Inhibition of HER3 activation and tumor growth with a human antibody binding to a conserved epitope formed by domain III and IV

Schmitt, Lisa C.; Rau, Alexander; Seifert, Oliver; Honer, Jonas; Hutt, Meike; Schmid, Simone; Zantow, Jonas; Hust, Michael; Dübel, Stefan; Kontermann, Roland E.

doi:10.1080/19420862.2017.1319023

Cited by 20 publications

(31 citation statements)

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“…In these formats, a single-chain version of TRAIL that consists of amino acids 118 to 281 with a single glycine residue as linker to connect the protomers [ 21 ] was fused to the C-terminus of a human γ1 Fc region, while a TAA-targeting single-chain variable fragment was optionally located N-terminally (Figure 1A, 1B ). Five different antibody moieties directed against four distinct tumor-associated antigens were employed, including the EGFR-targeting antibody hu225 derived from antibody C225 used in cetuximab [ 29 ] and humanized by CDR grafting [ 30 ], the trastuzumab-derived 4D5 directed against HER2 [ 31 ], the HER3-targeting antibodies 3M6 (a modified version of MM-121, Ab#6 [ 32 ] with a mutation of C89 of the V L according to the Kabat numbering scheme to serine) and 3-43 [ 33 ], as well as the humanized version 323/A3hu3 [ 34 ] of the anti-EpCAM antibody 323/A3 [ 35 , 36 ]. All molecules further comprised a FLAG-tag at the N-terminus allowing purification of the proteins from the supernatant of stably transfected HEK293T cells by FLAG affinity chromatography.…”

Section: Resultsmentioning

confidence: 99%

“…Modular vectors for sequential insertion of the Fc region, scTRAIL, and the antibody moiety were created based on pSecTagAL1, a modified version of pSecTagA (Invitrogen, Thermo Fisher Scientific, V90020) comprising an AgeI restriction site at the 3’-end of the Igκ chain leader sequence. In order to eliminate potential protease cleavage sites, K447 of the human IgG1 Fc (EU numbering scheme) was mutated to Q. Single-chain variable fragments hu225 [ 30 ], 4D5 [ 31 ], 3M6 (derived from MM-121, Ab #6 [ 32 ] comprising a cysteine to serine mutation at position 89 (Kabat numbering scheme) in the variable domain of the light chain), 3–43 [ 33 ], and 323/A3hu3 [ 34 ] directed against EGFR, HER2, HER3, and EpCAM were used. A single-chain version of TRAIL (scTRAIL) containing amino acid residues 118–281 of human TRAIL and a linker composed of a single glycine residue was used to create the various fusion proteins [ 21 ].…”

Section: Methodsmentioning

confidence: 99%

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Targeting scFv-Fc-scTRAIL fusion proteins to tumor cells

et al. 2018

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Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Targeting scFv-Fc-scTRAIL fusion proteins to tumor cells

et al. 2018

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“…The variable domains of a humanized version of anti-EGFR antibody cetuximab (hu225) 28 and anti-HER3 antibody IgG 3-43 29 were used to generate tetravalent bispecific Db-Ig molecules. In total, four different tetravalent bispecific molecules were produced using different dimerization domains (DD): C H 1/C L , EHD2, MHD2, and hetEHD2 (Figure 2(a)).…”

Section: Tetravalent Bispecific Db-igs Targeting Egfr and Her3mentioning

confidence: 99%

“…Similar to the ELISA binding studies, concentration-dependent binding was detected for all analyzed antibodies. As FaDu cells express very high amount of EGFR (~140,000 receptors per cell) and low amounts of HER3 (~3,000 receptors per cell) on their surface, 29 cell binding was obviously dominated by EGFR, which resulted in binding of IgG hu225 and of all bispecific antibodies with similar EC 50 values in the range between 129 and 238 pM ( Table 1).…”

Section: Tetravalent Bispecific Db-igs Targeting Egfr and Her3mentioning

confidence: 99%

Diabody-Ig: a novel platform for the generation of multivalent and multispecific antibody molecules

Seifert

Rau

Beha

et al. 2019

mAbs

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Multivalent mono-or bispecific antibodies are of increasing interest for therapeutic applications, such as efficient receptor clustering and activation, or dual targeting approaches. Here, we present a novel platform for the generation of Ig-like molecules, designated diabody-Ig (Db-Ig). The antigen-binding site of Db-Ig is composed of a diabody in the V H-V L orientation stabilized by fusion to antibody-derived homo-or heterodimerization domains, e.g., C H 1/C L or the heavy chain domain 2 of IgE (EHD2) or IgM (MHD2), further fused to an Fc region. In this study, we applied the Db-Ig format for the generation of tetravalent bispecific antibodies (2 + 2) directed against EGFR and HER3 and utilizing different dimerization domains. These Db-Ig antibodies retained the binding properties of the parental antibodies and demonstrated unhindered simultaneous binding of both antigens. The Db-Ig antibodies could be purified by a single affinity chromatography resulting in a homogenous preparation. Furthermore, the Db-Igs were highly stable in human plasma. Importantly, only one short peptide linker (5 aa) per chain is required to generate a Db-Ig molecule, reducing the potential risk of immunogenicity. The presence of a fully functional Fc resulted in IgG-like pharmacokinetic profiles of the Db-Ig molecules. Besides tetravalent bispecific molecules, this modular platform technology further allows for the generation of other multivalent molecules of varying specificity and valency, including mono-, bi-, tri-and tetraspecific molecules, and thus should be suitable for numerous applications.

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“…These libraries were derived from 44 donors and contain around 5 billion independent clones. From these libraries, more than 1,000 antibodies for international proteome binder consortia [43][44][45], diagnostic antibodies [46,47] as well as candidates for therapeutic applications [48][49][50] were selected. The next generation of human naïve antibody gene libraries (HAL9/10) was derived from 98 donors with a broad spectrum of ethnic origins and contains a diversity of more than 10 billion independent clones [32].…”

Section: Phage Display Is a Robust And Reliable Source For Human Monomentioning

confidence: 99%

Designing Human Antibodies by Phage Display

Frenzel

Kügler²,

Helmsing

et al. 2017

Transfus Med Hemother

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ever, are recognized as foreign proteins by humans and therefore induce immune reactions against the therapeutic reagent (human anti-mouse antibody; HAMA) [3]. A solution to this problem was only brought by recombinant DNA technology. Using genetic engineering, the murine sequences were exchanged in parts of the molecule by the homologous human sequences. The result were 'chimeric' (with murine constant domains replaced by human constant domains) or 'humanized' antibodies (only the antigen-binding loops / complementarity determining regions (CDRs) were transferred to human variable region frameworks) [4,5]. These engineered mouse antibodies dominated the first decade of therapeutic antibody approvals, while today it is preferred to use completely human antibodies from the start, thanks to a number of novel technologies allowing to identify them without the necessity to immunize humans. These are on the one hand transgenic animals, typically mice or rats, which carry genetically introduced human immunoglobulin loci while their own antibody genes were knocked out [6][7][8]. Consequently, after immunization they utilize this sequence repertoire to generate IgG from human germ-line sequences, thereby allowing to generate monoclonals by means of classical hybridoma technology. An even more radical way was introduced by the development of antibody phage display, which allowed for the first time to generate human antibodies completely in the test tube and without immunization. Inspired by the work of G.P. Smith on peptide display using filamentous phage [9], antibody phage display was development independently in Heidelberg by Breitling and Dübel [10], in Cambridge by McCafferty et al. [11], and in California by Barbas et al. [12]. The method is based on a physical link between function (antigen binding) and information (antibody gene) in a nanoparticle (the phage virus particle). To achieve this, the antigen binding parts of the antibodies, either as Fab (fragment antigen binding) [13,14] or scFv (single chain fragment variable) [15][16][17], are genetically linked to the surface protein III (pIII) of the M13 phage and thus expressed on the surface of the virus particle. Mixtures of such phage particles, each enKeywords Human monoclonal antibodies · Phage display · Immunotherapy · In vitro evolution · Panning · scFv Summary With six approved products and more than 60 candidates in clinical testing, human monoclonal antibody discovery by phage display is well established as a robust and reliable source for the generation of therapeutic antibodies. While a vast diversity of library generation philosophies and selection strategies have been conceived, the power of molecular design offered by controlling the in vitro selection step is still to be recognized by a broader audience outside of the antibody engineering community. Here, we summarize some opportunities and achievements, e.g., the generation of antibodies which could not be generated otherwise, and the design of antibody properties by different panning strategie...

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Inhibition of HER3 activation and tumor growth with a human antibody binding to a conserved epitope formed by domain III and IV

Cited by 20 publications

References 46 publications

Targeting scFv-Fc-scTRAIL fusion proteins to tumor cells

Targeting scFv-Fc-scTRAIL fusion proteins to tumor cells

Diabody-Ig: a novel platform for the generation of multivalent and multispecific antibody molecules

Designing Human Antibodies by Phage Display

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