Empty Class II Major Histocompatibility Complex Created by Peptide Photolysis Establishes the Role of DM in Peptide Association

Grotenbreg, Gijsbert M.; Nicholson, Megan; Fowler, Kevin; Wilbuer, Kathrin; Octavio, Leah; Yang, Maxine; Chakraborty, Arup K.; Ploegh, Hidde L.; Wucherpfennig, Kai W.

doi:10.1074/jbc.m702844200

Cited by 49 publications

(69 citation statements)

References 42 publications

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“…The k den found here correspond to t 1/2 values of 38-88 min (at 37 8C). These values (∼50 min on average) (Table S1) are similar to the only other t 1/2 (55 min) for an empty MHC of which we are aware; the latter was found for a human class II MHC, HLA-DR [calculated by Kevin Fowler from data in the work by Grotenbreg et al (32) using a model that differed considerably from the model used here]. Whether these unexpectedly long-lived empty MHCs found for one mouse class I and one human class II MHC are representative of MHC proteins in general remains to be seen.…”

Section: Discussionsupporting

confidence: 72%

“…The procedures used to measure k on for peptide binding to ostensibly empty MHC molecules have varied widely, and the reported association rate constants have spanned a wide range, roughly from 10 2 to 10 6 M −1 s −1 . Many reported values are at the low end of this range (21) (SI Text, R16 and R17), similar to those values found here and also for peptide binding to a class II MHC (32). When expressed in conventional units (M −1 s −1 ) rather than in the units (M −1 h −1 ) used in Table 1, we found 4,900 M −1 s −1 for OVA-K b and 217 M −1 s −1 for SIY-K b (Table 1).…”

Section: Discussionsupporting

confidence: 68%

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Promiscuous binding of extracellular peptides to cell surface class I MHC protein

Eisen

Hou

Shen

et al. 2012

Proc. Natl. Acad. Sci. U.S.A.

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Algorithms derived from measurements of short-peptide (8-10 mers) binding to class I MHC proteins suggest that the binding groove of a class I MHC protein, such as K b , can bind well over 1 million different peptides with significant affinity (<500 nM), a level of ligand-binding promiscuity approaching the level of heat shock protein binding of unfolded proteins. MHC proteins can, nevertheless, discriminate between similar peptides and bind many of them with high (nanomolar) affinity. Some insights into this high-promiscuity/high-affinity behavior and its impact on immunodominant peptides in T-cell responses to some infections and vaccination are suggested by results obtained here from testing a model developed to predict the number of cell surface peptide-MHC complexes that form on cells exposed to extracellular (exogenous) peptides.

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Section: Discussionsupporting

confidence: 72%

Section: Discussionsupporting

confidence: 68%

Promiscuous binding of extracellular peptides to cell surface class I MHC protein

Eisen

Hou

Shen

et al. 2012

Proc. Natl. Acad. Sci. U.S.A.

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“…During such peptide exchange, the MHCII-binding groove is temporarily empty, a state that is rather unstable and prone to aggregation (Germain and Rinker 1993;Rabinowitz et al 1998). DM prevents this aggregation and stabilizes empty MHCII molecules, keeping them in a peptide-receptive state (Kropshofer et al 1997;Grotenbreg et al 2007;Anders et al 2011). This important DM-catalyzed editing process favors the generation of high-affinity pMHCII complexes and is facilitated by the acidic milieu in late endosomes.…”

Section: Endosomal Mhc Class II Processingmentioning

confidence: 99%

MHC Class II Antigen Presentation by Dendritic Cells Regulated through Endosomal Sorting

Broeke

Wubbolts

Stoorvogel

2013

Cold Spring Harbor Perspectives in Biology

139

102

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For the initiation of adaptive immune responses, dendritic cells present antigenic peptides in association with major histocompatibility complex class II (MHCII) to naïve CD4 þ T lymphocytes. In this review, we discuss how antigen presentation is regulated through intracellular processing and trafficking of MHCII. Newly synthesized MHCII is chaperoned by the invariant chain to endosomes, where peptides from endocytosed pathogens can bind. In nonactivated dendritic cells, peptide-loaded MHCII is ubiquitinated and consequently sorted by the ESCRT machinery to intraluminal vesicles of multivesicular bodies, ultimately leading to lysosomal degradation. Ubiquitination of newly synthesized MHCII is blocked when dendritic cells are activated, now allowing its transfer to the cell surface. This mode of regulation for MHCII is a prime example of how molecular processing and sorting at multivesicular bodies can determine the expression of signaling receptors at the plasma membrane.

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“…1). After UV irradiation, the peptide fragments are believed to be liberated from the complex (5)(6)(7)(8)12). The uncaged complex can be rescued from degradation when UV-mediated cleavage is performed in the presence of a ligand capable of stabilizing the MHC molecule (Fig.…”

Section: The Concept Of the Bead-based Peptide-mhc Binding Assay-mentioning

confidence: 99%

“…Cell-free biophysical methods that employ soluble complexes purified to homogeneity have the advantage of directly measuring the molecular interaction between the peptide and MHC without the confounding effects of simultaneous expression of multiple MHC variants in a cellular context. Limitations on the expeditious and high throughput generation of collections of recombinantly produced pMHC products have largely been resolved with the introduction of conditional ligands for class I human leukocyte antigens (HLAs), (5-7) murine MHC, (5, 8 -11), and class II MHC molecules (12) and have been exploited for an ELISA-based MHC stability assay (6,13). Nevertheless, methods that employ cell lines defective in antigen presentation, where the exogenous addition of peptide can measurably restore MHC surface expression, such as the murine RMA-S (14,15) or human T2 lines transfected with an MHC of choice (16), remain unceasingly popular.…”

mentioning

confidence: 99%

Stability Screening of Arrays of Major Histocompatibility Complexes on Combinatorially Encoded Flow Cytometry Beads

Chew

Chang

et al. 2011

Journal of Biological Chemistry

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The binding and stabilization capacity of potential T cell epitopes to class I MHC molecules form the basis for their immunogenicity and provide fundamental insight into factors that dictate cellular immune responses. We have developed a versatile high throughput cell-free method to measure MHC stability by capturing a variety of MHC products on the surface of streptavidin-coated particles followed by flow cytometry analysis. Arrays of peptide-MHC combinations, generated by exchanging conditional ligand-loaded MHC, could be probed in a single experiment, thus combining the molecular precision of biochemically purified MHCs with high content multiparametric flow cytometry-based assays. Semiquantitative determination of the peptide affinity for the restriction element could also be accomplished through competition experiments using this bead-based assay. Furthermore, the generated peptide-MHC reagents could directly be applied to antigen-specific CD8 ؉ T lymphocyte analysis. The combinatorial labeling of beads allowed straightforward identification by their unique fluorescent signatures and provided a convenient means for extended assay multiplexing.Class I MHC molecules are crucially tasked with presenting repertoires of peptides at the cell surface for inspection by CD8 ϩ T cells, thereby allowing the immune system to respond to degradation products of proteins that are indicative of exposure to infectious disease or cellular transformation. The rational design of vaccines and immunotherapeutics depends on the accurate identification and characterization of those peptide antigens capable of precipitating a robust immune response. Such efforts are confronted with both an overwhelming diversity of potentially immunogenic peptide sequences and the polymorphism of the MHC system whereby each allelic product has a distinct peptide-binding motif that dictates their interactions. This has led to the development of a myriad of assays to probe either the ability of peptide-MHC (pMHC) 4 molecules to stimulate a specific population of T cells or ascertain the specificity and affinity of the peptide for a particular MHC variant (1-4). Cell-free biophysical methods that employ soluble complexes purified to homogeneity have the advantage of directly measuring the molecular interaction between the peptide and MHC without the confounding effects of simultaneous expression of multiple MHC variants in a cellular context. Limitations on the expeditious and high throughput generation of collections of recombinantly produced pMHC products have largely been resolved with the introduction of conditional ligands for class I human leukocyte antigens (HLAs), (5-7) murine MHC, (5, 8 -11), and class II MHC molecules (12) and have been exploited for an ELISA-based MHC stability assay (6, 13). Nevertheless, methods that employ cell lines defective in antigen presentation, where the exogenous addition of peptide can measurably restore MHC surface expression, such as the murine RMA-S (14, 15) or human T2 lines transfected with an MHC of choice...

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Empty Class II Major Histocompatibility Complex Created by Peptide Photolysis Establishes the Role of DM in Peptide Association

Cited by 49 publications

References 42 publications

Promiscuous binding of extracellular peptides to cell surface class I MHC protein

Promiscuous binding of extracellular peptides to cell surface class I MHC protein

MHC Class II Antigen Presentation by Dendritic Cells Regulated through Endosomal Sorting

Stability Screening of Arrays of Major Histocompatibility Complexes on Combinatorially Encoded Flow Cytometry Beads

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