Allergy Clinical Trial
Official title:
Individual Risk Factors for Enhanced Inflammation to Arthroplasty Wear Particles: Analysis of Cytokine Polymorphisms and in Vitro Cytokine Production to Wear Particles (Ceramic, Metal, XPE)
Assessment of cytokine polymorphisms in 100 patients with aseptic complications to
arthroplasty as compared to 100 symptom-free arthroplasty patients.
In selected patients additional in-vitro cytokine release assay with peripheral blood
mononuclear cells (PBMC) stimulated with different wear particles.
A cytokine polymorphism analysis in 100 individuals with aseptic implant intolerance reaction
(patients of the implant allergy special ambulance) and in 100 asymptomatic patients with
implanted endoprostheses will be done. Furthermore, supplementary clinical data (such as type
of implant, hospital stay, discomfort), questionnaire-based history and a clinical score
(WOMAC score) are recorded. In the subgroup analysis in 10 patients of implant patients with
complaints with special found cytokine polymorphisms and 10 implant patients without problems
the cytokine response to particles in vitro will assessed.
Test parameters:
1. total collective:
the DNA of cryopreserved blood sample will be isolated. By polymerase chain reaction,
four different known polymorphisms will be analyzed, three IL-1B genes (IL-1B-3954
IL-1B-31, and IL-1B-511), and a IL-1ß receptor antagonist gene (IL -1-RN, intron 2
VNTR). Molecular analysis includes DNA isolation, polymerase chain reactions (PCR) and
gel electrophoresis.
2. Subgroup analysis:
Peripheral blood cells will be isolated from 10 implant patients with complications and 10
symptom-free persons and stimulated in cell culture with control stimuli, the IL-1ß-inducer
lipopolysaccharide (LPS) and ceramic particles (BIOLOX delta)*, CoCrMo particles and
XPE-particles** cultured separately or in combination. The secretion of IL-1ß and selected
proinflammatory cytokines will be measured. The methods include cell isolation by density
centrifugation and analysis of cell culture supernatants by a multiplex cytokine measurement
assay by flow cytometry.
* Supplied CeramTec
** Generated and processed by the Working Group of the cooperation partner Prof. R. Bader
(University Hospital Rostock) in special carrier system for cell culture stimulation approach
;
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