Human Major Histocompatibility Complex (MHC) Class I Molecules with Disulfide Traps Secure Disease-related Antigenic Peptides and Exclude Competitor Peptides

Truscott, Steven M.; Wang, Xiaoli; Lybarger, Lonnie; Biddison, William E.; McBerry, Cortez; Martinko, John M.; Connolly, Jennifer M.; Linette, Gerald P.; Fremont, Daved H.; Hansen, Ted H.; Carreño, Beatriz M.

doi:10.1074/jbc.m709935200

Cited by 21 publications

(38 citation statements)

References 55 publications

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“…Bypassing the normal epitope processing requirements and increasing the rate of assembly of the class I molecule would be expected to increase significantly the steadystate level of presented peptide epitope at the cell surface, and hence increase the CD8 ϩ T cell response (22). A second potential advantage is that SCTs have increased cell surface stability, as compared with the equivalent wild-type MHC class I molecules (3,23). Recently, it has been shown that at equivalent levels of cell surface expression, antigenic peptide-MHC class I molecules with longer half-lives stimulate greater CD8 ϩ T cell responses (24).…”

Section: Discussionmentioning

confidence: 99%

“…1A), we have found that poorly immunogenic epitopes that have low binding affinities for class I fail to assemble efficiently as SCTs and are expressed poorly at the cell surface (K. Gould, unpublished results). However, recent ingenious improvements in SCT design by Hansen and colleagues, in particular the introduction of a disulfide trap to anchor the peptide epitope in the peptide binding groove of class I (23,28,29), offer the promise that even weakly binding peptide epitopes may be expressed as stable SCTs, and thereby improve their ability to stimulate CD8 ϩ T cell responses in vivo. This remains to be tested experimentally, but our results emphasize that such studies would be worthwhile.…”

Section: Discussionmentioning

confidence: 99%

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A Single-Chain H-2Db Molecule Presenting an Influenza Virus Nucleoprotein Epitope Shows Enhanced Ability at Stimulating CD8+ T Cell Responses In Vivo

Palmowski

Parker

Choudhuri

et al. 2009

The Journal of Immunology

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We have generated a construct encoding a single-chain H-2Db mouse MHC class I molecule in which an influenza virus nucleoprotein (NP) epitope, amino acid sequence ASNENMDAM, is fused to mouse β2-microglobulin and the Db H chain via flexible linker sequences. This single-chain trimer (SCT) was efficiently expressed at the cell surface independently of TAP and endogenous β2-microglobulin, and it was recognized directly and efficiently by specific T cells in vitro. A recombinant vaccinia virus encoding the Db NP SCT primed a CD8+ T cell response in C57BL/6 mice 4-fold greater than an equivalent virus expressing the NP epitope as a minigene, as shown by tetramer staining, whether or not the minigene was directed into the endoplasmic reticulum by a signal sequence. This response was functional as shown by in vivo lysis assays with peptide-pulsed target cells, and it was greatly expanded following secondary challenge in vivo with influenza virus. The SCT was also significantly more immunostimulatory for CD8+ cells than the NP minigene in adoptive transfer experiments using F5 TCR transgenic spleen cells, in which the magnitude of the T cell response was much greater. Our results extend previous DNA vaccination studies using SCTs, which demonstrated that such molecules are capable of generating functional CD8+ T cell responses. We have shown that class I SCTs are more immunogenic than even preprocessed Ag in the form of an epitope minigene, and they therefore should be considered for use when the generation of optimal CD8+ T cell responses is required.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

A Single-Chain H-2Db Molecule Presenting an Influenza Virus Nucleoprotein Epitope Shows Enhanced Ability at Stimulating CD8+ T Cell Responses In Vivo

Palmowski

Parker

Choudhuri

et al. 2009

The Journal of Immunology

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“…On the other hand, the concept of antibody-mediated delivery of pMHCI complexes to tumor cells as a therapeutic approach was never tested with unstimulated human PBMCs (19,25,28) although most likely these cells would constitute the primary source of CD8 þ effector T cells. It was unclear, however, whether naturally observed frequencies of CMV-specific effector CD8 þ T cells were sufficient to mediate significant tumor cell killing.…”

Section: Discussionmentioning

confidence: 99%

“…Importantly, a single virus-derived peptide is sufficient to attract a large number of T cells. The concept of mimicking a viral infection in cancer cells by targeting pMHCI complexes to their surface was proposed already several years ago (19,28). To date, various fusion molecules were designed for this purpose; basically all of them were produced as antibody fragments in bacteria (combined with refolding), followed in most cases by in vitro peptide-loading, chemical-conjugation, or T-cell group) or pMHCI-IgG constructs were administered at 50 mg/mouse ($2 mg/kg) beginning 6 hours after engraftment (day 0), after 24 hours (day 1), and then every 2 to 3 days.…”

Section: Discussionmentioning

confidence: 99%

“…The recombinant pMHCI complexes have been described previously as single-chain trimers (27)(28)(29). Recombinant pMHCI-IgG fusions were cloned into standard mammalian expression vectors (pcDNA3-derived; Life Technologies) and consist of viral peptide, first linker (sequence: (G 4 S) 3 ), b-2-microglobulin, second linker (sequence: (G 4 S) 4 ), a 1-3 domains of HLA-A Ã 0201, third linker (sequence: GS) followed by the antibody heavy chain.…”

Section: Cloning Transient Transfection and Protein Productionmentioning

confidence: 99%

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Committing Cytomegalovirus-Specific CD8 T Cells to Eliminate Tumor Cells by Bifunctional Major Histocompatibility Class I Antibody Fusion Molecules

Schmittnaegel¹,

Levitsky

Hoffmann³

et al. 2015

Cancer Immunology Research

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Tumor cells escape immune eradication through multiple mechanisms, including loss of antigenicity and local suppression of effector lymphocytes. To counteract these obstacles, we aimed to direct the unique cytomegalovirus (CMV)-specific immune surveillance against tumor cells. We developed a novel generation of fusion proteins composed of a tumor antigen-specific full immunoglobulin connected to a single major histocompatibility class I complex bearing a covalently linked virus-derived peptide (pMHCI-IgG). Here, we show that tumor antigen-expressing cancer cells, which are decorated with pMHCI-IgGs containing a HLA-A Ã 0201 molecule associated with a CMV-derived peptide, are specifically eliminated through engagement of antigen-specific CD8 þ T cells isolated from peripheral blood mononuclear cell preparations of CMV-infected humans. These CD8 þ T cells act without additional expansion, preactivation, or provision of costimulatory signals. Elimination of tumor cells is induced at similar concentrations and with similar time kinetics as those seen with bispecific T-cell engagers (BiTE). However, while BiTElike reagents indiscriminately activate T cells through binding to the T-cell receptor complex, pMHCI-IgGs selectively engage antigen-specific, constantly renewable, differentiated effector cytotoxic T lymphocytes to tumor cells, thereby representing a novel class of anticancer immunotherapeutics with potentially improved safety and efficacy profiles.

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Preparation of Stable Single‐Chain Trimers Engineered with Peptide, β2 Microglobulin, and MHC Heavy Chain

Hansen

Fremont

2009

CP in Immunology

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This unit describes a method for constructing a class I MHC molecule with a bound peptide as a single polypeptide chain, termed SCT, for single chain trimer. The component organization of the SCT appears to be widely applicable to different mouse or human MHC class I isotypes bound by different antigenic peptides. The enhanced peptide occupancy afforded by the SCT format makes these molecules effective reagents as DNA vaccines, multimeric staining reagents to enumerate CD8 T cells, and probes of lymphocyte biology.

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Human Major Histocompatibility Complex (MHC) Class I Molecules with Disulfide Traps Secure Disease-related Antigenic Peptides and Exclude Competitor Peptides

Cited by 21 publications

References 55 publications

A Single-Chain H-2Db Molecule Presenting an Influenza Virus Nucleoprotein Epitope Shows Enhanced Ability at Stimulating CD8+ T Cell Responses In Vivo

A Single-Chain H-2Db Molecule Presenting an Influenza Virus Nucleoprotein Epitope Shows Enhanced Ability at Stimulating CD8+ T Cell Responses In Vivo

Committing Cytomegalovirus-Specific CD8 T Cells to Eliminate Tumor Cells by Bifunctional Major Histocompatibility Class I Antibody Fusion Molecules

Preparation of Stable Single‐Chain Trimers Engineered with Peptide, β2 Microglobulin, and MHC Heavy Chain

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