Posted by Leoncio Vergara-2 on
URL: http://confocal-microscopy-list.275.s1.nabble.com/detecting-apoptosis-in-one-cell-type-in-coculture-tp7584201p7584211.html

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Thanks for the responses so far. I am getting some interesting leads to
follow but I am realizing the solution may not be straightforward. I have
quite a bit of experience in several forms of optical microscopy but I am
new apoptosis. I am quite excited with my involvement in image based high
throughput screening for cancer research.

We are trying to develop an image based assay moving from flow cytometry to
imaging. Our first approach was to modify the Flow assay already in place
for use in imaging and it was then that we found this new set of problems.
Our goal is to setup an assay on fixed cells in large format multiwell
plates. In the process we plan to do live cell imaging experiments our
final goal is to setup a drug screening protocol.

I was hoping to find a marker ( or combination of markers) to quantify cell
toxicity which can be loaded into cells and then washed before adding T
cells to the cultures. Non wash assays like CellEvent and Annexin V have
the problem of interference from the Tcells. An option is to label the
Tcells to separate them on analysis, but at high seeding ratios the Tcells
cover most of the well area and at the low magnifications (and hence low
NA) used for screening we don't have enough z-discrimination to separate
the Tcells on top from the tumor cells underneath. We have 4 channels
available, the classical DAPI, FITC, TRITC and Cy5 combination (405,
488,561 and 640 excitations).

One of the goals is to work with multiple cell lines (more than a dozen) so
any method based on expressing FP based indicators would make the assay too
complicated.

Leoncio



On Thu, Sep 10, 2015 at 2:41 AM, Markus Rehm <[hidden email]> wrote: