Ce5a06f4a1ec44d018f73e7dd15f26134%7C1%7C0%7C637389588655076957%7CUnknown%7CTWFpbGZsb3d8eyJWIjoiMC4wLjAwMDAiLCJQIjoiV2luMzIiLCJBTiI6Ik1haWwiLCJXVCI6Mn0%3D%7C1000&amp;sdata=iA3i5r0r42CHR8lmYOkrhokFZjcr0nN345Bz4NlGNEM%3D&amp;reserved=0>

However, we haven’t had the results we anticipated. The former only worked for 2D images for us.

Anyone has experience with this and can recommend us a good software? Perhaps even with a tutorial Video (e.g. the first plug in above has a nice tutorial: https://nam03.safelinks.protection.outlook.com/?url=https%3A%2F%2Fwww.youtube.com%2Fwatch%3Fv%3DSKW1xwhsxdo&amp;data=04%7C01%7Cmmodel%40KENT.EDU%7C04a87804f41142af488808d876742e4e%7Ce5a06f4a1ec44d018f73e7dd15f26134%7C1%7C0%7C637389588655076957%7CUnknown%7CTWFpbGZsb3d8eyJWIjoiMC4wLjAwMDAiLCJQIjoiV2luMzIiLCJBTiI6Ik1haWwiLCJXVCI6Mn0%3D%7C1000&amp;sdata=nr8xGrAA9I2mu%2Fvo%2B%2FtwiROQ3Ej%2B55ylx3%2Bq7RscbL8%3D&amp;reserved=0 <https://nam03.safelinks.protection.outlook.com/?url=https%3A%2F%2Fwww.youtube.com%2Fwatch%3Fv%3DSKW1xwhsxdo&amp;data=04%7C01%7Cmmodel%40KENT.EDU%7C04a87804f41142af488808d876742e4e%7Ce5a06f4a1ec44d018f73e7dd15f26134%7C1%7C0%7C637389588655076957%7CUnknown%7CTWFpbGZsb3d8eyJWIjoiMC4wLjAwMDAiLCJQIjoiV2luMzIiLCJBTiI6Ik1haWwiLCJXVCI6Mn0%3D%7C1000&amp;sdata=nr8xGrAA9I2mu%2Fvo%2B%2FtwiROQ3Ej%2B55ylx3%2Bq7RscbL8%3D&amp;reserved=0>).

Thank you!
Nino Karpf



__________________________________
Prof. Dr. Sebastian 'Nino' Karpf
Juniorprofessor


University of Lübeck
Institute for Biomedical Optics (BMO)

Tel +49 451 3101 3240
E-Mail [hidden email]<mailto:[hidden email]> <mailto:[hidden email]>
https://nam03.safelinks.protection.outlook.com/?url=http%3A%2F%2Fwww.bmo.uni-luebeck.de%2F&amp;data=04%7C01%7Cmmodel%40KENT.EDU%7C04a87804f41142af488808d876742e4e%7Ce5a06f4a1ec44d018f73e7dd15f26134%7C1%7C0%7C637389588655076957%7CUnknown%7CTWFpbGZsb3d8eyJWIjoiMC4wLjAwMDAiLCJQIjoiV2luMzIiLCJBTiI6Ik1haWwiLCJXVCI6Mn0%3D%7C1000&amp;sdata=xPJVIr%2FnrW7%2BuaHEb3DuzIkXqmrjEhYL5%2FxFZw%2FfIEI%3D&amp;reserved=0 <https://nam03.safelinks.protection.outlook.com/?url=http%3A%2F%2Fwww.bmo.uni-luebeck.de%2F&amp;data=04%7C01%7Cmmodel%40KENT.EDU%7C04a87804f41142af488808d876742e4e%7Ce5a06f4a1ec44d018f73e7dd15f26134%7C1%7C0%7C637389588655076957%7CUnknown%7CTWFpbGZsb3d8eyJWIjoiMC4wLjAwMDAiLCJQIjoiV2luMzIiLCJBTiI6Ik1haWwiLCJXVCI6Mn0%3D%7C1000&amp;sdata=xPJVIr%2FnrW7%2BuaHEb3DuzIkXqmrjEhYL5%2FxFZw%2FfIEI%3D&amp;reserved=0>

Peter-Monnik-Weg 4
23562 Lübeck
Germany

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** vendor reply **


Dear Nino,

Two, or even more, 3D volumes with similar structures can be
automatically aligned by treating them as different channels within our
Huygens Chromatic Aberration Corrector.
See https://svi.nl/Chromatic-Aberration-Corrector-Software

This tool estimates and corrects shifts, rotational differences and
changes in magnification. Typically these parameters are to be estimated
from a known structure like a multicolored bead, and then applied to the
biological image data acquired under the same conditions.

You can contact me offline for more info and a trial version.
Good luck,

Vincent

Vincent Schoonderwoert, PhD
Director Marketing & Science - imaging Specialist
Scientific Volume Imaging bv
Laapersveld 63, 1213VB
Hilversum, The Netherlands
Phone: +31 35 642 1626
[hidden email]






On 22-10-2020 12:10, Sebastian 'Nino' Karpf wrote:
Email Signature

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Hi Radek,

glad to hear it worked out for you at the end.

Yes, "a bit of hacking around" describes it quite appropriately, I am
afraid. Backup is essential, so that you can go back to the starting
point, if everything else should fail.

BTW, should you plan to upgrade to the linear scanning electronics
(Klondike Upgrade), that would come with a Win10 upgrade included (and
possibly new computer), since it does not run on Win7. From memory, it
increases the duty cycle in unidirectional mode from 25% to 65% (i.e.
the percentage of the total time during which photons are collected.)
With the same line frequency and pixel size, pixel dwell time goes up.
For some, it may be easier to convince funders to pay for 2.6x more
photons in the same time period (or respectively shorter acquisition
times), rather than a windows upgrade, although it is likely to be
several times more expensive than what Arnim mentioned as Win10 upgrade
costs.

But I totally agree with others that fencing Win7 systems off the
internet with a gateway computer is an efficient, fast and relatively
inexpensive way to solve the problem in many settings. I did that once
with a Win XP system hidden behind a NAS which had several Ethernet
ports, one to the outside net, and one to the microscope computer. That
worked very nicely.

Steffen

Am 22.10.2020 um 02:59 schrieb Radek Machan (Dr):
--
------------------------------------------------------------
Steffen Dietzel, PD Dr. rer. nat
Ludwig-Maximilians-Universität München
Biomedical Center (BMC)
Head of the Core Facility Bioimaging

Großhaderner Straße 9
D-82152 Planegg-Martinsried
Germany

http://www.bioimaging.bmc.med.uni-muenchen.de

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Hi Blaise,

I heard about the ESU option from one of your colleagues and had been
exploring it when this thread came up, great timing.  I am curious if
you or anyone else who has gone the ESU route has had any issues with
the updates interfering with the microscope control software at all?  I
know that sometimes security updates can include changes to the .net
framework which I've been warned about in the past.  Is this a valid
concern?

Thanks,
Ben

On 10/21/20 11:22 AM, Blaise Ndjamen wrote:
--
Benjamin Abrams,  Ph.D.
(He/Him/His)
Director
UCSC Life Sciences Microscopy Center

University of California, Santa Cruz
1156 High Street
150 Sinsheimer labs
Santa Cruz, CA 95064

Office/voicemail: (831) 459-3999
Mobile: (831) 332-0911

http://stemcell.soe.ucsc.edu/facilities/microscopy

Training Request Form:
http://goo.gl/forms/M9jd1ZHyohTnj0xk1

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Correct 3D Drift works really well.  In FIJI, go to
Plugins->Registration->Correct 3D Drift.  Some really nice features is that
it can register across multiple time domains (rather than just frame to
frame), can do subpixel registrations, and will drag along all the other
channels with the registered channel.  In fact, despite its name, we often
use this to register XYZ and XYT stacks because of the multiple time domain
feature.  The only catch is that it can only do rigid transforms, so no
rotation, affine, etc.

Cheers,
   Ben Smith

On Thu, Oct 22, 2020 at 6:07 AM MODEL, MICHAEL <[hidden email]> wrote:

--
Benjamin E. Smith, Ph. D.
Imaging Specialist, Vision Science
University of California, Berkeley
195 Life Sciences Addition
Berkeley, CA  94720-3200
Tel  (510) 642-9712
Fax (510) 643-6791
e-mail: [hidden email]
https://vision.berkeley.edu/faculty/core-grants-nei/core-grant-microscopic-imaging/

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We also went with extended Windows 7 security. We contacted the university IT and we didn't even have to pay for it. The university had purchased limited extended licenses. Was a quick fix!