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Pre-Clinical Division, Faculty of Veterinary Medicine and Conway Institute, University College Dublin, UK1
Federal Research Centre for Virus Diseases of Animals, PO Box 1149, 72001 Tübingen, Germany2
Department of Pathology, Central Veterinary Laboratory, Abbottstown, UK3
Author for correspondence: Martin H. Groschup. Fax +49 7071 967 105. e-mail martin.groschup{at}tue.bfav.de
Different strains of transmissible spongiform encephalopathies in humans and rodent models are associated with the accumulation of PrPSc of distinct molecular characteristics. These characteristics include glycosylation profiles, fragment sizes and long-term resistance of PrPSc to proteinase K. The first objective of this study was to determine the applicability of these criteria to characterize and differentiate sheep scrapie PrPSc and bovine spongiform encephalopathy (BSE) PrPSc. PrPSc in sheep scrapie samples from Ireland had clearly distinct molecular characteristics to PrPSc in cattle BSE samples using a monoclonal antibody (MAb P4) directed to position 89104 of ovine PrP using either brain homogenates or semi-purified scrapie-associated fibrils. Similar glycoprofiles were found when analysing scrapie PrPSc in six different CNS regions (thoracic spinal cord, thalamus, basal ganglia, mediobasal hypothalamus, medulla oblongata and cortex). While the long-term resistance results using a different monoclonal antibody (raised to ruminant PrP positions 145163; MAb L42) were similar to the results obtained with MAb P4, different glycotyping results were obtained. Given the variation in glycosylation patterns using different antibodies, we conclude that standardization of methodology and antibodies is crucial to the applicability of molecular analysis of ruminant BSE and scrapie samples.
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