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Demonstration of a novel technique to quantitatively assess inflammatory mediators and cells in rat knee joints. | LitMetric

AI Article Synopsis

  • The inflammation in osteo- and rheumatoid arthritis is driven by various inflammatory mediators, particularly cytokines and prostaglandins, which contribute to pain, swelling, and joint damage.
  • A new technique for analyzing rat joint synovial fluid was developed, allowing for precise measurement of inflammatory mediators by infusing and withdrawing saline from the knee joint.
  • Results showed significant increases in pro-inflammatory cytokines, confirming the technique's effectiveness in studying arthritis and providing insights into the inflammation occurring directly within the joint.

Article Abstract

Background: The inflammation that accompanies the pain and swelling associated with osteo- and rheumatoid arthritis is mediated by complex interactions of inflammatory mediators. Cytokines play a pivotal role in orchestrating many of these processes, including inflammatory cell recruitment, adhesion and activation. In addition, prostaglandins are secreted into the synovial cavity and are involved in perpetuation of local inflammation, vasodilatation and vasoconstriction, and also with bone resorption. Pre-clinical models have been developed in order to correlate to the human disease and principle among these is the adjuvant-induced arthritis model in the rat.

Methods: We have developed a technique to quantitatively assess the contents of synovial fluid samples from rat joints. Two needles joined together are inserted into the knee joint of anaesthetised rats and connected to a Watson-Marlow perfusion pump. Sterile saline is infused and withdrawn at 100 microl min-1 until a 250 microl sample is collected.

Results: Our results demonstrate up to 125 fold increases in synovial IL1alpha and IL1beta concentrations, approximately 30 fold increases in levels of IL6 and IL10 and a 200-300 fold elevation in synovial concentrations of TNFalpha during FCA-induced experimental arthritis. Finally, this novel technique has demonstrated a dose-response relationship between FCA and the total cell counts of synovial perfusates.

Conclusion: In summary, this new technique provides a robust method for quantifying inflammatory mediators and cells from the synovial cavity itself, thereby detailing the inflammatory processes from within the capsule and excluding those processes occurring in other tissues surrounding the entire articulation.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC1919375PMC
http://dx.doi.org/10.1186/1476-9255-4-13DOI Listing

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