Conformation-locking antibodies for the discovery and characterization of KRAS inhibitors

Davies, C.; Oh, Angela; Mroue, Rana; Steffek, Micah; Bruning, John M.; Xiao, Yang; Feng, Siyu; Jayakar, Sangeeta; Chan, Emily; Arumugam, Vidhyalakshmi; Uribe, Sean Carlo; Drummond, Jake; Frommlet, Alexandra; Lü, Cheng; Franke, Yvonne; Merchant, Mark; Koeppen, Hartmut; Quinn, John; Malhotra, Sushant; Do, Steve; Gazzard, Lewis; Purkey, Hans E.; Rudolph, Joachim; Mulvihill, Melinda M.; Koerber, James T.; Wang, Weiru; Evangelista, Marie

doi:10.1038/s41587-021-01126-9

Cited by 6 publications

(13 citation statements)

References 44 publications

(6 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Remarkably, this RAS-specific Nb further inhibits the intrinsic nucleotide exchange of RAS, locking it in a fully inactive conformation. We hypothesize that the interactions of Nb84 with the switch-1 loop of RAS prevent the conformational changes required to exchange the nucleotide, very similar to the conformation-locking antibodies discovered by the Evangelista lab 15 .…”

Section: Resultsmentioning

confidence: 60%

“…PPI-stabilizing Nanobodies to facilitate precision drug discovery. Because many Nbs act as structural chaperones that stabilize specific conformations or interactions, they facilitate small molecule/fragment library screenings by enhancing the binding of (weak) ligands that bind the same conformer 15,25,26 . Previously, a series of indolo-4-aminopiperidines was previously identified as compounds that binds the SOS1•RAS interface and elicits the acceleration of SOS1-catalyzed nucleotide exchange 8 .…”

Section: Nb14 and Ras•gtp Modulate Sos1 Activity By A Similar Alloste...mentioning

confidence: 99%

See 1 more Smart Citation

Competitive, connective and allosteric Nanobodies that modulate the SOS1•RAS protein-protein interactions and tune the nucleotide exchange rate as a starting point for drug design

Fischer

Uchański

Sheryazdanova

et al. 2022

Preprint

View full text Add to dashboard Cite

Protein-protein interactions (PPIs) are central in cell metabolism but research tools for the structural and functional characterization of these PPIs are often missing. Here we introduce novel and broadly applicable immunization (Cross-link PPIs and immunize llamas, ChILL) and selection strategies (Display and co-selection, DisCO) for the discovery of diverse Nanobodies that either stabilize or disrupt PPIs in a single experiment. We applied ChILL and DisCO to identify competitive, connective or fully allosteric Nanobodies that inhibit or facilitate the formation of the SOS1-RAS complex and modulate the nucleotide exchange rate on this pivotal GTPase in vitro and RAS signalling in cellulo. One of these connective Nanobodies fills a cavity that was previously identified as the binding pocket for a series of therapeutic lead compounds. The long complementarity-determining region (CDR3) that penetrates this binding pocket serves as an innovative pharmacophore for extending the repertoire of potential leads.

show abstract

Section: Resultsmentioning

confidence: 60%

Section: Nb14 and Ras•gtp Modulate Sos1 Activity By A Similar Alloste...mentioning

confidence: 99%

Competitive, connective and allosteric Nanobodies that modulate the SOS1•RAS protein-protein interactions and tune the nucleotide exchange rate as a starting point for drug design

Fischer

Uchański

Sheryazdanova

et al. 2022

Preprint

View full text Add to dashboard Cite

show abstract

“…Together, these data suggested that it would be feasible to design a covalent KRAS G12C inhibitor from the non-covalent binders discovered in this study. In contrast, a previously described fragment (GNE-2897, 13 ) and also the switch II pocket binding core groups of two reported KRAS G12C inhibitors ( 14 , 15 ) did not display tight binding to KRAS without their covalent warheads. We hypothesized that the use of a KRAS binding core with native affinity to the protein should enable the discovery of a covalent inhibitor with greater selectivity against other cysteines and therefore lower toxicity as well as a higher second-order rate constant and improved KRAS G12C inhibition, resulting in a stronger antiproliferative effect.…”

Section: Resultsmentioning

confidence: 70%

Fragment Optimization of Reversible Binding to the Switch II Pocket on KRAS Leads to a Potent, In Vivo Active KRAS^G12C Inhibitor

et al. 2022

View full text Add to dashboard Cite

Activating mutations in KRAS are the most frequent oncogenic alterations in cancer. The oncogenic hotspot position 12, located at the lip of the switch II pocket, offers a covalent attachment point for KRAS G12C inhibitors. To date, KRAS G12C inhibitors have been discovered by first covalently binding to the cysteine at position 12 and then optimizing pocket binding. We report on the discovery of the in vivo active KRAS G12C inhibitor BI-0474 using a different approach, in which small molecules that bind reversibly to the switch II pocket were identified and then optimized for non-covalent binding using structure-based design. Finally, the Michael acceptor containing warhead was attached. Our approach offers not only an alternative approach to discovering KRAS G12C inhibitors but also provides a starting point for the discovery of inhibitors against other oncogenic KRAS mutants.

show abstract

“…After homogenization of the core needle biopsy, an aliquot of the lysate with 20 μg of total protein was incubated with anti-RAS antibody clone RAS10, which was pre-immobilized to Protein A magnetic beads. RAS10 has been shown to possess comparable affinity to KRAS G12C with or without covalent modification by immunoprecipitation . After on-bead tryptic digestion, the concentrations of both free and GDC-6036-bound KRAS G12C were determined with 4 μg of total protein using an ultra-sensitive targeted 2D-LC–MS/MS technology, which enables up to 100-fold increase in sensitivity compared to the conventional LC–MS/MS method .…”

Section: Resultsmentioning

confidence: 99%

“…RAS10 has been shown to possess comparable affinity to KRAS G12C with or without covalent modification by immunoprecipitation. 13 After on-bead tryptic digestion, the concentrations of both free and GDC-6036bound KRAS G12C were determined with 4 μg of total protein using an ultra-sensitive targeted 2D-LC−MS/MS technology, which enables up to 100-fold increase in sensitivity compared to the conventional LC−MS/MS method. 12 KRAS G12C engagement was calculated as the ratio of GDC-6036-bound KRAS G12C/ (free KRAS G12C + GDC-6036-bound KRAS G12C).…”

Section: Immunoaffinity Enrichment and Targeted 2d-lc− Ms/ms Approach...mentioning

confidence: 99%

Assessment of KRAS G12C Target Engagement by a Covalent Inhibitor in Tumor Biopsies Using an Ultra-Sensitive Immunoaffinity 2D-LC–MS/MS Approach

Meng¹,

Chan²,

Ng³

et al. 2022

Anal. Chem.

Self Cite

View full text Add to dashboard Cite

KRAS is one of the most frequently mutated oncogenes, with KRAS G12C recently becoming an actionable target for small molecule intervention. GDC-6036 is an investigational KRAS G12C inhibitor that acts by irreversibly binding to the switch II pocket of KRAS G12C when in the inactive GDP-bound state, thereby blocking GTP binding and activation. Assessing target engagement is an essential component of clinical drug development, helping to demonstrate mechanistic activity, guide dose selection, understand pharmacodynamics as it relates to clinical response, and explore resistance. Here, we report the development of an ultra-sensitive approach for assessing KRAS G12C engagement. Immunoaffinity enrichment with a commercially available anti-RAS antibody was combined with a targeted 2D-LC–MS/MS technique to quantify both free and GDC-6036-bound KRAS G12C proteins. A KRAS G12C-positive non-small cell lung cancer xenograft model was dosed with GDC-6036 to assess the feasibility of this assay for analyzing small core needle biopsies. As predicted, dose-dependent KRAS G12C engagement was observed. To date, a sensitivity of 0.08 fmol/μg of total protein has been achieved for both free and GDC-6036-bound KRAS G12C with as little as 4 μg of total protein extracted from human tumor samples. This sub-fmol/μg level of sensitivity provides a powerful potential approach to assess covalent inhibitor target engagement at the site of action using core needle tumor biopsies from clinical studies.

show abstract

Conformation-locking antibodies for the discovery and characterization of KRAS inhibitors

Cited by 6 publications

References 44 publications

Competitive, connective and allosteric Nanobodies that modulate the SOS1•RAS protein-protein interactions and tune the nucleotide exchange rate as a starting point for drug design

Competitive, connective and allosteric Nanobodies that modulate the SOS1•RAS protein-protein interactions and tune the nucleotide exchange rate as a starting point for drug design

Fragment Optimization of Reversible Binding to the Switch II Pocket on KRAS Leads to a Potent, In Vivo Active KRAS^G12C Inhibitor

Assessment of KRAS G12C Target Engagement by a Covalent Inhibitor in Tumor Biopsies Using an Ultra-Sensitive Immunoaffinity 2D-LC–MS/MS Approach

Contact Info

Product

Resources

About

Conformation-locking antibodies for the discovery and characterization of KRAS inhibitors

Cited by 6 publications

References 44 publications

Competitive, connective and allosteric Nanobodies that modulate the SOS1•RAS protein-protein interactions and tune the nucleotide exchange rate as a starting point for drug design

Competitive, connective and allosteric Nanobodies that modulate the SOS1•RAS protein-protein interactions and tune the nucleotide exchange rate as a starting point for drug design

Fragment Optimization of Reversible Binding to the Switch II Pocket on KRAS Leads to a Potent, In Vivo Active KRASG12C Inhibitor

Assessment of KRAS G12C Target Engagement by a Covalent Inhibitor in Tumor Biopsies Using an Ultra-Sensitive Immunoaffinity 2D-LC–MS/MS Approach

Contact Info

Product

Resources

About

Fragment Optimization of Reversible Binding to the Switch II Pocket on KRAS Leads to a Potent, In Vivo Active KRAS^G12C Inhibitor