LaVision TriM multiphoton microscope

There is a system developed 2 years ago by Light 4 Tech in Siena.

64 beams from a diffractive lens. It works fine and is very fast.

You should see the papers Prof. Pavone have read at Neuroscience or contact him directly.

vincenzo

 

Vincenzo Ricco

technical director

Crisel Instruments srl

via Mattia Battistini 177

00167 Roma

ITALY 

phone +39 06 35402933

fax: +39 06 35402879

<a href="blocked::mailto:ricco@crisel-instruments.it" title="blocked::mailto:ricco@crisel-instruments.it">ricco@...

www.crisel-instruments.it

---

From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Phillips, Thomas E.
Sent: Monday, April 26, 2010 4:15 AM
To: [hidden email]
Subject: LaVision TriM multiphoton microscope

 

I have been reading about the TriM multiphoton microscope from LaVision BioTec (http://www.lavisionbiotec.com/en/microscopy-products/trim-scope/). They use a combination of mirrors and a beam splitting substrate to divide the incoming beam into 64 beamlets and this lets them scan with 64 lines at once thereby cutting the scan time. They also use a combination of CCDs and NDDs as detectors. Can anybody comment on how effective this system is? Tom

 

Thomas E. Phillips, Ph.D.

Professor of Biological Sciences

Director, Molecular Cytology Core

2 Tucker Hall

Biological Sciences

University of Missouri

Columbia, MO 65211-7400

573-882-4712 (voice)

573-882-0123 (fax)

 

Internal Virus Database is out of date.
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Tom, you might want to contact them by phone (either through the US office at Ragona Scientific or at the German headquarter) and ask for a user reference list if you do not receive enough feedback through this listserv. I have seen their 64 beam system but I do not have enough experience on it to comment on effectiveness.

Urs Utzinger, University of Arizona

The TriM scope is a great system.  We demo-ed it here in New York a
couple of years ago.  I was particularly impressed by the fact that they
shipped it out here from Germany and then had it up and running well on
live samples within about 2 hours.  You can use it either in single-beam
mode if you need to image deep, or in the 64-beam mode if you need to go
fast but don't have such a requirement for depth.  In the 64-beam mode I
seem to remember we were limited to about 100-150 microns in depth,
while in the regular mode we could go to around 300 microns or deeper,
depending on the tissue.  But the 64-beam mode certainly is fast, so
although there are several excellent multiphoton options out in the
field now - Olympus, Prairie, Zeiss etc. - I do think that the TriM has
its own niche.
A good thing about the company is that they are extremely knowledgeable
and also very flexible about the system design - for example, they have
integrated OPO lasers on their systems for some time now.  The only
downside as far as we were concerned is that it is a multiphoton-only
system, and although I can see many advantages to that myself, some of
my users were adamant about wanting visible lasers on our system as
well.  If you contact Sid Ragona, their US rep,
(www.RagonaScientific.com) he can give you names of people in the US who
are using the system.

Best,
Alison



Phillips, Thomas E. wrote:
--
Alison J. North, Ph.D.,
Research Assistant Professor and
Director of the Bio-Imaging Resource Center,
The Rockefeller University,
1230 York Avenue,
New York,
NY 10065.
Tel: office ++ 212 327 7488
Tel: lab     ++ 212 327 7486
Fax:         ++ 212 327 7489

I have a confocal extension on the "TriM scope I" and it is attached to the OPO port.

Hello,
          We are trying to harvest adherent cells following activation
with IL-1 for certain receptor upregulation. However, we  feel that the
trypsin-EDTA mixture used for harvesting is cleaving the receptors.
Can somebody suggest a proven non-enzymatic cell harvesting solution.


Thanks,

-Prabhakar

I think you should test all reagents against your protein of interest - but I use TryplE Express for my receptor tyrosine kinases with success.

Sent from my Verizon Wireless BlackBerry

-----Original Message-----
From: "B. Prabhakar Pandian" <[hidden email]>
Date: Mon, 26 Apr 2010 11:25:48
To: <[hidden email]>
Subject: Non Enzymatic Cell Harvesting Buffer

Hello,
          We are trying to harvest adherent cells following activation
with IL-1 for certain receptor upregulation. However, we  feel that the
trypsin-EDTA mixture used for harvesting is cleaving the receptors.
Can somebody suggest a proven non-enzymatic cell harvesting solution.


Thanks,

-Prabhakar

El 26/04/2010 18:25, B. Prabhakar Pandian escribió:
Hi,

Using cold PBS-EDTA (no trypsin), adherent cells detach although more
slowly.

Javier

Dear all,

Can anyone tell me which is the optimal mounting media (composition) for
quantum dots labelled samples? Which reactives should be avoided  during
the immunochemistry with QD?

Thank you for your help!

Maria Calvo

--
Dra. Maria Calvo

 Microscòpia Confocal. Unitat de Microscòpia
 Serveis Cientificotècnics-Campus Casanova
 Facultat de Medicina
 Universitat de Barcelona. IDIBAPS
 Casanova 143
 Barcelona 08036

 Tel: 34 934037159
 Fax: 34 934044408
 E-mail: [hidden email]

As far as I remember only cytoseal can be used.  Others will kill the QD's.

Diane

-----Original Message-----
From: Confocal Microscopy List
[mailto:[hidden email]]On Behalf Of Maria Calvo
Sent: Monday, April 26, 2010 2:30 PM
To: [hidden email]
Subject: Quantum dots mounting media


Dear all,

Can anyone tell me which is the optimal mounting media (composition) for
quantum dots labelled samples? Which reactives should be avoided  during
the immunochemistry with QD?

Thank you for your help!

Maria Calvo

--
Dra. Maria Calvo

 Microscòpia Confocal. Unitat de Microscòpia
 Serveis Cientificotècnics-Campus Casanova
 Facultat de Medicina
 Universitat de Barcelona. IDIBAPS
 Casanova 143
 Barcelona 08036

 Tel: 34 934037159
 Fax: 34 934044408
 E-mail: [hidden email]

This is correct. Some mounting media can not be used with Qdots.
Invitrogen sells a mounting media specifically for Qdots called QMount.

Kelly
-no commercial interest



Kelly Rogers PhD
The Walter & Eliza Hall Institute
1G Royal Parade, Parkville
Victoria 3052, Australia
ph: +61_3_9345 2450


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Which mounting solutions should be avoided? I'd like to increase the
time spent in the 'off state' for a QD labelled sample.

Colin
--

Dr Colin Rickman
Department of Chemistry (WP 2.03)
School of Engineering and Physical Sciences
Heriot-Watt University
Edinburgh
EH14 4AS

Tel: +44 131 4514193 (Office)
Tel: +44 131 6511512
Fax: +44 131 650312


On 27/04/2010 02:27, Diane G Miller wrote: 8

I've also had great experiences with LaVision. They are willing into incorporate custom ordered components, which they can produce with exquisite craftsmanship and elegant design. Very knowledgeable staff and most importantly, a desire to sell and support products that work.

I order a modified version of the TriM a couple of years ago, which now can be ordered as a standard model, so I can't comment on the 64 beam mode. This microscope is dedicated to a single beam of a two-photon laser and has a motorized control of the fill of the back aperture of the objective. It has been a total workhorse in an in vivo imaging facility that scans for hours at a time, day after day. The software doesn't have the same glitz and gloss that the major manufacturers offer, but the plus side is that it is easy to write macros that can be plugged into the software (if you are into that sort of thing).

They have a number of microscope in the US, but are a moderate sized company based in Germany. However, they respond quickly to my emails and phone calls and will stop by when they are in the area visiting other installed microscopes or conferences. I have even had a video conference once to assess a potential issue in real time, transcontinental, more quickly than a representative could have arrived.

Feel free to call with questions you might have,
Ann



--
Ann Haberman, PhD

Department of Laboratory Medicine
Yale University School of Medicine
300 Cedar Street
TAC S541
New Haven, CT 06510

203-785-7349
203-785-5415 (fax)
[hidden email]

Hi,

Answering the question from Colin Rickman, I found in the archives from
2006 an answer from Mike Ignatius to a similar question (he talks about
blinking).

My question was also related to that mail, what types of mounting media
are compatible to Quantum dots?

Thank you!
Maria Calvo

Find below the mail from the archives:

Dear Laurent,

Caution, Vendor's somewhat torn response.

We sell both products and have of course compared them. (I will assume
since you call them QDots that you are using our product.) You asked
about size and blinking.

Size:

The QDot nanocrystal conjugates are indeed larger than organic dyes.
Depending on the color (the redder the bigger) they can reach 10 to 15
nm's and with full IgGs decorating them (2-4 on average) even larger. So
like DPI for printers, larger is not better for high resolution ICC.
However, we only see real big differences when we deconvolve the images,
since this is all sub-resolution.

However, the packing density is less. So while QDot nanocrystals are
brighter in the vial, on your prep they are more likely equivalent in
terms of brightness to Alexa dyes - less dots per unit area when
compared to dyes.

A cautionary note: Please do not use Prolong or Prolong Gold or anything
but cytoseal or PBS glycerol type mountants, such as our SlowFade gold
for mounting QDot Nanocrystals. They will disappear overnight. We have
an ever growing "n" value on this behavior. Our PIS stipulates this with
the product.)

Blinking:

The blinking is certainly apparent to the eye and thus to fast cameras.
Integrating over time avoids this concern - merely reduce your lamp
intensity to help out. We see the blinking with individual dots the
most, while ensembles tend to average out. It is worth noting that some
have found the blinking a nice confirmation that they are looking at a
nanocrystals, not background or organic dyes.

When to use Organic dyes when to use Nanocrystals?

This is where we are sometimes torn. The narrow full width half maximums
of Qdot nanocrystals, as you describe, indeed allow more colors. The
photostability, while terrific for live cell work, rare event detection
and repeated scanning of confocal stacks, is less of a boon in wide
field, single scan experiments. Especially with good dyes and antifades.
So when you need photostability or more colors, nanocrystals are worth
considering.

Mike Ignatius

Molecular Probes/Invitrogen.

------------------------------------------------------------------------

*From:* Confocal Microscopy List [mailto:[hidden email]]
*On Behalf Of *laurent barbe
*Sent:* Thursday, July 27, 2006 12:49 AM
*To:* [hidden email]
*Subject:* Qdot vs Alexa

Search the CONFOCAL archive at
http://listserv.acsu.buffalo.edu/cgi-bin/wa?S1=confocal

Dear users,

I have a quite broad, general question for users who experienced these 2
dyes. I’m doing colocalization study with 3d stacks, which means quite
long exposure. I am doing 4 color imaging, which made me try Qdots to be
able to fit all probes trying to reduce overlapping.

Obviously Qdots are more stable for long exposure than Alexa dyes but
I’d like to have user’s feedbacks from people who compared both.

I also read many times that Qdots blink, even thouh I haven’t faced this
problem yet, as well as Qdots are more ‘bulky’ after conjugation
compared to Alexa.

Any thoughts and feedbacks would be appreciated.

Thanks

Laurent

______________________________________________

Laurent Barbe, Research Fellow

Royal University of Technology (KTH)

School of Nanobiotechnology - Dpt of Biotechnology

Roslagstullsbacken 21, 10601 STOCKHOLM

SWEDEN

Tel: (+46) 855378832

Fax: (+46) 855378323



--


___________________________________

Dra. Maria Calvo

Unitat de Microscòpia Confocal
Serveis Cientificotècnics-C.Casanova
Facultat de Medicina
Universitat de Barcelona- IDIBAPS
C/ Casanova 143
Barcelona 08036

Tel: 34 934037159/39930
Fax: 34 934039946
E-mail: [hidden email]
___________________________________

Hi

Thanks for the archive email. My question wasn't so much about observing
blinking but enhancing it (hence I have changed the subject line to
reflect this). Most recent research has been focused on trying to reduce
or eliminate the blinking observed by Quantum dots. I would like to know
if anybody has any ideas on how to increase either the frequency of
blinking or increase the time the quantum dot spends in the "off" state.

Any advice gratefully received

Regards

Colin

--
Dr Colin Rickman
Department of Chemistry (WP 2.03)
School of Engineering and Physical Sciences
Heriot-Watt University
Edinburgh
EH14 4AS

Tel: +44 131 4514193 (Office)
Tel: +44 131 6511512
Fax: +44 131 6503128



On 28/04/2010 17:24, Maria Calvo wrote:

Colin,

We have been doing this with QDs for some time now.
But it really depend on what sample you're tryin to image.
There are a number of ways to go about this. First you
have to realize that generally, aside from size, QDs' fluorescence
properties (QY, Blinking) will depend on their surface.
Commercial QDs come in different forms, most of the "good ones"
come with a well passivated surface. Assuming that these are the ones you're using, you can try to do the following to make them blink more:
1. easiest: max power excitation. Put your laser on max and go.
2. Adding stuff to your imaging buffer- purging your buffer with Oxygen gas, or adding just adding oxidants, chelates, reductants etc
might do the job and increase blinking.
3. Diminishing the surface quality of QDs before using them.
This could be done by:
- spin down your QDs stock, and grab the ones that precipitated,
these will have bad surface quality.
-using and aged stock.
- storing them at RT for a few hrs/day/wks.
- storing them at RT + exposing them to light.
-Sonicating them.(vary the time)
Combining any of the above.
You can also combine it with 1 and 2.
And again, this will also depend on whatever you're tryin to image
in solution, live cells, fixed cells, method of conjugation etc
Hope this helps.

Eli



---- Original message ---- ________________________________
Eli Rothenberg, Ph.D.
Postdoctoral Fellow,
Department of Physics,
NSF Center for the Physics
of Living Cells,
University of Illinois - Urbana,
1110 W. Green St.
Urbana, 61801.
Illinois, USA
Tel: +217-244-5829;
Email: [hidden email]