SP5 vs fluoview 1000 for FCS modification ?

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Hi,

I'm wondering if onyone has experience with modifying a SP5 or a Fluoview
1000 for FCS mesures ? I work with Olympus stands before and they generally
offer good access to external ports. But what a bout the SP5 ?
 

Thanks

JP

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Dear Jean-Pierre,

I've do direct experience with an SP5 but we have a functional FCS setup
on an SP2. As far as I know in this respect there is no difference
between the SP2 and the SP5. There is simply an external port on the
confocal head-where you can insert your detector. As far as I know you
can purchase an FCS unit also from Leica. One of the advantages if you
do this, that you can use the APD-s for imaging and their sensitivity is
superior compared to the PMT-s.

Cheers    Gabor

--
Gabor Csucs
Light Microscopy Centre, ETH Zurich
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Jean-Pierre,

on both systems one needs to install the external port modification (X1
/ port 4 option), in order to bring the light out of the scan-head.
Beside that, it's just another discussion about which system offers
better transmission - dichromatic mirrors or AOBS.

Gabor, can you control the APDs for imaging via the Leica software, or
do you have to use an external solution?

Michael


Jean-Pierre CLAMME wrote:

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Dear Jean-Pierre,

on both systems one needs to install the external port modification (X1
/ port 4 option), in order to bring the light out of the scan-head.
Beside that, it's just another discussion about which system offers
better transmission - dichromatic mirrors or AOBS.

Gabor, can you control the APDs for imaging via the Leica software, or
do you have to use an external solution? It's pity that Leica doesn't
offer an internal APD-option including "spectral freedom".

Michael


Jean-Pierre CLAMME wrote:

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Ts, first rejected, then sent... I don't get it. Sorry for the
double-posting.

Michael


Michael Weber wrote:

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Dear Michael,

You can control the APDs from the Leica software - you see them like
"normal" PMTs. I agree with you that it would be nice (especially with
the resonant scanner of the SP5) to have them "behind" the spectral
separation.

Cheers   Gabor

--
Gabor Csucs
Light Microscopy Centre, ETH Zurich
Schafmattstrasse 18, HPM F16
CH-8093, Zurich, Switzerland

Web: www.lmc.ethz.ch
Phone: +41 44 633 6221
Fax: +41 44 632 1298
e-mail: [hidden email]

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Hi Jean-Pierre,

We did modify a FV300 system for FCS measurement, there is detailed
description about modification with technical drawing in our paper
published on Review of Scientific Instrument, here is the link
(http://dx.doi.org/10.1063/1.2740053 ).

It should not be very difficult if you also need to do APD imaging,  in
principle, you can bypass one fluorescence channel and connect that in
control box to APD output (maybe signal conversion needed here). The
modified system is not expensive and its performance is pretty good.

Best Regards,
Xiaotao



Jean-Pierre CLAMME wrote:

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Could you please send me a pdf version of your paper ?

Thanks

Jean-Pierre

Pan Xiaotao wrote:
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Dr. Jean-Pierre CLAMME
Supervisor 2-Photon Imaging Facility
Dept. of Immunology, IMM-1, R310
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Hi,

First thank you for the infos.

Second do you need to go back through the scan heads ? Is it possible to
use another side port to extract the light for example to do cross
correlation ? I worked on two home made systems (FCS + imaging and
single molecule) were we would collect the light directly  after the
objective and redirect the signal to multiple APDs. On the SP5 we have
here we have external detectors. Could that kind of approach  be used ?

Thanks

JP

Michael Weber wrote:
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Dr. Jean-Pierre CLAMME
Supervisor 2-Photon Imaging Facility
Dept. of Immunology, IMM-1, R310
The Scripps Research Institute
10550 North Torrey Pines Rd.
La Jolla, California 92037

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When I say external detectors for the SP5 I mean NDDs.

JP


Jean-Pierre CLAMME wrote:
--
Dr. Jean-Pierre CLAMME
Supervisor 2-Photon Imaging Facility
Dept. of Immunology, IMM-1, R310
The Scripps Research Institute
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La Jolla, California 92037

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Hi Folks,
Please circulate the job posting below to anybody you think would be interested. Please apply through the website.
Thanks,
Tony



A Research Assistant is required to support the management of the day-to-day activities of the robotic cell culture and liquid handling systems at the McMaster Biophotonics Facility.  The Facility is an integrated suite of state-of-the-art fluorimetry, microscopy, cytometry and high-content screening systems serving McMaster University and Southern Ontario.  The successful candidate will work under the direction of the Manager and Director of the McMaster Biophotonics Facility.  Duties include:  Support of the Facility's automated cell culture and high content screening platforms including ThermoFisher WorkCells, ArrayScan, PE Opera, Nikon Biostation; Responsible for the routine administration of the high content screening system in the Facility; Assist in the organization of workshops at the Facility; Maintenance, calibration, programming and upgrading instruments in the Facility as directed.  The incumbent must have demonstrated experience and knowledge in high content screening including skill in individual support to personnel on the use and applications of high content screening is desirable; Ability to organize and conduct imaging workshops, and willingness to work effectively with researchers with diverse goals and experience is essential; Experience in programming for image processing and acquisition routines; Experience in cell culture and molecular biology are desirable.  Applicants must possess a minimum BSc degree in biology, chemistry, biochemistry, physics or medical engineering and appropriate experience.

http://www.workingatmcmaster.ca/careers/job_details.php?PHPSESSID=8d63c417c23654624eed50909255c6ba&selected_job=3467

Tony J. Collins, Ph.D.
McMaster Biophotonics Facility
Dept. Biochemistry and Biomedical Sciences HSC 4H21A
McMaster University, Hamilton, ON, Canada, L8N 3Z5
[hidden email]     www.macbiophotonics.ca

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That's right, Gabor.

We have an SP5 with a dual channel FCS unit attached. The version we
have was supplied by Leica and is made by ISS. The Leica software has a
pretty good FCS "wizard" that manages the interface between the Leica
and the ISS gear, which is run off a second computer. After a very
shakey start, it now works well.

I think it would be possible to put your own FCS unit on the external
port and control the lightpath selection, scan parameters manually, but
you'd need to check, I reckon.

IAN

On Wednesday, June 18, 2008, at 03:18  PM, Csucs Gabor wrote:

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Prof Ian Gibbins
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The light path on the SP5 goes to the side port via the scan mirrors
but not the spectral separation path. Going via the scan mirrors allows
you to place the beam at a series of locations when collecting a set of
FCS data (though you could do this by moving the stage with a simply
parked beam I suppose). The set-up we have uses a dichroic and barrier
filters to separate emission bands to two APDs. It works well, but, of
course, you have to change the filter / mirror combinations if you
change your cross-correlation fluorophores, but that is pretty easy too.

IAN


On Thursday, June 19, 2008, at 02:45  AM, Jean-Pierre CLAMME wrote:

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Prof Ian Gibbins
Anatomy & Histology
Flinders University
GPO Box 2100
Adelaide SA 5001
AUSTRALIA

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This is what we were doing on our system. We would choose  a point and
then move the table to bring that point under the parked beam.
I'm just wondering, is the fact  that scanning moves the beam  changing
the focal volume from one point to the other ? Or is it negligible ?

Thanks

JP
> The light path on the SP5 goes to the side port via the scan mirrors
> but not the spectral separation path. Going via the scan mirrors
> allows you to place the beam at a series of locations when collecting
> a set of FCS data (though you could do this by moving the stage with a
> simply parked beam I suppose).
This is what we were doing on our system. We would choose  a point and
then move the table to bring that point under the parked beam.
I'm just wondering Is the fact that when you use the scanner, you  but
the fact that when you use the scanner,


>
> [hidden email]
> voice: +61-8-8204 5271
> fax: +61-8-8277 0085
>
> http://som.flinders.edu.au/FUSA/Anatomy/
> http://www.flinders.edu.au/neuroscience
>

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We've measured that and it's negligible under our usual conditions,
which is a relief...

IAN


On Thursday, June 19, 2008, at 08:54  AM, Jean-Pierre CLAMME wrote:

* * * * * * * * * * *
Prof Ian Gibbins
Anatomy & Histology
Flinders University
GPO Box 2100
Adelaide SA 5001
AUSTRALIA

[hidden email]
voice: +61-8-8204 5271
fax: +61-8-8277 0085

http://som.flinders.edu.au/FUSA/Anatomy/
http://www.flinders.edu.au/neuroscience

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There is also a way to use external detectors, pretty much with any confocal
microscope, without worrying about alignment issues. We have used an
external APD to perform FCS at any chosen position in the image. More
details are in  "Fluorescence correlation microscopy with real-time
alignment readout", Kaushalya et al., Applied Optics, vol. 44 (2005) p.3262.
You may contact me off the list if you need to know more.
Sudipta

On Wed, 18 Jun 2008 16:24:49 -0700, Jean-Pierre CLAMME wrote

Dr. Sudipta Maiti
Associate Professor
Dept. of Chemical Sciences
Tata Institute of Fundamental Research
Homi Bhabha Raod, Colaba, Mumbai 400005
Ph. 91-22-2278-2716 / 2539
Fax: 91-22-2280-4610
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