Detailed studies on the effects of TAMs on tumour cells will furt

Detailed studies on the effects of TAMs on tumour cells will further help in understanding the mechanisms of action of TAMs. Together, these would aid in the development of strategies to manipulate and re-educate TAMs to mount anti-tumour responses. All blood samples and procedures in this study were approved by the Domain Specific Review Board (DSRB), National Healthcare Group, Singapore (Reference code: 08-352E). Informed consent was given in accordance with the Declaration of Helsinki. Peripheral blood mononuclear cells were isolated from buffy coats (National University Hospital Blood Donation Center, Singapore) by Ficoll-Hypaque

density gradient centrifugation; monocytes were positively selected using CD14 Microbeads (Miltenyi). Purity and viability Selleckchem Ganetespib of monocytes obtained were 98.0±1.7 and 98.7±0.8%, respectively, assessed by flow cytometry. Dasatinib Human colorectal cancer cell lines (HT29, SW620, LS174T, authenticated

by CellBank, Australia), prostate cancer cell lines (Du145, DuCap and LnCap), ovarian cell line (ES2) and breast cancer cell lines (MCF7 and SKBR3) were used to generate MCTSs by the liquid overlay method: 104 tumour cells and 104 monocytes (co-culture spheroids) or only 104 tumour cells (tumour spheroids) or 104 monocyte (monocyte culture) were seeded in 200 μL medium in 96-well coated with 0.8% w/v Agar Noble (Difco, BD). Cells were cultured in IMDM (Hyclone) with 5% human serum (HS; Innovative Research) at 37°C with 5% CO2 for 8 days. Culture medium was changed on day 4, when half the medium was replaced with fresh medium. Monocytes were treated with 100 ng/mL M-CSF for 8 days to generate macrophages, or 100 ng/mL GM-CSF and 25 ng/mL IL-4 for 8 days to generate DCs. Dead cells were excluded using live/dead fixable dead cell stain (Invitrogen).

For intracellular labelling, manufacturer’s instructions for the fixation/permeabilisation kit (BD Biosciences) were followed. Antibodies: EpCAM (9C4), CD68 (Y1/82A), CD14 (61D3), HLA-DR (LN3), CD40 (5C3), CD80 (2D10), CD86 (IT2.2), CD54 (HA58), CD3 (III471), Casein kinase 1 CD25 (BC96), IFN-γ (4S.B3), IL-4 (8D48), IL-17A (64DEC17), FoxP3 (PCH101) and their respective isotypes were from eBioscience. CD74 (LN2) was from BioLegend. Data were analysed using FlowJo (Tree Star, Ashland, OR, USA). Co-culture MCTSs were dissociated with Accumex (Innovative Cell Technologies) and labelled with anti-EpCAM-FITC (tumour cells), anti-CD14-PE (macrophages) for sorting (FACSAriaII, BD). The percentage of TAMs in the co-culture spheroids after 8 days of culture was 7±2% (n=4). Tumour cells were sorted directly into Trizol-LS (Invitrogen). Chloroform (0.2 mL) was added per 1 mL Trizol-LS, mixed and centrifuged (12 000 rpm, 15 min, 4°C). The upper aqueous phase was extracted and an equal volume of 70% ethanol was added.

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