I've never worked with C elegans but menthol is an effective anaesthetic
for many invertebrates. Just put a lump in the medium and remove it
when they stop moving. Rinse and dry the menthol for next time.
Guy
Optical Imaging Techniques in Cell Biology
by Guy Cox CRC Press / Taylor & Francis
http://www.guycox.com/optical.htm______________________________________________
Associate Professor Guy Cox, MA, DPhil(Oxon)
Australian Centre for Microscopy & Microanalysis,
Madsen Building F09, University of Sydney, NSW 2006
Phone +61 2 9351 3176 Fax +61 2 9351 7682
Mobile 0413 281 861
______________________________________________
http://www.guycox.net
-----Original Message-----
From: Confocal Microscopy List [mailto:
[hidden email]]
On Behalf Of Jay Vyas
Sent: Thursday, 26 August 2010 2:03 AM
To:
[hidden email]
Subject: Protocol for imaging C. elegans on inverted spinning disk
confocal microscope
Hi-
We have a collaborator who is interested in confocal microscopy of C.
elegans. We have not done work with this organism and are looking for
the
best way to immobilize the worm and prepare the sample for imaging on
our
spinning disk confocal microscope. We have a typical inverted microscope
set-
up (Nikon body).
The collaborator prefers to keep the worm(s) alive, so we need a method
to
immobilize them (anesthesia?).
Do folks use agar when mounting samples? Which slides are typically used
for
this purpose? If there is a reference, I would love to get the citation.
Thanks,
Jay Vyas
Massachusetts General Hospital
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