Femoral neck impingement occurs clinically in total hip replacements (THR) when the acetabular liner articulates against the neck of a femoral stem prosthesis. This may occur Neck impingement testing per ASTM F2582-14 was carried out on four groups of artificially aged acetabular liners (per ASTM F2003-15) made from GUR 1020 UHMWPE which was re-melted and cross-linked at 7.5 Mrad. Group A (n=3) and B (n=3) consisted of 28mm diameter femoral heads articulating on 28mm ID × 44mm OD acetabular liners. Group C (n=3) and D (n=3) consisted of 40mm diameter femoral heads articulating on lipped 40mm ID × 56mm OD 10° face changing acetabular liners. All acetabular liners were tested in production equivalent shell-fixtures mounted at 0° initial inclination angle. Femoral stems were potted in resin to fit respective simulator test fixtures. Testing was conducted in bovine serum diluted to 18mg/mL protein content supplemented with sodium azide and EDTA. Groups A and C were tested on a Prosim; Groups B and D were tested on an AMTI. Physical examination and coordination measurement machine (CMM) analyses were conducted on all liners pre-test and at 0.2 million cycle intervals to monitor possible failure mechanisms. Testing was conducted for 1.0 million cycles or until failure. An Abaqus/Explicit model was created to investigate relative motions and contact areas resulting from initial impingement kinematics for each test group.Introduction
Method
Multiple sources have consistently reported oxidation indices less than 0.1 with Marathon® inserts implanted up to 10 years. Understanding effects of oxidation level on UHMWPE wear GUR 1050 UHMWPE acetabular inserts, re-melted and cross-linked at 5.0Mrad (Marathon®, DePuy Synthes Joint Reconstruction, Warsaw, IN), were artificially aged per ASTM F-2003 in a stainless steel chamber at 5 atm. oxygen pressure and 70°C. Samples were maintained at temperature for 9, 10.4 and 11 weeks. After aging was completed, Fourier Transform Infra-Red (FTIR) spectroscopy was employed on one insert from each time point to evaluate the induced oxidation as a result of artificial aging. Resulting induced BOI values measured by FTIR were 0.195, 0.528 and 1.184. UHMWPE inserts had an inner diameter of 28mm and an outer diameter of 48mm and were articulated against 28mm diameter M-Spec® metal femoral heads (DePuy Synthes Joint Reconstruction, Warsaw, IN). Testing was conducted on a 12-station AMTI ADL hip simulator (AMTI, Watertown, MA) with load soak controls per ISO 14242-1:2014(E) in bovine serum (18mg/mL total protein concentration) supplemented with 0.056% sodium azide (preservative) and 5.56mM EDTA (calcium stabilizer). The UHMWPE inserts were removed from the machine, cleaned, and gravimetric wear determined per ISO 14242-2:2000(E) every 0.5 million cycles (MCyc) for 4.0 MCyc total. A two-tailed student's t-test was used (variance determined by F-test results) to analyze differences in wear rates between the three test groups.INTRODUCTION
METHODS
Adolescent idiopathic scoliosis (AIS) is the most common paediatric spinal deformity, affecting about 3% of school-aged children worldwide. This disorder occurs in otherwise healthy children who bear no obvious deficiencies in the components of the spinal column itself. The cause of AIS is poorly understood, as is implied by the name. Lesions of the bony composition of the vertebrae, the vertebral endplates, the paraspinous muscles, or the neurological system each have been proposed to explain disease pathogenesis. Progress has been hampered by the absence of an obvious AIS animal model. Consequently we have used genetic studies in human populations to identify factors underlying AIS susceptibility. The complex inheritance and population frequency of AIS suggest that many genetic factors are involved in this disease. To search comprehensively for such factors we previously undertook the first genome-wide association study (GWAS) of AIS susceptibility in a cohort of 419 families in Texas, USA. We found that chromosome 3 SNPs in the proximity of the We tested more than 327 000 single-nucleotide polymorphisms (SNPs) across all human autosomes for association with disease.Introduction
Methods
