Importing Leica time-lapse sequences into ImageJ

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Hi all,

Can anyone tell me whats the easiest way to import a multiple channel
with z stacks time-lapse sequence into imageJ?  We used a Leica sp2 so
the file type is Leica .lei

thanks,

Matt Pearson.

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Hi Matt,
        Would something like this do what your after?

http://rsbweb.nih.gov/ij/plugins/leica.html


and possibly the BioFormats plugin might do it too


http://www.loci.wisc.edu/ome/formats.html


Cheers


Cam


Cameron Nowell
Research and Microscopy Imaging Core
Peter MacCallum Cancer Centre
Melbourne, Australia

-----Original Message-----
From: Confocal Microscopy List [mailto:[hidden email]] On
Behalf Of Matthew Pearson
Sent: Tuesday, 19 August 2008 9:49 PM
To: [hidden email]
Subject: Importing Leica time-lapse sequences into ImageJ


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Hi all,

Can anyone tell me whats the easiest way to import a multiple channel
with z stacks time-lapse sequence into imageJ?  We used a Leica sp2 so
the file type is Leica .lei

thanks,

Matt Pearson.

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Hi,

I have used bioformat to import leica z stacks time-lapse files and then
the image5D (http://rsbweb.nih.gov/ij/plugins/image5d.html ) plugin to
visualize them.

Jean-Pierre


Matthew Pearson wrote:
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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

Lab number: (858)784-8184
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Dear Matt,

use the LOCI bio-formats plugin for imageJ.
It reads nearly everything, and also lets you see all the meta data!

BioImageXD should also read your .lei files for easier 3D rendering
and movie making than imageJ (at the moment)

cheers

Dan



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I ran into this problem several years ago, with a Leica sp1.  At the
time, Benjamin Matthieu wrote up a set of routines that import the
files, allowing you to select which ones you want.  The set has not
been made publically available because they are still somewhat crude.
 However, I would be happy to share them.

My file structure involves a file name of the form:  
r5 6-8-04_Series002_t00_z002_ch00.tif  

in which the channels switch at each z level.

Mattieu's plugin has an option called : time proj.  This reads the
selected channel, and then for each time point, reads all of the z
positions into a temporary stack, and then does a Max projection of
the stack.  That projection is then added to a new stack that grows
with each time point.  The end result is a single stack in which each
image is the max projection of the images of a "single" time point.

The process is quite slow, since it involves reading and writing a
large number of images.  

A major problem with these routines is that they do not insert the
calibration data into the images.  You do that by clicking on
"parameters", and entering the data manually into the properties
fields.
Also, when you select a file, you have to reclick on it to cancel.  

Nevertheless, I find them quicker than the LOCI routines, and they
are sensitive to sequential scan records.

Joel


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Biology Department, Temple University
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