Methods

Primary TKA patients were randomized into either a control or cryoneurolysis treatment group. Both followed the same preoperative, intraoperative, and postoperative pain management protocol, except the treatment group had cryoneurolysis of their superficial genicular nerves 3–7 days prior to surgery. All patients were prescribed 40 narcotic pills at discharge and pills were counted at 72 hours and at 2,6, and 12 weeks postoperatively. The primary endpoint was daily morphine equivalent (DME) based on pill count and secondary endpoints were changes in pain and Knee Injury and Osteoarthritis Outcome Score for Joint Replacement (KOOS, Jr.) scores.

Methods

After Institutional Review Board (IRB) approval, 50 patients were enrolled in the study into two cohorts. 25 patients presented with a painful TKA and 25 patients had a painful native knee with primary osteoarthritis (OA). Synovial fluid was obtained from each patient's affected knee. Appropriate lab and culture data was also obtained from the painful TKA group. An ELISA was used to determine GSN levels and the groups were compared. Two tailed Student's t tests were used to compare means while Pearson's Correlation Coefficient and linear regression analyses were used to determine association between laboratory findings and GSN levels.

METHODS

IRB approval was obtained prior to our study. We have analyzed 19 control (asymptomatic MoM THR patients > 6 years after surgery) and 19 disease (revised MoM THR for high metal ions and ALTR). The 38 sample intensity files were subject to sample Quality Control (QC) using Contrast QC (< 0.4) with an Affymetrix Genotyping Console. The resulting 38 sample files with genotype calls were loaded and further analyzed using the Association Workflow in Partek Genomics Suite 6.6 (Partek, Missouri). Hardy-Weinberg equilibrium test was performed on the single nucleotide polymorphism (SNP) level. The difference between the observed and expected frequencies of each allele at each locus were tested by Fisher's exact test and χ2 test. To get the working SNP list, two filters were used: (1) a SNP no-call rate should be less than 5%, and (2) minor allele frequency of a SNP should be greater than 5%.

After filtering, association analysis of the SNPS with disease was done using Chi² Test. In this study, χ² statistic was used to assess the difference in allele frequencies between the control and disease samples. The value of χ2 statistic, degrees of freedom, and the associated p-value for each SNP were calculated. Dot Plot was used to visualize the genotypes of all samples.

To measure the non-random association of alleles at different loci, Linkage Disequilibrium analysis was performed using the neighborhood size of 20 and statistic r². The resulting correlations show the value of r² for SNPs. The r² = 1 means that two SNPs are tightly associated.