Features of TAP-independent MHC class I ligands revealed by quantitative mass spectrometry.

6533b85efe1ef96bd12c08f2

RESEARCH PRODUCT

Features of TAP-independent MHC class I ligands revealed by quantitative mass spectrometry.

Andreas O. Weinzierl Hans-georg Rammensee Stefan Stevanovic Peter Van Endert Peter Van Endert Nina Hillen Hansjörg Schild Despina Rudolf Stefan Tenzer

subject

Proteasome Endopeptidase Complex Immunology Antigen presentation Epitopes T-Lymphocyte Gene Expression Human leukocyte antigen Cysteine Proteinase Inhibitors Protein Sorting Signals Major histocompatibility complex Cell Line Antigen ATP Binding Cassette Transporter Subfamily B Member 3 HLA Antigens Tandem Mass Spectrometry MHC class I HLA-A2 Antigen Immunology and Allergy Humans Amino Acid Sequence ATP Binding Cassette Transporter Subfamily B Member 2 Antigen Presentation biology HLA-A Antigens Antigen processing Histocompatibility Antigens Class I Proteins Transporter associated with antigen processing MHC restriction Molecular biology Peptide Fragments Cell biology HLA-B Antigens Isotope Labeling biology.protein ATP-Binding Cassette Transporters Proteasome Inhibitors Gene Deletion Protein Binding

description

TAP is responsible for transferring cytosolic peptides into the ER, where they can be loaded onto MHC molecules. Deletion of TAP results in a drastic reduction of MHC class I surface expression and alters the presented peptide pattern. This key molecule in antigen processing is tackled by several viruses and lost in some tumors, rendering the altered cells less vulnerable to T cell-based immune surveillance. Using the TAP-deficient cell line LCL721.174 and its TAP-expressing progenitor cell line LCL721.45, we identified and quantified more than 160 HLA ligands, 50 of which were presented TAP-independently. Peptides which were predominantly presented on the TAP-deficient LCL721.174 cell line had a decreased MHC binding affinity according to their SYFPEITHI and BIMAS score. About half of the identified TAP-independently presented peptides were not derived from signal sequences and may partly be generated by the proteasome. Furthermore, we have excluded the possibility that differences in HLA ligand presentation between LCL721.45 and LCL721.174 were due to varying expression of the source proteins or due to changes in the antigen loading complex. Features of peptides presented independently of TAP as well as proteasomal contribution to their generation provide an insight into basic immunological mechanisms.

year	journal	country	edition	language
2008-04-29	European journal of immunology

10.1002/eji.200838136 https://pubmed.ncbi.nlm.nih.gov/18446792