Isolation of high affinity human antibodies directly from large synthetic repertoires.

Griffiths, Andrew D.; Williams, S.; Hartley, Oliver; Tomlinson, Ian M.; Waterhouse, Peter M.; Crosby, William L.; Kontermann, Roland E.; Jones, Peter; Low, Nigel M.; Allison, Tyler J.

doi:10.1002/j.1460-2075.1994.tb06626.x

Cited by 908 publications

(546 citation statements)

References 75 publications

(42 reference statements)

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“…The dissociation constant of CEA6 for CEA is in the nanomolar range (7.7 x 10-9 M), which is typical of antibodies isolated from very large repertoires (Perelson and Oster, 1979;Griffiths et al, 1994;Vaughan et al, 1996). Our early work showed that the antibody binds CEA-expressing cells by flow cytometry and immunocytochemistry, and localizes to CEA-expressing human tumour xenografts in nude mice.…”

Section: Discussionmentioning

confidence: 95%

Antigen specificity and tumour targeting efficiency of a human carcinoembryonic antigen-specific scFv and affinity-matured derivatives

Jackson

Bacon²,

Pedley³

et al. 1998

Br J Cancer

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Summary We have examined the biological properties of CEA6, a human carcinoembryonic antigen (CEA)-specific single-chain Fv (scFv) isolated by phage display, and five related clones derived by affinity maturation and selected for improved off-rate (Kff). All clones bind strongly and specifically to CEA-positive human tumours by immunocytochemistry and show negligible cross-reactivity with normal colon. Flow cytometry of scFv on human liver cells indicates a shift in fine epitope specificity resulting from mutagenesis. All monomeric scFv have been radioiodinated, retaining effectively full binding activity. A single intravenous injection into nude mice bearing human colon tumour xenografts confirms tumour targeting in all cases. As reported in other studies, the kidney is the main route of elimination of scFv at early time points. Tumour binding of the parental antibody CEA6 consistently gives the highest tumour-blood ratios at 24 h (mean 16:1). Clone T06D11, which has a sevenfold reduced K0ff relative to CEA6, showed no difference in tumour uptake at 24 h but persisted at the tumour site for longer than CEA6. This study demonstrates a possible correlation between binding affinity and tumour residence time when examined in this model. Keywords: human scFv; carcinoembryonic antigen; affinity maturation Advances in recombinant antibody technology have allowed many of the problems encountered in antibody targeting of tumours to be overcome (Huston et al, 1993). Poor tumour penetrance of whole immunoglobulin has been addressed through the use of smaller fragments derived both enzymatically and by recombinant methods (Yokota et al, 1992;Hu et al, 1996;Rowlinson-Busza et al, 1996). Further advantages of fragments are their rapid extravasation and pharmacokinetic clearance, which are clearly contributing factors in their improved performance as imaging agents (Colcher et al, 1990;Milenic et al, 1991;Verhaar et al, 1995). Moreover, the immunogenicity of rodent monoclonal antibodies (mAbs) has been reduced either by humanization strategies or by de novo isolation of antibody fragments from combinatorial libraries of human V genes (reviewed by Johnson and Chiswell, 1993). Rapid expression in bacteria has greatly assisted the study of improved engineered antibody fragments and has avoided timeconsuming and expensive mammalian cell expression systems.The isolation and characterization of scFv from large phage display libraries has demonstrated several instances where the dissociation constant of the molecule, and more specifically the off-rate (Kodf), is the main predictive factor in performance in in vitro bioassays (Thompson et al, 1996;Schier et al, 1996; Roberts et al, in preparation). The relationship between binding kinetics and tumour targeting efficiency is rather more complicated, mainly because so many additional factors (tumour size, antigen density and rate of turnover, epitope, size and charge of antibody, dose, isotope and labelling chemistry used, presence of circulating antigen) are known to influence the...

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Section: Discussionmentioning

confidence: 95%

Antigen specificity and tumour targeting efficiency of a human carcinoembryonic antigen-specific scFv and affinity-matured derivatives

Jackson

Bacon²,

Pedley³

et al. 1998

Br J Cancer

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“…2A, curves b,c). This was unexpected as the rotational correlation time of a scFv molecule can be calculated according to Visser et al [17] as [10][11][12][13][14][15][16][17][18][19][20] ns. It appears that this discrepancy may be due to association of scFv molecules by hydrophobic interactions in the presence of salt, as in experiments performed in the absence of NaC1 (%crv shifts to about 20 ns (data not shown).…”

Section: Characterization Of Scfv Fragmentsmentioning

confidence: 99%

Phage antibodies against an unstable hapten: Oxygen sensitive reduced flavin

et al. 1996

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It is difficult to raise antibodies against haptens and antigens that are unstable under the physiological conditions of the serum. Here we have used a phage antibody library to isolate antibody fragments against oxygen sensitive reduced flavin, by selection of the phage under anaerobic and reducing conditions at pH 5 and a pre-elution step with the oxidized flavin. The binding of the reduced hapten to one of the antibody fragments was characterised by time-resolved polarised fluorescence, and shown to be highly specific for the reduced flavin.

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“…The theoretical advantages of recombinant human antibodies over mouse monoclonals as therapeutic agents are well recognized [1][2][3][4][5]. However, the optimal source of immunoglobulin genes for the construction of these libraries remains uncertain.…”

Section: Introductionmentioning

confidence: 99%

“…Moreover, it has recently been demonstrated that the retrieval of specific antibodies can be enhanced by increasing the library size and by using synthetic immunoglobulin genes [3,4,8]. The diversity and size of synthetic libraries, and thus the affinity of particular antibodies, can be further increased by combinatorial infection and in vitro recombination strategies [3,9,10]. However, this artificial construction of large non-immune libraries is technically challenging and introduces a number of potential problems.…”

Section: Introductionmentioning

confidence: 99%

Isolation of human anti-c-erbB-2 Fabs from a lymph node-derived phage display library

Clark

Hawkins²,

Papaioannou

et al. 1997

Clinical and Experimental Immunology

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SUMMARYAn immunoglobulin phage display library constructed from a tumour-associated pericolic lymph node was panned against the extracellular domain of the oncoprotein c-erbB-2. Sixteen independent clones were confirmed as positive binders based on ELISA analysis of soluble Fabs. Nucleotide sequencing demonstrated that the V H region of 12 clones belonged to four different V gene families, and the clones demonstrated varying degrees of somatic mutation compared with germ-line sequences. Fab fragments were examined for cross-reactivity by ELISA and shown to be negative against a panel of irrelevant self and non-self antigens, including bovine serum albumin (BSA), mouse immunoglobulin, tetanus toxoid, heregulin-PE40-FLAG and insulin. Reactivity of Fabs in vitro was verified by immunocytochemistry, which showed binding to the c-erbB-2 over-expressing breast cancer cell line SKBR3 but not to the lowexpressing cell line MDA-MB-231. We conclude that a single lymph node library of moderate diversity (2 × 10 7 k light chain and g heavy chain clones), when derived from an individual whose colorectal tumour over-expressed c-erbB-2, can be successfully panned to isolate a number of unique Fabs specific for this antigen. The nature of the anti-c-erbB-2 Fabs recovered from this library suggests that they may have resulted from a humoral immune response in the individual, and that in vivo antibody responses to tumour-associated antigens may be exploited in vitro for the production of tumour-specific recombinant antibodies.

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Isolation of high affinity human antibodies directly from large synthetic repertoires.

Cited by 908 publications

References 75 publications

Antigen specificity and tumour targeting efficiency of a human carcinoembryonic antigen-specific scFv and affinity-matured derivatives

Antigen specificity and tumour targeting efficiency of a human carcinoembryonic antigen-specific scFv and affinity-matured derivatives

Phage antibodies against an unstable hapten: Oxygen sensitive reduced flavin

Isolation of human anti-c-erbB-2 Fabs from a lymph node-derived phage display library

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