LISTSERV - CONFOCALMICROSCOPY Archives

CONFOCALMICROSCOPY Archives

September 2011

CONFOCALMICROSCOPY@LISTS.UMN.EDU

	LISTSERV Archives
	CONFOCALMICROSCOPY Home
	CONFOCALMICROSCOPY September 2011

	Log In
	Register

	Subscribe or Unsubscribe

	Search Archives

Options:	Use Monospaced Font Show Text Part by Default Show All Mail Headers
Message:	[<< First] [< Prev] [Next >] [Last >>]
Topic:	[<< First] [< Prev] [Next >] [Last >>]
Author:	[<< First] [< Prev] [Next >] [Last >>]

Subject:	C. elegans imaging
From:	"Claire Brown, Dr." <[log in to unmask]>
Reply To:	Confocal Microscopy List <[log in to unmask]>
Date:	Sat, 24 Sep 2011 01:37:24 +0000
Content-Type:	text/plain
Parts/Attachments:	text/plain (22 lines)

*****
To join, leave or search the confocal microscopy listserv, go to:
http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
*****


We have a lab that wants to screen a C. Elegans genetic library with about 18,000 genes. They want to take images of the worms on 24 well plates and measure the distance between 2 of 3 EGFP spots on the worms.

We would like to do the experiments on an inverted HCS automated microscope. The problem is they have the worms growing on a ~1 mm thick nutrient-rich agar layer.

We need to image the worms through the agar so we need to find a different way to prepare the samples. Has anyone ever tried something like this? If so do you have a solution for this? The agar is poured by hand so getting it much thinner than 1 mm would be difficult.


Sincerely,

Claire

--------------------------------------------------------------------------------
Claire M. Brown, PhD
McGill University
Life Sciences Complex Imaging Facility Director

ATOM RSS1 RSS2

LISTS.UMN.EDU