A Comparative Analysis of the Immunological Evolution of Antibody 28B4

Yin, Jun; Mundorff, Emily C.; Yang, Priscilla L.; Wendt, K. Ulrich; Hanway, D.; Stevens, Raymond C.; Schultz, Peter G.

doi:10.1021/bi010536c

Cited by 76 publications

(72 citation statements)

References 33 publications

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“…4). This ''lock-and-key'' binding mode (22) of the affinity-matured antibody versus ''induced-fit'' binding mechanism (23) in the germ-line antibody was also observed in the antibodies 48G7, AZ28, and 28B4 (19,24,25) and further supports the hypothesis that the structural plasticity of germ-line antibodies is a critical factor in the ability of the immune system to evolve antibodies that bind many distinct chemical structures.…”

Section: Comparison Of the Antibody-combining Site In The Germ-line Andsupporting

confidence: 66%

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Structural evidence for substrate strain in antibody catalysis

Yin

Andryski

Beuscher

et al. 2003

Proc. Natl. Acad. Sci. U.S.A.

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The crystal structure of the Michaelis complex between the Fab fragment of ferrochelatase antibody 7G12 and its substrate mesoporphyrin has been solved to 2.6-Å resolution. The antibodybound mesoporphyrin clearly adopts a nonplanar conformation and reveals that the antibody catalyzes the porphyrin metallation reaction by straining͞distorting the bound substrate toward the transition-state configuration. The crystal structures of the Fab fragment of the germ-line precursor antibody to 7G12 and its complex with the hapten N-methylmesoporphyrin have also been solved. A comparison of these structures with the corresponding structures of the affinity-matured antibody 7G12 reveals the molecular mechanism by which the immune system evolves binding energy to catalyze this reaction.M odern theories of biological catalysis date from Haldane's theory of strain: ''using Fischer's lock and key simile, the key does not fit the lock perfectly but exercises a certain strain on it'' (1). Although the notion that enzymes use binding energy to strain or distort substrates is a fundamental theory of enzyme catalysis (2), it has proven difficult to experimentally validate (3). One approach that has proven effective in testing theories of biological catalysis involves the use of the programmable nature of antibody binding energy to evolve selective catalysts. Antibody catalysis has allowed us to dissect the energetic contributions of transition state stabilization, general base and covalent catalysis, and proximity effects to catalysis (4-9, 29). More recently, we showed that an antibody (7G12) raised against a strained ground-state mimic acted as an efficient porphyrin metallation catalyst (10). We now report the x-ray crystal structure of the Michaelis complex formed between the Fab fragment of the ferrochelatase antibody 7G12 and its substrate mesoporphyrin IX (MP), in which the bound substrate is distorted toward the transition-state conformation for metal insertion. The structure of this complex provides unequivocal structural evidence for the strain theory proposed by Haldane more than 70 years ago. Moreover, the detailed structural and biophysical characterization of the germ-line and affinity-matured antibodies has provided a detailed mechanistic picture of the immunological evolution of this strain mechanism.The enzyme ferrochelatase catalyzes the insertion of Fe 2ϩ into protoporphyrin IX as the last step in heme biosynthesis pathway (11). It was proposed that the enzyme catalyzes the porphyrin metallation reaction by distorting the porphyrin substrate toward a transition state-like geometry in which the pyrrole nitrogen lone pairs are exposed for metal chelation (12). To test this notion, antibody 7G12 was generated against N-methylmesoporphyrin (NMP) in which the porphyrin macrocycle is distorted due to alkylation at one of the pyrrole nitrogens. The resulting antibody was found to catalyze the metallation of MP by Zn 2ϩ with a catalytic efficiency comparable to that of the natural enzyme (10). The same antibody also catal...

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Section: Comparison Of the Antibody-combining Site In The Germ-line Andsupporting

confidence: 66%

“…The binding properties (K d and k off ) of 7G12 Fab, germ-line Fab, and all of the mutants with NMP were measured by surface plasmon resonance on a Biacore 3000 biosensor following the published methods (19). BSA was conjugated with NMP and immobilized on a research grade CM5 sensor chip (Biacore).…”

Section: Methodsmentioning

confidence: 99%

Structural evidence for substrate strain in antibody catalysis

Yin

Andryski

Beuscher

et al. 2003

Proc. Natl. Acad. Sci. U.S.A.

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“…However, recent crystallographic and thermodynamic analyses of both germline and mature Ab-Ag complexes have suggested that the Ab repertoire can be further enhanced at the tertiary structural level (7,14,18,19,34,35). The present study provides an elegant correlation of CDR conformational versatility in a germline Ab with its multispecificity.…”

Section: Discussionmentioning

confidence: 74%

“…In the case of germline mAbs 28B4, 48G7, and AZ28, conformational rearrangement of CDRH3 has been shown to facilitate hapten binding. However, none of these studies have associated conformational flexibility of CDRs with degenerate specificity (14,(35)(36)(37).…”

Section: Discussionmentioning

confidence: 99%

Structural Elucidation of the Mechanistic Basis of Degeneracy in the Primary Humoral Response

Khan

Salunke

2012

The Journal of Immunology

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The mechanistic basis for efficient combating of the infinite range of foreign Ags by the limited repertoire of naive Abs expressed on primary B cell surfaces during their first encounter was addressed through elegantly designed crystallographic analyses. Resolution of the discrepancy arising from the limited number of possible germline Ab receptors on primary B cells for recognizing the unlimited pool of possible Ags has been attempted by invoking the degenerate recognition potential of the germline Abs. Structural analyses of germline mAb BBE6.12H3 in an Ag-free state, as well as bound to four different peptide Ags, established the correlation of its degenerate specificity with conformational versatility of the paratope. Six distinct paratope topologies observed for a single germline mAb provided a quantitative description of the primary Ag recognition repertoire at the tertiary structural level. Each of the four different peptide Ags was bound specifically to a distinct conformation of the paratope, which was also different from that of the Ag-free states of the same germline mAb. A minimal conserved motif in the pristine Ag-combining site essential for multispecificity and Ag binding-mediated change in the elbow angle of Fab was also discernible. It is proposed that the generation of a primary Ab repertoire involves large, yet finite, germline Ab clones, each capable of adopting discrete conformations, which in turn exhibit diverse binding modes.

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“…The dissociation constant K D , the dissociation rate constant k off , and the association rate constant k on of the Ab-Fl complexes were determined by using surface plasmon resonance on a Biacore 3000 biosensor (Biacore, Uppsala, Sweden) following published methods (38). Briefly, BSA was conjugated with Fl and immobilized on a research-grade CM5 sensor chip.…”

Section: Methodsmentioning

confidence: 99%

Antibody evolution constrains conformational heterogeneity by tailoring protein dynamics

Zimmermann¹,

Oakman²,

Thorpe

et al. 2006

Proc. Natl. Acad. Sci. U.S.A.

114

141

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The evolution of proteins with novel function is thought to start from precursor proteins that are conformationally heterogeneous. The corresponding genes may be duplicated and then mutated to select and optimize a specific conformation. However, testing this idea has been difficult because of the challenge of quantifying protein flexibility and conformational heterogeneity as a function of evolution. Here, we report the characterization of protein heterogeneity and dynamics as a function of evolution for the antifluorescein antibody 4-4-20. Using nonlinear laser spectroscopy, surface plasmon resonance, and molecular dynamics simulations, we demonstrate that evolution localized the Ab-combining site from a heterogeneous ensemble of conformations to a single conformation by introducing mutations that act cooperatively and over significant distances to rigidify the protein. This study demonstrates how protein dynamics may be tailored by evolution and has important implications for our understanding of how novel protein functions are evolved.flexibility ͉ nonlinear spectroscopy ͉ fluorscein ͉ molecular recognition

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A Comparative Analysis of the Immunological Evolution of Antibody 28B4

Cited by 76 publications

References 33 publications

Structural evidence for substrate strain in antibody catalysis

Structural evidence for substrate strain in antibody catalysis

Structural Elucidation of the Mechanistic Basis of Degeneracy in the Primary Humoral Response

Antibody evolution constrains conformational heterogeneity by tailoring protein dynamics

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