The monocyte-derived dendritic cell (MoDC) assay – an in vitro assay for testing the immunogenicity of cellular therapies

Make PBMCs using preferred method from whole blood

Take whole PBMCs and enrich for CD14+ cells using magnetic activated cell sorting (MACS) with CD14+ microbeads

Count monocytes, then seed in a 96 well plate at 150,000 cells/well in 200 ul RPMI + 10% P/S + 5% human AB serum (HAB) + 50 ng/ml rhIL-4 and 50 ng/ml rhGM-CSF (day 0)

Incubate in 3^ooC incubator for 7 days refreshing half media on day 3 and 6

Each media refresh should be done with double concentration IL-4 and GM-CSF to account for half media change: remove 100 ul media, add 100 ul RPMI + 10% P/S + 5% HAB + 100 ng/ml rhIL-4 and 100 ng/ml rhGM-CSF

Day 6 media change, plus 100 ng/ml LPS for activation : remove 100 ul media, add 100 ul RPMI + 10% P/S + 5% HAB + 100 ng/ml rhIL-4 and 100 ng/ml rhGM-CSF + 200 ng/ml LPS

Optional : collect monocytes (day 0), immature moDCs (day 6) and mature moDCs (day 7) to check purity of MACS enrichment by flow cytometry

Monocytes: CD14+

Immature DCs: CD14-, CD80+, CD86+, HLA-ABC+, HLA-DR+

Mature DCs: CD14-, CD80+, CD86+, HLA-ABC+, HLA-DR+, CD83+

Using the CD14- population, enrich for T cells using MACS with a PanT negative selection kit

If specific T cell population is required, perform MACS or FACS (fluorescence activated cell sorting) for required population

Optional : collect PanT to check purity of MACS enrichment by flow cytometry

Stain T cells with proliferation dye as per preferred protocol

Count then freeze the stained-T cells in FBS + 10% DMSO for the duration of the monocyte-DC differentiation

Prepare your "cells of interest" (COI) ready to have enough for 150,000 cells per well on day 7

Thaw proliferation dyed-T cells as per preferred protocol

Remove all media from moDCs and wash once with PBS (moDCs are adherent but aspirate gently to avoid disturbing cells)

Experimental wells:

Seed 150,000 autologous T cells per well in 150 ul RPMI + 10% P/S + 5% HAB

Seed 150,000 COI per well with 150 ul media specific to cells of interest (+ ROCKi if required)

Final: 1:1:1 ratio of moDC:T cell:COI in 300 ul of 50:50 media RPMI media: COI media

Note : optimisation will be required to ensure both cell types survive and proliferate as expected in the 1:1 media mix

Positive control wells:

(1) Allogeneic Tcell-moDC C

Seed 150,000 allogeneic T cells into moDC wells in 150 ul RPMI + 10% P/S + 5% HAB

Add 150 ul media specific to cells of interest

(2) Polyclonally activated T cells

Seed 150,000 T cells into an empty well (no moDC) in 150 ul RPMI + 10% P/S + 5% HAB

Add activation beads at recommended ratio in 150 ul media specific to cells of interest

Incubate co-culture for 5 days, refreshing half media every 48 hours (day 2 and day 4)

Each change: remove 150 ul media and add 150 ul prepared 1:1 media

For cytokine assays:

Collect 150 ul supernatant per well into a v-bottom 96 well plate

Centrifuge supernatants plate 1500 g x 10 minutes then re-collect supernatants avoiding any pellet/debris that have collected

Freeze supernatants at -80^oC until use.

Perform ELISA or luminex cytokine assays including IFNg and TNFa as readouts of immunogenicity.

For flow cytometry:

Collect remaining supernatants containing non-adherent T cells by agitating gently, washing the well 1-2 times with the supernatant.

Note : moDCs are adherent so will not be collected, consider that COI may be adherent or non-adherent (it is ok if some are collected as they will be gated out during flow cytometry).

Perform flow cytometry immediately, including a minimum panel of: CD3, CD4 and CD8 (T cell markers), CD25 (activated T cell marker) and live/dead stain.

Note e: cells are already pre-stained with proliferation dye

Activated T cells (CD25+, proliferation dye low/negative) are used as readout of immunogenicity of COI