A scDb-based trivalent bispecific antibody for T-cell-mediated killing of HER3-expressing cancer cells

Beha, Nadine; Steinlein, Sophia; Kühl, Lennart; Seifert, Oliver; Kontermann, Roland E.

doi:10.1038/s41598-021-93351-0

Cited by 7 publications

(18 citation statements)

References 69 publications

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“…Human anti-HER3 antibody 3–43 34 and a humanized version of anti-CD3 UCHT1 27 were used to generate the different trivalent, bispecific antibodies. Genes encoding the different polypeptide chains (see figure 1 ) were cloned into the pSecTagAL1 vector (a modified version of pSecTagA (Invitrogen, Thermo Fisher Scientific, V90020)) and were produced in transiently transfected HEK293-6E cells (NRC Biotechnology Research Institute, Canada) using polyethylenimine (linear, 25 kDa, Sigma-Aldrich, 764604) as described previously.…”

Section: Methodsmentioning

confidence: 99%

“…T-cell proliferation PBMCs were stained with carboxyfluorescein diacetate succinimidyl ester (CFSE) at 625 nM/1×10 6 cells/mL to analyze the proliferative effect on T-cells. 27 MCF-7 cells (2×10 4 cells/well) were incubated with a serial dilution of the trivalent, bispecific antibodies for 15 min at RT and 2×10 5 CFSE-labeled PBMCs/well were added subsequently. Following an incubation for 6 days at 37°C and 5% CO 2 , fluorescence-conjugated antibodies directed against cell surface markers were used to label immune cells of interest and their proliferation was determined Open access by multicolor flow cytometry analysis using MACSQuant Analyzer 10 (Miltenyi Biotec) as described previously.…”

Section: Open Accessmentioning

confidence: 99%

“…Following an incubation for 6 days at 37°C and 5% CO 2 , fluorescence-conjugated antibodies directed against cell surface markers were used to label immune cells of interest and their proliferation was determined Open access by multicolor flow cytometry analysis using MACSQuant Analyzer 10 (Miltenyi Biotec) as described previously. 27…”

Section: Open Accessmentioning

confidence: 99%

“…[53][54][55] Our results are in accordance with recent findings for an Fc-less trivalent, bispecific scDb-scFv fusion protein directed against HER3 and CD3 that, compared with a bivalent bispecific scDb, mediated a strongly increased cytotoxicity toward medium HER3-expressing target cells, which correlated with increased target cell binding, while cytokine release was unaffected. 27 Thus, cytotoxicity mediated by the best (1-2)+1 scDb/scFv-Fc molecule was only reduced 3-fold to 13-fold to that of the scDb-scFv fusion protein described in the previous study, for example, with an EC 50 value of 3 nM for the (1-2)+1 scDb/scFv-Fc and 1 nM for scDb-scFv for MCF-7 and 3 nM vs 41 nM for LIM1215, respectively. 27 Of note, only medium HER3-expressing cells were lysed by the (1-2)+1 scDb/scFv-Fc molecule, while low HER3-expressing cells remained basically unaffected.…”

Section: Open Accessmentioning

confidence: 99%

“… 17 24–26 We have recently demonstrated that a small trivalent, bispecific single-chain diabody (scDb)-scFv showed superior binding to target expressing tumor cells translating into more efficient target cell killing by peripheral blood mononuclear cells (PBMCs). 27 Small bispecific formats such as BiTEs, 28 dual-affinity re-targeting antibodies (DARTs) 29 and scDb 30 have been reported to mediate tight contacts between target cell and T-cells due to their small size and the short distance between the two binding sites, resulting in efficient T-cell activation. However, their pharmacokinetic properties are characterized by a very short serum half-life and continuous infusion is necessary.…”

Section: Introductionmentioning

confidence: 99%

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Fc-comprising scDb-based trivalent, bispecific T-cell engagers for selective killing of HER3-expressing cancer cells independent of cytokine release

Beha

Kühl

Seifert

et al. 2021

J Immunother Cancer

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BackgroundBispecific T-cell engagers are an established therapeutic strategy for the treatment of hematologic malignancies but face several challenges when it comes to their application for the treatment of solid tumors, including on-target off-tumor adverse events. Employing an avidity-mediated specificity gain by introducing an additional binding moiety for the tumor-associated antigen can be achieved using formats with a 2+1 stoichiometry.MethodsBesides biochemical characterization and validation of target cell binding to cancer cells with different HER3 expression, we used in vitro co-culture assays with human peripheral blood mononuclear cells (PBMCs) and HER3-expressing target cells to determine T-cell activation, T-cell proliferation and PBMC-mediated cancer cell lysis of HER3-positive cell lines by the trivalent, bispecific antibodies.ResultsIn this study, we developed trivalent, bispecific antibodies comprising a silenced Fc region for T-cell retargeting to HER3-expressing tumor cells, combining a bivalent single-chain diabody (scDb) fused to a first heterodimerizing Fc chain with either an Fab or scFv fused to a second heterodimerizing Fc chain. All these HER3-targeting T-cell engagers comprising two binding sites for HER3 and one binding site for CD3 mediated target cell killing. However, format and orientation of binding sites influenced efficacy of target cell binding, target cell-dependent T-cell activation and T-cell-mediated target cell killing. Beneficial effects were seen when the CD3 binding site was located in the scDb moiety. These molecules showed efficient killing of medium HER3-expressing cancer cells with very low induction of cytokine release, while sparing target cells with low or undetectable HER3 expression.ConclusionOur study demonstrates that these trivalent, bispecific antibodies represent formats with superior interdomain spacing resulting in efficient target cell killing and a potential advantageous safety profile due to very low cytokine release.

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Section: Methodsmentioning

confidence: 99%

Section: Open Accessmentioning

confidence: 99%

Section: Open Accessmentioning

confidence: 99%

Section: Open Accessmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

Fc-comprising scDb-based trivalent, bispecific T-cell engagers for selective killing of HER3-expressing cancer cells independent of cytokine release

Beha

Kühl

Seifert

et al. 2021

J Immunother Cancer

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Prognostic characteristics of T-cell mediated cell killing-related genes in lung adenocarcinoma

Bi,

Ai,

Zhang

et al. 2023

Autoimmunity

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The eIg technology to generate Ig-like bispecific antibodies

Kühl

Beha

Kontermann

et al. 2022

mAbs

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Bispecific antibodies have emerged as therapeutic molecules with a multitude of modes of action and applications. Here, we present a novel approach to solve the light-chain problem for the generation of bispecific Ig-like antibodies using the second constant domain of IgE (EHD2) genetically modified to force heterodimerization. This was achieved by introducing a C14S mutation in one domain and a C102S mutation in the other domain, which removed of one of the crossover disulfide bonds. Substituting the C H 1 and C L domains of an antigen binding fragment (Fab) with these heterodimerizing EHD2 (hetEHD2) domains resulted in Fab-like building blocks (eFab). These eFabs were used to generate different bispecific antibodies of varying valency and molecular composition employing variable domains with different specificities and from different origins. Formats included bivalent bispecific IgG-like molecules (eIgs) and Fc-less Fab-eFab fusion proteins, as well as tri- and tetravalent Fab-eIg fusion proteins. All proteins, including bispecific antibodies for dual receptor targeting and for retargeting of T cells, efficiently assembled into functional molecules. Furthermore, none of the hetEHD2-comprising molecules showed binding to the two Fcε receptors and are thus most likely do not induce receptor cross-linking and activation. In summary, we established the eIg technology as a versatile and robust platform for the generation of bispecific antibodies of varying valency, geometry, and composition, suitable for numerous applications. Abbreviations: antibody drug conjugate (ADC), acute lymphocytic leukemia (ALL), constant domain of IgE (Cε), receptor of Cε (CεRI or CεRII), cluster of differentiation (CD), constant domain of heavy chain (C H ), constant domain of light chain (C L ), (single-chain) diabody ((sc)Db), diabody-immunoglobulin (Db-Ig), dynamic light scattering (DLS), Fragment antigen-binding (Fab), Fab with hetEHD2 (eFab), Fab-EHD2 with T121G in chain 1 and S10I in chain 2 (EFab), bispecific Ig domain containing hetEHD2 (eIg), extracellular domain (ECD), epidermal growth factor receptor 1, 2, 3 (EGFR, HER2, HER3), heavy chain domain 2 of IgE (EHD2), EHD2 domain with C102S (EHD2-1), EHD2 domain with C14S and N39Q (EHD2-2), (human or mouse) fragment crystalline ((hu or mo)Fc), heavy chain (HC), heterodimerized second domain of IgE (hetEHD2), high molecular weight (HMW), immunoglobulin (Ig), light chain (LC), liquid chromatography-mass spectrometry (LC-MS), mesenchymal epithelial transition factor (MET), heavy chain domain 2 of IgM (MHD2), peripheral blood mononuclear cell (PBMC), prolactin receptor (PRLP), Stokes radius (R S ), single-chain Fragment variable (scFv), tumor necrosis factor (TNF), TNF receptor 2 (TNFR2), single-chain TNF-related apoptosis-inducing ligand (scTRAIL), variable domain of heavy chain (V H ), variable domai...

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A scDb-based trivalent bispecific antibody for T-cell-mediated killing of HER3-expressing cancer cells

Cited by 7 publications

References 69 publications

Fc-comprising scDb-based trivalent, bispecific T-cell engagers for selective killing of HER3-expressing cancer cells independent of cytokine release

Fc-comprising scDb-based trivalent, bispecific T-cell engagers for selective killing of HER3-expressing cancer cells independent of cytokine release

Prognostic characteristics of T-cell mediated cell killing-related genes in lung adenocarcinoma

The eIg technology to generate Ig-like bispecific antibodies

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