TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES

A Gordon; E Kiss-Toth; I Stockley; A Hamer; R Eastell; JM Wilkinson

doi:10.1302/0301-620X.88BSUPP_II.0880236a

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TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES

A Gordon
E Kiss-Toth
I Stockley
A Hamer
R Eastell
JM Wilkinson

TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES

Gordon A, Kiss-Toth E, Stockley I, Hamer A, Eastell R, Wilkinson J. TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES. Orthop Procs. 2006;88-B(SUPP_II):236-236. doi:10.1302/0301-620X.88BSUPP_II.0880236a

Gordon, A, et al. “TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES.” Orthopaedic Proceedings, vol. 88-B, no. SUPP_II, 2006, pp. 236-236., https://doi.org/10.1302/0301-620X.88BSUPP_II.0880236a

Gordon, A., Kiss-Toth, E., Stockley, I., Hamer, A., Eastell, R., & Wilkinson, J. (2006). TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES. Orthopaedic Proceedings, 88-B(SUPP_II), 236-236. https://doi.org/10.1302/0301-620X.88BSUPP_II.0880236a

Gordon, A., Kiss-Toth, E., Stockley, I., Hamer, A., Eastell, R. and Wilkinson, J. (2006) “TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES.” Orthopaedic Proceedings, 88-B(SUPP_II), pp. 236-236. Available at: https://doi.org/10.1302/0301-620X.88BSUPP_II.0880236a

Gordon, A, E Kiss-Toth, I Stockley, A Hamer, R Eastell, and JM Wilkinson. “TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES.” Orthopaedic Proceedings 88-B, no. SUPP_II (2006): 236-236. https://doi.org/10.1302/0301-620X.88BSUPP_II.0880236a

Gordon A, Kiss-Toth E, Stockley I, Hamer A, Eastell R, Wilkinson J. TNFα AND IL-1β CYTOKINE MRNA EXPRESSION IN POLYETHYLENE STIMULATED MACROPHAGES. Orthop Procs. 2006 May 1;88-B(SUPP_II):236-236. https://doi.org/10.1302/0301-620X.88BSUPP_II.0880236a

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Abstract

Cytokine mediated activation of osteoclasts can lead to peri-implant osteolysis and aseptic loosening. The aim of this study was to determine the IL-1β and TNFα mRNA cytokine expression profile of human macrophages when stimulated with polyethylene particles using relative quantitative real-time polymerase chain reaction (rqRT-PCR).

Human peripheral blood monocytes or human monocytes from the cell line THP-1 were used in this study. rqRT-PCR conditions were optimized by stimulating human macrophages with 200ng/ml lipopolysaccharide (LPS). The median CV% value for duplicate measures was 12.6 (range 4.5–54). Stimulation assays were performed using unfractionated endotoxin-free commercial polyethylene particles (median size 7μm); or fractionated particles (size range 0.1–1.2μm). Human macrophages were stimulated with high dose unfractionated polyethylene particles at 0, 3500 or 10500 mm³/cell or with fractionated polyethylene particles at 0 and 100mm³/cell at time points 0 and 3 hours. Low dose unfractionated polyethylene stimulation was performed on THP-1 cells at 0, 50, 100, 1000 and 10000 mm³/cell. In all experiments LPS stimulation was used as a positive control. RNA was extracted and rqRT-PCR was performed using standard techniques

High dose unfractionated polyethylene stimulation did not result in a significant difference in cytokine mRNA levels between groups. Using fractionated polyethylene, a small increase in IL-1β mRNA was identified (21% versus maximal stimulation using LPS). Low dose unfractionated polyethylene stimulation of THP-1 cells demonstrated dose dependent decreases in TNFα and IL-1β mRNA expression that was not due to inhibition of RNA extraction or a decrease of cell viability.

Endotoxin-free polyethylene particles do not appear to be a major stimulus for IL-1β and TNFα mRNA production as measured by rqRT-PCR. We did observe a small positive effect on IL-1β mRNA expression using a fractionated polyethylene stimulus. However it remains unclear whether this effect is due to fractionation of particles into the submicron range or is due to introduction of endotoxin during the filtration process.

Editoral Secretary Mr Peter Howard. Correspondence should be addressed to BHS at the Royal College of Surgeons, 35 - 43 Lincoln’s Inn Fields, London WC2A 3PN.