K. Christian Schuster

Development of a Fast and Reliable Method for the Assessment of Microbial Colonization and Growth on Textiles by DNA Quantification

There is a lack of relevant methods to assess the colonization of textiles by skin bacteria because present methods are mainly culture-based procedures. Therefore, the goal of this study was to develop a fast and sensitive culture-independent procedure for the quantification of microbial colonization and growth on textiles. We have established a suitable protocol to use DNA quantification as a reliable method for in vitroand in vivoinvestigations of textiles. For DNA extraction, a two-step procedure comprising treatment of the textile with a solution containing Triton X-100 and lysozyme for 1 h and a successive treatment by SDS and proteinase K for 2 h turned out to be most efficient. DNA extracted from textiles and fabrics was than quantified with the highly sensitive PicoGreen fluorescent dye. In vitrochallenge tests demonstrated a strong correlation between numbers of bacteria on textiles and amount of DNA extracted from textiles. Therefore, this method was used to compare different materials after in vivotrials for assessment of their susceptibility for microbial colonization and growth.

A morphological interpretation of water chemical exchange and mobility in cellulose materials derived from proton NMR T2 relaxation

Proton T2 relaxation times of water in cellulosic fibres have been interpreted using a 3-term average model. Motional and chemical exchange contributions to relaxation show opposing temperature behaviour, enabling the use of Arrhenius analysis to determine proton exchange rates and water rotational correlation times. Both parameters vary dramatically with extent of hydration, with chemical exchange dominating relaxation at saturated water contents. Interpretations are based on a morphological model with two types of accessible cellulose, at void surfaces and internally within the cellulose phase. In native cellulose fibres, the presence of crystalline fibrils with low internal accessibility leads to rapid proton exchange at low moisture contents. Regenerated cellulose fibres typically have lower crystallinity and higher internal accessibility, which results in slower exchange as result of migration of water between void and internal environments. Exchange behaviour in regenerated fibres is highly dependent on structural organisation, which depends on the manufacturing process.