Human Antibodies with Sub-nanomolar Affinities Isolated from a Large Non-immunized Phage Display Library

Vaughan, Tristan J.; Williams, Andrew; Pritchard, Kevin; Osbourn, Jane; Pope, Anthony R.; Earnshaw, J. C.; McCafferty, John; Hodits, Regina A.; Wilton, Jane; Johnson, Kevin S.

doi:10.1038/nbt0396-309

Cited by 934 publications

(635 citation statements)

References 42 publications

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“…The results (not shown) demonstrated that at least 60% percent, and probably more, of the randomly picked clones were efficiently displayed using the phage production methods described in the Materials and Methods. This value is similar or better to those reported for human scFv libraries (Vaughan et al, 1996;O'Connell et al, 2002). The failure to observe scFv/pIII fusion proteins in some clones is likely caused by the poor expression levels of these scFv fusions, or by aberrant or introduced stop codons.…”

Section: Rat Scfv Primer Design and V-domain Amplificationsupporting

confidence: 86%

Design and testing of PCR primers for the construction of scFv libraries representing the immunoglobulin repertoire of rats

Sepúlveda

Shoemaker

2008

Journal of Immunological Methods

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Rats are widely used as a model in the study of many important diseases, yet their utility in research is limited by the lack of robust technology for the production of rat recombinant antibodies. Here we have identified and compiled putative rat immunoglobulin sequences by bioinformatic analysis of recently available genomic and EST databases, and used this information to design PCR primers to amplify rat V H and V L domain coding DNA representing the expressed repertoire of the animal. These primer sets were successfully tested and used to produce a scFv phage display library from rats that had been infected by the blood fluke, Schistosoma mansoni. The library was selected for scFvs that bind to extracellular loop epitopes on either of two known immunogenic S. mansoni membrane proteins, Sm23 and SmTsp2, both of the tetraspanin protein family. Two unique scFvs were identified that bind to each tetraspanin and shown to have excellent specificity for the target, including recognition of the native tetraspanins produced by the fluke. The primers and methods developed for rat scFvs should be of use to others seeking to characterize the antibody repertoire and/or prepare recombinant antibodies from this model.

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Section: Rat Scfv Primer Design and V-domain Amplificationsupporting

confidence: 86%

Design and testing of PCR primers for the construction of scFv libraries representing the immunoglobulin repertoire of rats

Sepúlveda

Shoemaker

2008

Journal of Immunological Methods

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“…To neutralize the inhibitory activity of CRP and to potentiate complement-mediated killing of B lymphoma cells, we have isolated scFv to CD55 and CD59 from a human phage-display library [18] to be used in combination with complement-fixing Rituximab and other complement-activating mAb. The human phage Ab libraries offer the advantage over conventional mAb of a large Ab repertoire that is not shaped by the constraints of the immune system, with a dramatic increase in the chances of isolating Ab to selfantigens [20]. On the other hand, the Ab currently used in cancer therapy, unlike human scFv, are of murine origin and, although engineered to become chimeric or humanized, they still contain murine variable portions of the original Ig that may elicit an anti-idiotypic response [21,22] resulting in their rapid clearance.…”

Section: Discussionmentioning

confidence: 99%

Controlling complement resistance in cancer by using human monoclonal antibodies that neutralize complement-regulatory proteins CD55 and CD59

et al. 2005

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Expression of the complement-regulatory proteins (CRP) CD46, CD55 and CD59 represents a strategy used by tumor cells to evade complement-dependent cell cytoxicity stimulated by monoclonal antibodies. We have isolated two single-chain variable fragments (scFv) to CD55 and CD59 from a human phage-display library and from these scFv we have produced two miniantibodies (MB), MB-55 (against CD55) and MB-59 (against CD59), containing the human hinge-CH2-CH3 domains of IgG1. The specificity of the two MB for the corresponding CRP was assessed by ELISA using purified CD46, CD55 and CD59. MB-55 and MB-59 neutralized the inhibitory activity of CD55 and CD59, respectively, restoring the complement-mediated lysis of sheep and guinea pig erythrocytes that was otherwise inhibited by the two CRP. FACS analysis revealed binding of MB-55 and MB-59 to the lymphoma cell line Karpas 422. The two MB induced a two-fold increase in the complement-dependent killing of these cells stimulated by Rituximab, a chimeric anti-CD20 monoclonal antibody. Transfection of HEK293T cells with vectors encoding MB-55 or MB-59 markedly reduced the expression of CD55 and CD59. We conclude that the human antibodies MB-55 and MB-59 may represent a therapeutic tool to increase the complement-dependent killing activity of Rituximab in the treatment of non-Hodgkin's lymphoma.

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“…Human soluble extracellular domain (ECD) TRAIL-R1-flag fusion protein at 10 mg ml À1 in PBS was immobilised onto immunotubes (Nunc, Rochester, NY, USA) overnight at 41C. Three or four rounds of panning selections were performed using the scFv human antibody phage library with approximately 1.4 Â 10 10 individual recombinants (Vaughan et al, 1996). A deselection round was performed on an irrelevant fusion protein to remove any nonspecific binders.…”

Section: Selection and Generation Of A Trail-r1 Agonist Monoclonal Anmentioning

confidence: 99%

HGS-ETR1, a fully human TRAIL-receptor 1 monoclonal antibody, induces cell death in multiple tumour types in vitro and in vivo

et al. 2005

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Tumour necrosis factor-related apoptosis-inducing ligand (TRAIL) induces apoptosis in a variety of tumour cells through activation of TRAIL-R1 and TRAIL-R2 death signalling receptors. Here, we describe the characterisation and activity of HGS-ETR1, the first fully human, agonistic TRAIL-R1 mAb that is being developed as an antitumour therapeutic agent. HGS-ETR1 showed specific binding to TRAIL-R1 receptor. HGS-ETR1 reduced the viability of multiple types of tumour cells in vitro, and induced activation of caspase 8, Bid, caspase 9, caspase 3, and cleavage of PARP, indicating activation of TRAIL-R1 alone was sufficient to induce both extrinsic and intrinsic apoptotic pathways. Treatment of cell lines in vitro with HGS-ETR1 enhanced the cytotoxicity of chemotherapeutic agents (camptothecin, cisplatin, carboplatin, or 5-fluorouracil) even in tumour cell lines that were not sensitive to HGS-ETR1 alone. In vivo administration of HGS-ETR1 resulted in rapid tumour regression or repression of tumour growth in pre-established colon, non-smallcell lung, and renal tumours in xenograft models. Combination of HGS-ETR1 with chemotherapeutic agents (topotecan, 5-fluorouracil, and irinotecan) in three independent colon cancer xenograft models resulted in an enhanced antitumour efficacy compared to either agent alone. Pharmacokinetic studies in the mouse following intravenous injection showed that HGS-ETR1 serum concentrations were biphasic with a terminal half-life of 6.9 -8.7 days and a steady-state volume of distribution of approximately 60 ml kg À1 . Clearance was 3.6 -5.7 ml À1 day À1 kg À1 . These data suggest that HGS-ETR1 is a specific and potent antitumour agent with favourable pharmacokinetic characteristics and the potential to provide therapeutic benefit for a broad range of human malignancies.

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Human Antibodies with Sub-nanomolar Affinities Isolated from a Large Non-immunized Phage Display Library

Cited by 934 publications

References 42 publications

Design and testing of PCR primers for the construction of scFv libraries representing the immunoglobulin repertoire of rats

Design and testing of PCR primers for the construction of scFv libraries representing the immunoglobulin repertoire of rats

Controlling complement resistance in cancer by using human monoclonal antibodies that neutralize complement-regulatory proteins CD55 and CD59

HGS-ETR1, a fully human TRAIL-receptor 1 monoclonal antibody, induces cell death in multiple tumour types in vitro and in vivo

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