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Purification of erythropoietin from human plasma samples using an immunoaffinity well plate
Authors:J Mallorquí  E Llop  C de Bolòs  R Gutiérrez-Gallego  J Segura  JA Pascual
Institution:1. Bioanalysis Group, Neuropsychopharmacology Research Program, IMIM-Hospital del Mar. PRBB, Barcelona, Spain;2. Department of Experimental and Health Sciences, Pompeu Fabra University, PRBB, Barcelona, Spain;3. Gastric Carcinogenesis Group, Cancer Research Program, IMIM-Hospital del Mar. PRBB, Barcelona, Spain
Abstract:A method is described to isolate human erythropoietin (hEPO) from plasma using an EPO-specific immunoaffinity micro well plate (IAP). The operating conditions of the method (binding, blocking and elution) were optimised to avoid isoform discrimination and cross-contamination with other glycoproteins. The overall hEPO recovery was ca. 56% and significant clean-up for plasmatic hEPO was achieved. Polyvinylpyrrolidone (PVP) was used as a blocking reagent and elution took place at pH 11.0. Under these conditions all isoforms from recombinant human EPOs (rhEPOs) and analogues were uniformly recovered guaranteeing lack of discrimination. The resulting procedure allowed isolating erythropoietin from plasma in conditions amenable to hEPO analysis by other techniques such as SDS-PAGE or IEF. Moreover, avoiding contamination with other glycosylated material allowed the identification in human plasma samples of the non-human N-glycolyl-neuraminic acid (Neu5Gc) using HPLC-FLD. Neu5Gc is present as 1–2% of the sialic acid content in rhEPO so this approach could be used to unequivocally detect abuse of rhEPOs or analogues as part of the doping control.
Keywords:hEPO  human erythropoietin  NESP  novel erythropoiesis stimulating protein  rhEPO  recombinant human EPO  CERA  Continuous Erythropoietin Receptor Activator  uhEPO  urinary human EPO  Neu5Gc  N-glycolyl-neuraminic acid  IAP  immunoaffinity plate  IAC  immunoaffinity column  ELISA  enzyme linked immunosorbent assay  mAb  monoclonal antibody  HPLC-FLD  high performance liquid chromatography with fluorescence detection  HRP  horseradish peroxidase  SDS-PAGE  sodium dodecyl sulphate polyacrylamide gel electrophoresis  IEF  isoelectric focusing  BSA  bovine serum albumin  PVP  polyvinylpyrrolidone  TFA  trifluoroacetic acid  WADA  World Anti-Doping Agency
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