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NACE–ESI-MS/MS method for separation and characterization of phosphorylation and acylation isomers of lipid A
Authors:Viktor Sándor  Balázs Viktor Berkics  Anikó Kilár  Béla Kocsis  Ferenc Kilár  Ágnes Dörnyei
Institution:1. Institute of Bioanalysis, Medical School and Szentágothai Research Centre, University of Pécs, Pécs, Hungary;2. Institute of Bioanalysis, Medical School and Szentágothai Research Centre, University of Pécs, Pécs, Hungary

Viktor Sándor and Balázs Viktor Berkics contributed equally to this work.;3. Department of Microbiology and Immunology, Medical School, University of Pécs, Pécs, Hungary;4. Department of Analytical and Environmental Chemistry, Faculty of Science, University of Pécs, Pécs, Hungary

Abstract:Lipid A represents a heterogeneous group of bacterial outer membrane phosphoglycolipids, which play a major role in the pathogenesis of Gram-negative sepsis. The number and position of phosphoryl and acyl groups in lipid A molecules are key structural determinants in their bioactivities. In this study, a NACE–ESI-MS/MS method was developed for the simultaneous analysis of lipid A isomers possessing a different degree of phosphorylation and acylation. Various C4’- and C1-monophosphorylated lipid A isobars, as well as acylation isomers, were baseline separated within 43 min in a separation medium of methanol/dichloromethane/triethylamine/acetic acid 60:40:1.08:0.36 (v/v/v/v). Both normal and reverse CE polarities could be applied for proper detection of the analytes owing to the combination of a suction effect caused by the nebulizer gas at the outlet end of the capillary and external pressure applied on the inlet vial. The separated lipid A species could be identified unequivocally by their characteristic fragmentation patterns through CID performed in both negative- and positive-ionization modes. The uniqueness of the NACE–ESI-MS/MS method lies in its simplicity and reliability for proving the phosphorylation isomerism (C1 or C4’) and acylation pattern of native lipid A species or those designed for therapeutic applications.
Keywords:Acylation isomerism  Lipid A  Nonaqueous CE–MS/MS  Normal and reverse polarity  Phosphorylation isomerism
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