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- W3047420265 abstract "L-asparaginase (L-ASNase) is an important bacterial enzyme used as a biopharmaceutical to treat acute lymphoblastic leukemia (ALL). Side effects of L–ASNase therapy have been counteracted by polyethylene glycol (PEG)-modification of L-ASNase; however, immunogenicity of PEG has been observed in patients. Here we explore L-ASNase glycosylation as a biological alternative to the PEGylation industrial process. In our results, a recombinant Erwinase expressed in the Glycoswitch® Pichia pastoris strain occurred in three extracellular and glycosylated active variants; two tetrameric forms: Erw240 (240 kDa) and Erw160 (160 kDa), with a specific activity of 15.71 and 302.02 U mg−1 respectively; and one monomeric version: Erw40 (40 kDa), with a specific activity of 48.45 U mg−1. The lighter tetramer and the monomer showed a catalytic efficiency of 7.7 × 105 and 1.05 × 106 M−1 s−1 respectively, while the heaviest form considerably lost its activity. Mass spectrometry analysis determined that Erw40 and Erw160 tetramer were N-glycosylated at Asn170 mostly with GlcNAc2Man7 N-glycans. These glycosylation sites are part of a predicted immunogenic T-cell epitope related to ASNase allergy in ALL patients. ELISA assay showed a significant reduction of antibody recognition of the glycosylated Erwinase suggesting that the glycans had a cloaking effect against antibodies. The new L-ASNase versions reported here could provide an alternative for the treatment of ALL." @default.
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- W3047420265 date "2020-11-01" @default.
- W3047420265 modified "2023-10-18" @default.
- W3047420265 title "Glycosylation of Erwinase results in active protein less recognized by antibodies" @default.
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- W3047420265 doi "https://doi.org/10.1016/j.bej.2020.107750" @default.
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