Seeking high-priority mutations enabling successful antibody-breeding: systematic analysis of a mutant that gained over 100-fold enhanced affinity

Oyama, Hiroyuki; Kiguchi, Yuki; Morita, Izumi; Yamamoto, Chika; Higashi, Yuka; Taguchi, Miku; Enami, Yuri; Takamine, Yuriko; Hasegawa, Hirotsugu; Takeuchi, Atsuko; Kobayashi, N.

doi:10.1038/s41598-020-61529-7

Cited by 12 publications

(17 citation statements)

References 46 publications

(108 reference statements)

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“…4 A), represented by the less substitutions (and insertions) that were concentrated more in the V H and in CDRs. It should be noted that no scFv mutant obtained with CAP, as well as that recovered from the panning, had substitution/insertion in the V H -CDR3 that is regarded as the most crucial among the six CDRs to generate affinity and specificity against a definite antigen structure 11 (Fig. 4 A).…”

Section: Discussionmentioning

confidence: 99%

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Clonal array profiling of scFv-displaying phages for high-throughput discovery of affinity-matured antibody mutants

Kiguchi

Oyama

Morita

et al. 2020

Sci Rep

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"Antibody-breeding" approach potentially generates therapeutic/diagnostic antibody mutants with greater performance than native antibodies. Therein, antibody fragments (e.g., single-chain Fv fragments; scFvs) with a variety of mutations are displayed on bacteriophage to generate diverse phage-antibody libraries. Rare clones with improved functions are then selected via panning against immobilized or tagged target antigens. However, this selection process often ended unsuccessful, mainly due to the biased propagation of phage-antibody clones and the competition with a large excess of undesirable clones with weaker affinities. To break radically from such panning-inherent problems, we developed a novel method, clonal array profiling of scFv-displaying phages (CAP), in which colonies of the initial bacterial libraries are examined one-by-one in microwells. Progenies of scFv-displaying phages generated are, if show sufficient affinity to target antigen, captured in the microwell via pre-coated antigen and detected using a luciferase-fused anti-phage scFv. The advantage of CAP was evidenced by its application with a small error-prone-PCR-based library (~ 10 5 colonies) of anti-cortisol scFvs. Only two operations, each surveying only ~ 3% of the library (9,400 colonies), provided five mutants showing 32–63-fold improved K a values (> 10 10 M −1 ), compared with the wild-type scFv ( K a = 3.8 × 10 8 M −1 ), none of which could be recovered via conventional panning procedures operated for the entire library.

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Section: Discussionmentioning

confidence: 99%

“…1 B). To enable more sensitive immunochemical analyses 10 , 11 , we have generated affinity-matured scFv mutants against estradiol-17β 12 – 14 , cotinine 15 , and cortisol 16 , each of which gained an equilibrium affinity constant ( K a ) enhanced by > 150-fold, > 40-fold, and > 30-fold, respectively (Fig. 2 A–C).…”

Section: Introductionmentioning

confidence: 99%

Clonal array profiling of scFv-displaying phages for high-throughput discovery of affinity-matured antibody mutants

Kiguchi

Oyama

Morita

et al. 2020

Sci Rep

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“…However, there seems to be an “affinity ceiling” for the native antibodies obtained from immunized animals through conventional hybridoma-based methods 4 . Indeed, murine antibodies against small biomarkers, such as steroids or synthetic drugs categorized as haptens, rarely show equilibrium affinity constants ( K a s) that exceed the range of 10 10 M −1 , which hampers the development of immunoassay systems with subfemtomole-range sensitivities 5 , 6 .…”

Section: Introductionmentioning

confidence: 99%

The VH framework region 1 as a target of efficient mutagenesis for generating a variety of affinity-matured scFv mutants

Kiguchi

Oyama

Morita

et al. 2021

Sci Rep

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In vitro affinity-maturation potentially generates antibody fragments with enhanced antigen-binding affinities that allow for developing more sensitive diagnostic systems and more effective therapeutic agents. Site-directed mutagenesis targeting “hot regions,” i.e., amino acid substitutions therein frequently increase the affinities, is desirable for straightforward discovery of valuable mutants. We here report two “designed” site-directed mutagenesis (A and B) targeted the N-terminal 1–10 positions of the VH framework region 1 that successfully improved an anti-cortisol single-chain Fv fragment (Ka, 3.6 × 108 M−1). Mutagenesis A substituted the amino acids at the position 1–3, 5–7, 9 and 10 with a limited set of substitutions to generate only 1,536 different members, while mutagenesis B inserted 1–6 random residues between the positions 6 and 7. Screening the resulting bacterial libraries as scFv-phage clones with a clonal array profiling system provided 21 genetically unique scFv mutants showing 17–31-fold increased affinity with > 109 M−1Ka values. Among the mutants selected from the library A and B, scFv mA#18 (with five-residue substitutions) and mB1-3#130 (with a single residue insertion) showed the greatest Ka value, 1.1 × 1010 M−1.

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“…37 Indeed, we have generated scFv mutants that showed approximately 10-150-fold increased K a s over parental antibodies against various haptens, enabling immunoassays with improved sensitivities. 9,15,[38][39][40][41][42][43] We have also found an alternative approach for enhancing sensitivity of immunoassay for hapten molecules. 44 For example, the hallucinogenic compound psilocin (the hapten of interest) was detected aer chemical derivatization into its tertbutyldimethylsilyl (TBS) ether that has a larger M r and a wider Connolly molecular area.…”

Section: Backgrounds Of the Present Derivatization-assisted Immunoassaysmentioning

confidence: 99%

“…The latter challenge arises from the fact that the haptenic antigens as small as (S)-MAP and -AP usually equip with only a few functional groups that are available for interaction with antibody paratopes. [7][8][9] Owens et al, however, have generated hybridoma-derived monoclonal antibodies (mAbs) that bind to (S)-MAP with an equilibrium dissociation constant (K d ) of $10 nM by immunizing mice with systematically designed haptenic derivatives. 5,10 However, these antibodies unfortunately failed to recognize (S)-AP with similar affinities.…”

Section: Introductionmentioning

confidence: 99%

Derivatization-assisted immunoassays: application for group-specific detection of potent methamphetamine and amphetamine enantiomers

et al. 2022

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Seeking high-priority mutations enabling successful antibody-breeding: systematic analysis of a mutant that gained over 100-fold enhanced affinity

Cited by 12 publications

References 46 publications

Clonal array profiling of scFv-displaying phages for high-throughput discovery of affinity-matured antibody mutants

Clonal array profiling of scFv-displaying phages for high-throughput discovery of affinity-matured antibody mutants

The VH framework region 1 as a target of efficient mutagenesis for generating a variety of affinity-matured scFv mutants

Derivatization-assisted immunoassays: application for group-specific detection of potent methamphetamine and amphetamine enantiomers

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