Methods for determining the spatial distribution of oxidation in ultra-high molecular-weight polyethylene prostheses

Oxidative degradation is a well-known problem for UHMWPE used in prostheses. The aim of the present study has been to find suitable techniques to study the spatial distribution of this oxidation in 8 retrieved acetabular cups. The techniques used were visual examination using an optical microscope and computer scanner, FTIR mapping, imaging chemiluminescence, and staining with SO₂ and HCl. The staining technique is based on a previous study which showed that by treating oxidized UHMWPE with SO₂ followed by heat treatment, the hydroperoxides present in the sample react with the SO₂ and discolor the sample. The intensity of this discoloring is, at low levels of oxidation, proportional to the amount of hydroperoxides and accordingly to the level of the oxidation. The same study also showed that staining a sample with hot HCl resulted in a brown discoloration which was proportional to the amount of carbonyls. It was found that the staining techniques do not give as much information about the chemical and physical changes in the material as FTIR mapping but have a great advantage in better spatial resolution of the oxidation and are also much quicker and easier to use. Imaging chemiluminescence turned out not to be a suitable method to use, compared to the other two, since it gives less information and is more difficult to interpret.When interpreting the results from the different techniques used, it was found that all cups showed the typical oxidation behavior of gamma sterilized UHMWPE. All cups but one showed substantial wear of the articulating surface but very little backside wear. Examination of the oxidation and whitening profile suggests that at least some of the oxidation must have occurred in vivo.     

Oxidation of ultra high molecular weight polyethylene (UHMWPE) part 3: Decomposition of hydroperoxides with SO2 and its effect on the chemiluminescence signal

Samples of slightly oxidised UHMWPE were treated with SO₂ to decompose hydroperoxides prior to chemiluminescence measurements. It was found that the effect was quite substantial, but it was not just due to the elimination of hydroperoxides; a stabilising effect was also manifested. This effect increased with an increasing concentration of hydroperoxides in the samples. The stabilising effect could not be seen in fresh samples or when the hydroperoxides were decomposed by heating the sample in nitrogen. In addition, a stabilising effect was also observed for samples in which the hydroperoxides were reduced by DMS. It was concluded that the stabilisation was due to the formation of H₂SO₄ in the case of SO₂ and DMSO in the case of DMS. Both these substances can act as stabilisers against oxidative degradation of polymers and were evenly distributed in the sample films after the reaction with the hydroperoxides.     

Production of monoclonal antibodies against hop-derived (Humulus lupulus L.) prenylflavonoids and the development of immunoassays

Monoclonal antibodies against the hop-derived prenylated chalcone xanthohumol (X) and the prenylated flavonoids isoxanthohumol (IX) and 8-prenylnaringenin (8-PN) were developed. Carboxylic acid haptens of X, IX and 8-PN were synthesized by linking a spacer to their C4′-OH group followed by subsequent coupling to bovine serum albumin (BSA) to form conjugates that were employed as immunogens in BALB/c mice to raise antibodies. The monoclonal antibodies that were secreted from the established hybridoma cell lines proved, in cross-reactivity studies, to possess highly specific binding capacities in an optimized competitive indirect ELISA. The immunoassays make use of immunogen-coated microtiterplates and a peroxidase-labeled anti-mouse IgG₁ secondary antibody with ABTS as a chromogenic substrate. For X the IC₅₀ value derived from the standard curve was 62.91 ng mL⁻¹, and for both IX and 8-PN 37.15 ng mL⁻¹. The assay was validated for the quantitative analysis of X, IX and 8-PN in urine and serum. A simple sample pretreatment procedure using a diethyl ether extraction was optimized and the recoveries and matrix effects were assessed. The validity of the established assay was tested and mean inter- and intra-assay variations in urine were 2.32% and 1.91%, respectively for X, 6.24% and 2.39%, respectively for IX and 7.18% and 0.74%, respectively for 8-PN. In serum, the mean inter- and intra-assay variations were 8.90% and 1.37%, respectively for X, 6.13% and 1.57%, respectively for IX and 6.13% and 2.43%, respectively for 8-PN. Furthermore, the method demonstrated excellent accuracy and significant correlation with measurements by an established and validated HPLC-MS method.     

Thermodynamic and spectroscopic study of the interaction of Cu(II), Ni(II), Zn(II) and Ca(II) ions with 2-amino-N-(2-oxo-2-(2-(pyridin-2-yl)ethyl amino)ethyl)acetamide,a pseudo-mimic of human serum albumin

The protonation equilibria of 2-amino-N-(2-oxo-2-(2-(pyridin-2-yl)ethyl amino)ethyl)acetamide ([H₂(556)–N]) and the complexation of this ligand with Cu(II) Ca(II), Zn(II) and Ni(II) have been studied by glass electrode potentiometry and UV–visible spectrophotometry. From pH ∼2.00–11.00, five models for Cu(II) with the following complexes; MLH, ML, MLH₋₁, MLH₋₂ and MLH₋₃ were generated and observed to describe the experimental data equally well as far as the statistical criteria were concerned. The MLH₋₂ complex predominates at physiological pH in all five models, while the MLH₋₁ complex species exists only at low concentration in two models. The coordination in the MLH₋₂ complex suggested the involvement of one amino, two deprotonated peptides and one pyridyl nitrogen atoms. Molecular mechanics (MM) calculations confirmed the MLH₋₂ complex as the most stable species. Speciation calculations, using a blood plasma model, predicted that the Cu(II)–[H₂(556)–N] complex is able to mobilize Cu(II). Octanol/water partition of CuLH₋₂ showed that 30% of the complex went into the octanol phase, hence promoting percutaneous absorption of copper. The complex is a poor mimic of native copper–zinc superoxide dismutase.