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Targeted label‐free quantification of interleukin‐8 in PMA‐activated U937 cell secretome by nanoLC‐ESI‐MS/MS‐sSRM
Authors:Pelin Esma Emirbayer  Kerstin F. Gerer  Stefanie Hoyer  Monika Pischetsrieder
Affiliation:1. Food Chemistry Unit, Department of Chemistry and Pharmacy, Emil Fischer Center, Friedrich‐Alexander Universit?t Erlangen‐Nürnberg (FAU), Erlangen, Germany;2. Department of Dermatology, Forschungscampus, Universit?tsklinikum Erlangen, Erlangen, Germany;3. Department of Genetics, Friedrich‐Alexander‐Universit?t Erlangen‐Nürnberg (FAU), Erlangen, Germany
Abstract:Monocytes are a part of the innate immune system. Their differentiation into macrophages changes their cellular proteome and secretome. Particularly secretome components such as cytokines are crucial for immune response and inflammation in many diseases. Differentiation of human lymphoma cell line U937 can be triggered by phorbol 12‐myristate 13‐acetate (PMA). Screening of the cytokine release in U937 upon PMA stimulation by cytometric bead array almost exclusively showed interleukin‐8 (IL‐8). Next, a label‐free nanoLC‐ESI‐MS/MS‐sSRM method for quantification of IL‐8 in the cell secretome was established and applied to monitor the time kinetics of PMA treatment in different concentrations. Targeted secretome analysis was achieved by scheduled SRM‐MS using one proteotypic peptide as precursor ion and four mass transitions. Label‐free quantification was performed by external calibration using IL‐8 standard. Validation results indicated that the method was suited for the quantification of IL‐8 in the secretome. The maximal IL‐8 release of 62.4 ng/mL was observed after incubating cells treated by 50 ng/mL PMA for 48 h. The method can now be used for quantification of IL‐8 release from different cells under various conditions. Furthermore, it can be easily expanded to other secreted proteins detected by untargeted screening methods.
Keywords:Cytokine quantification  Interleukin‐8  Scheduled reaction monitoring  Secretome  Targeted mass spectrometry
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