Hands-on Confocal Course April 2010

CONFOCAL MICROSCOPY

4-Day Intensive Hands-On Course

Website: www.york.ac.uk/depts/biol/tf/imaging_course.htm

Basics, Live-cell imaging, FRET, FRAP and Spectral Unmixing

20-23 April 2010
Technology Facility, Dept. Biology
University of York, UK

Instructors will include

Peter O'Toole, University of York
Jo Marrison, University of York
Les Borland, Carl Zeiss
Colin Hornby, Perkin Elmer
and special guest lecture and practical session with Daniel Zicha (CRUK).

Tutorials and practical sessions will cover both basic and advanced
confocal microscopy. The course will enable participants to realise the
potential behind many developing confocal techniques and realise the
simplicity of applying the techniques to a broad range of sample types
and fluorescent labels. Both novice and more experienced users welcome.

Preliminary Programme
DAY AIMS
Day 1: Basics, Familiarisation, x,y,z and multicolour imaging.
Day 2: Live-cell imaging with spinning disk confocal microscopy, FRAP on
laser scanning confocal.
Day 3: Advanced Techniques covering spectral unmixing and FRET with
fluorescent proteins.
Day 4: Further advances. More samples to explore confocal limits, and
time for participants own samples.

Thursday evening will include a special guest speaker and course meal.

The course will utilise many different sample types ranging from
cultured monolayers to plant cells. A diverse range of fluorescent
labels will also be used, which will include various fluorescent
proteins (CFP, GFP and YFP) and classic antibody labels. Over the four
days, at least four confocal microscopes (2x Zeiss LSM 710 and 2x LSM
510 META on both an invert and upright microscopes, PerkinElmer
UltraVIEW LCI or VoX) will be utilised.

Accommodation (en-suite), breakfast and lunches will be provided for the
length of the course.  Evening meals will be provided on both Tuesday
and Thursday evenings.

Places are limited to 12 participants to permit full hands-on practice,
so please book early to avoid disappointment.
For further information, please visit the course website at:
www.york.ac.uk/depts/biol/tf/imaging-cytometry/imaging_course.htm

or contact Margaret Newton 01904 328821, [hidden email]

--
Dr Peter O'Toole
Head of Imaging and Cytometry
Technology Facility
Department of Biology (Area 15)
University of York
PO Box 373
YORK
YO10 5YW

Tel : +44 (0)1904 328722
Fax : +44 (0)1904 328804
email : [hidden email]
www.york.ac.uk/biology/tf

Hi Bertrand,

We need to get the Image J course on the map before somebody else thinks of it!

Best,

Patrizia


--
_______________________________________________________

Dr Patrizia Ferretti
Developmental Biology Unit
UCL Institute of Child Health
30 Guilford Street
London WC1N 1EH, UK

Tel:    (+44)  020-7829 8894 (direct line)
         (+44)  020 7905 2715 (secretary)
         (+44)  020 7242 9789 ICH switchboard

Fax:    (+44)  020 7831 4366

E-mail: [hidden email]

http://www.ich.ucl.ac.uk/ich/academicunits/Developmental_biology/Homepage
________________________________________________________

Carolina Workshop on Force Measurements and Manipulation in Biological Microscopy at UNC, Chapel Hill on May18-21, 2010.

We would like to let everyone know about our Sixth Annual Forces in Biology workshop.  It is back at its old time, mid-May, which is a great time to be in Chapel Hill.  The workshop is hosted by CISMM, our NIH resource (Computer Integrated Systems for Microscopy and Manipulation; CISMM.org). It consists of morning lectures followed by hands on force experiments on live specimens. The morning discussions provide a framework for understanding and analyzing forces on the micro and nanoscale, and serve as an introduction to the afternoon’s experiments. The afternoon sessions are hands-on laboratories where you perform force measurements such as fibrin fibers and perform biofluid rheology. Experiments use laser tweezers, an integrated atomic force microscopy/optical microscopy system, and 3D magnetic systems integrated with a fluorescence confocal microscope. We also include an introduction to microfluidics. Finally, participants spend a half day learning to use some of the many free software packages available from our resource that facilitate the analysis and visualization of 3D images and forces in biological systems (free analysis and visualization software is always available at CISMM.org). Registration is limited to 18, so you have lots of hands-on time with the microscopes and instructors. The $775 fee includes all supplies, light breakfasts, snacks and a conference dinner.
For more information go to http://cismm.cs.unc.edu/resources/events   Hope to see you there!

Hi!

I'm doing that for 5/6 six years ;)

Ecclesiastes 1:9

Nuno Moreno, PhD
___________
Equipment Management Unit, Head
Instituto Gulbenkian de Ciência
Fundação Calouste Gulbenkian
phone   +351 214464606
fax     +351 214407970

On 20-01-2010 15:33, Patrizia Ferretti wrote:

Hey, I've just had a great idea - what about a course that teaches the basics of ImageJ?

Patrizia Ferretti wrote:

Hi Bertrand,

We need to get the Image J course on the map before somebody else thinks of it!

Best,

Patrizia

CONFOCAL MICROSCOPY

4-Day Intensive Hands-On Course

Website: www.york.ac.uk/depts/biol/tf/imaging_course.htm

Basics, Live-cell imaging, FRET, FRAP and Spectral Unmixing

20-23 April 2010
Technology Facility, Dept. Biology
University of York, UK

Instructors will include

Peter O'Toole, University of York
Jo Marrison, University of York
Les Borland, Carl Zeiss
Colin Hornby, Perkin Elmer
and special guest lecture and practical session with Daniel Zicha (CRUK).

Tutorials and practical sessions will cover both basic and advanced confocal microscopy. The course will enable participants to realise the potential behind many developing confocal techniques and realise the simplicity of applying the techniques to a broad range of sample types and fluorescent labels. Both novice and more experienced users welcome.

Preliminary Programme
DAY AIMS
Day 1: Basics, Familiarisation, x,y,z and multicolour imaging.
Day 2: Live-cell imaging with spinning disk confocal microscopy, FRAP on laser scanning confocal.
Day 3: Advanced Techniques covering spectral unmixing and FRET with fluorescent proteins.
Day 4: Further advances. More samples to explore confocal limits, and time for participants own samples.

Thursday evening will include a special guest speaker and course meal.

The course will utilise many different sample types ranging from cultured monolayers to plant cells. A diverse range of fluorescent labels will also be used, which will include various fluorescent proteins (CFP, GFP and YFP) and classic antibody labels. Over the four days, at least four confocal microscopes (2x Zeiss LSM 710 and 2x LSM 510 META on both an invert and upright microscopes, PerkinElmer UltraVIEW LCI or VoX) will be utilised.

Accommodation (en-suite), breakfast and lunches will be provided for the length of the course.  Evening meals will be provided on both Tuesday and Thursday evenings.

Places are limited to 12 participants to permit full hands-on practice, so please book early to avoid disappointment.
For further information, please visit the course website at:
www.york.ac.uk/depts/biol/tf/imaging-cytometry/imaging_course.htm

or contact Margaret Newton 01904 328821, [hidden email]

--
Dr Peter O'Toole
Head of Imaging and Cytometry
Technology Facility
Department of Biology (Area 15)
University of York
PO Box 373
YORK
YO10 5YW

Tel : +44 (0)1904 328722
Fax : +44 (0)1904 328804
email : [hidden email]
www.york.ac.uk/biology/tf

I normally spend 6-8 weeks of my microscopy course on digital
imaging, based primarily on ImageJ.  

If you look at the ImageJ site, you will find several tutorials on
the subject.  Check:  
http://rsb.info.nih.gov/ij/docs/examples/index.html

Among the resources is an introductory powerpoint that I presented at
the M&M meeting in 2008:
 http://rsb.info.nih.gov/ij/docs/examples/IJ-M&M08.ppt 
 --of couse, in the past two years, there have been many
improvements, but the basics remain.

Joel


-------------- Original message ---------------
Hey, I've just had a great idea - what about a course that teaches
the basics of ImageJ?

Patrizia Ferretti wrote:
    Hi Bertrand,
   
    We need to get the Image J course on the map before somebody else
    thinks of it!
   
    Best,
   
    Patrizia

    CONFOCAL MICROSCOPY
   
    4-Day Intensive Hands-On Course
   
    Website: www.york.ac.uk/depts/biol/tf/imaging_course.htm
   
    Basics, Live-cell imaging, FRET, FRAP and Spectral Unmixing
   
    20-23 April 2010
    Technology Facility, Dept. Biology
    University of York, UK
   
    Instructors will include
   
    Peter O'Toole, University of York
    Jo Marrison, University of York
    Les Borland, Carl Zeiss
    Colin Hornby, Perkin Elmer
    and special guest lecture and practical session with Daniel Zicha
    (CRUK).
   
    Tutorials and practical sessions will cover both basic and advanced
    confocal microscopy. The course will enable participants to realise
    the potential behind many developing confocal techniques and realise
    the simplicity of applying the techniques to a broad range of sample
    types and fluorescent labels. Both novice and more experienced users
    welcome.
   
    Preliminary Programme
    DAY AIMS
    Day 1: Basics, Familiarisation, x,y,z and multicolour imaging.
    Day 2: Live-cell imaging with spinning disk confocal microscopy, FRAP
    on laser scanning confocal.
    Day 3: Advanced Techniques covering spectral unmixing and FRET with
    fluorescent proteins.
    Day 4: Further advances. More samples to explore confocal limits, and
    time for participants own samples.
   
    Thursday evening will include a special guest speaker and course
    meal.
   
    The course will utilise many different sample types ranging from
    cultured monolayers to plant cells. A diverse range of fluorescent
    labels will also be used, which will include various fluorescent
    proteins (CFP, GFP and YFP) and classic antibody labels. Over the
    four days, at least four confocal microscopes (2x Zeiss LSM 710 and
    2x LSM 510 META on both an invert and upright microscopes,
    PerkinElmer UltraVIEW LCI or VoX) will be utilised.
   
    Accommodation (en-suite), breakfast and lunches will be provided for
    the length of the course. Evening meals will be provided on both
    Tuesday and Thursday evenings.
   
    Places are limited to 12 participants to permit full hands-on
    practice, so please book early to avoid disappointment.
    For further information, please visit the course website at:
    www.york.ac.uk/depts/biol/tf/imaging-cytometry/imaging_course.htm
   
    or contact Margaret Newton 01904 328821, [hidden email]
   
    --
    Dr Peter O'Toole
    Head of Imaging and Cytometry
    Technology Facility
    Department of Biology (Area 15)
    University of York
    PO Box 373
    YORK
    YO10 5YW
   
    Tel : +44 (0)1904 328722
    Fax : +44 (0)1904 328804
    email : [hidden email]
    www.york.ac.uk/biology/tf
   


--

(Sent from my cra%#y non-Blackberry electronic device that still has
wires)

*********************************
John Runions, Ph.D.
School of Life Sciences
Oxford Brookes University
Oxford, UK
OX3 0BP

email: [hidden email]
phone: +44 (0) 1865 483 964
Runions´lab web site

Visit The Illuminated Plant Cell dot com
Oxford Brookes Master's in Bioimaging with Molecular Technology