Killing Assay with different abs and dyes 11-17-11

2015-01-13

azim58 - Killing Assay with different abs and dyes 11-17-11


Splenocytes from Balb Ova immunized mice were mixed with Ova peptide
pulsed target cells (Balb 3T3 and Balb CRL 2116).

Outline of Process 11-18-11.pdf

For the most part, our standard protocols were followed.
11-18-11 We added IL-2 to the mixed cultures one day after starting them.
We added 1 uL 100 ug/mL rh-IL-2 to 20 mL culture.
11-20-11 I added IL-2 to the mixed cultures 3 days after starting them.
Added 3 uL 100 ug/mL rh-IL-2 to 30 mL culture (10 more mL of DMEM
sensitization media was added to the 20 mL culture which looked fairly
yellow).

Results from the killing assay from the splenocytes used immediately
Results 11-18-11

11-21-11
When we tried to purify our T cells with the Robosep after 4 days of
incubation, we only had about 100,000 cells which was not enough. We
hypothesize that there could have been several reasons that we lost so
many T cells. One reason is that there was a lot of clumping that was
hard to get rid of. The Robosep may not have purified the cells
appropriately because of this clumping. Another possible reason we did
not obtain good results may have to do with the age of the Robosep T cell
enrichment kit we used. We found a large number (maybe about 20) old T
cell enrichment kits from 2006 (5 years old), and we used some of these
kits. Due to the age of these kits they may no longer be effective.

The next time we do an experiment for these CTL assays, we will most
likely take the spleen from a normal mouse, use a fresh Robosep kit, and
then perform some flow cytometry with CD8, CD3, and CD4 antibodies to
make sure that we have purified killer T cells and not helper T cells or
any other types of cells.

We also plan to become better at identifying which cells are the T cells
in our mixed cultures. We plan to do this by finding out the diameter of
a T cell, taking some images of our cultures, and placing a black scale
bar on these images so that we can characterize the different types of
cells we are looking at.

The next time we plan to do an actual killing assay, we are considering
culturing the splenocytes by themselves and just adding IL-2 (instead of
culturing the splenocytes with target cells). This way most of the
splenocyte cells would be in suspension and may be easier to handle.

Some details from experiment

o Last part of "Inducing cytolytic activity in CTL precursors"
o Purification of T cells with Robosep

protocol
o peptide: 207/4*2*10^4
o no peptide: 309/4*2*10^4

o 25/4*2*10^4 = 125,000