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"I would rather have questions that can't be answered than answers that can't be questioned."
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Quick Explanation
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Targeted KRAS inhibition resistance is mapped end-to-end
This work uses CRISPR base-editing tiling (βKras-TILEβ) and a cancer-mutation library to identify on-target KRAS second-site mutations and non-KRAS genetic bypasses that rewire signaling against three mechanistically distinct KRAS-targeted therapies (adagrasib, RMC-4998, RMC-7977). A key mechanistic spotlight is CIC R215Q, which drives resistance to RMC-7977 and correlates with NF-ΞΊB pathway activation; combining with an IKK inhibitor restores sensitivity in models.
Long Explanation
Paper Review (visual-first): Genetic mechanisms of resistance to targeted KRAS inhibition
What the authors did (in one line): They combine SpRY/CBE/ABE base-editing tiling + sensor-based sequencing + hit deconvolution to map genetic resistance mutations to three mechanistically distinct KRAS-targeted inhibitors, then validate top drivers (notably CIC R215Q) and test a signaling-combination strategy via IKK/NF-ΞΊB.
1) Evidence snapshots (from the paperβs reported numbers)
These plots summarize key scale parameters explicitly stated in the manuscript text provided.
Reported: MBES screen identifies 33 sgRNAs representing 23 distinct SNVs significantly enriched (median LFC > 1, p-adj < 0.05) across inhibitor arms with editing > 20% at sensor; MBES library size is described as 4686 sgRNAs targeting ~1177 recurrent cancer-associated mutations, and Kras-TILE is 1732 sgRNAs.
2) Mechanistic map (known vs inferred vs uncertain)
Known from the paperβs experiments (higher confidence)
KRAS-TILE base-editing sensors and editing-deconvolution via BEquant were necessary because SpRY-based base editors can cause sgRNA self-editing that breaks exact whitelist assignment; the authors report probabilistic matching improves assignment to >99% vs ~25β35% with exact matching.
Drug-specific second-site KRAS hotspots emerge in different inhibition contexts; adagrasib enriches guides at KRAS G12C allele and additional regions (including clinical adagrasib-resistance codons), while RMC-4998 shows a more restricted pattern consistent with its G12C-selective tri-complex mechanism, and RMC-7977 enriches SWII-region variants consistent with altered tri-complex inhibition.
CIC R215Q is reported as a recurrent genetic driver of RMC-7977 resistance in vitro and in vivo, and the authors connect its resistance phenotype to NF-ΞΊB pathway upregulation in RNA-seq followed by IKK-16 synergy restoring sensitivity.
βTri-complex disruptionβ mechanistic inference for specific RMC-7977 resistance KRAS variants is supported by structural proximity arguments and molecular dynamics modeling described by the authors; however, because modeling and screen-derived edits are not the same as direct biochemical binding assays, the exact biophysical mechanism remains partially indirect.
Key uncertainties / plausible alternative explanations
Model-system specificity: major validations rely on mouse KP-derived cell lines and a human Calu-1 context; resistance wiring can be context-dependent (other KRAS alleles, co-mutations, lineage states, and microenvironmental constraints).
Editor-specific effects: SpRY-based near-PAMless editing introduces self-editing and potentially other biases (e.g., editing window distributions); while BEquant addresses read assignment, off-target editing or enzyme-specific cellular effects can still confound genotypeβphenotype inference.
3) What this paper adds beyond prior knowledge
The main conceptual upgrade is systematic, mechanistically stratified mapping of resistance mutations to distinct KRAS-state-targeting drugs using true coding-sequence saturation base editing in a controlled genetic background. The study also contributes a computationally grounded solution (BEquant / LSH-based probabilistic readβguide assignment) to an important practical failure mode for near-PAMless SpRY editors (self-editing interfering with exact guide enumeration).
Additionally, the CICβNF-ΞΊB axis is positioned as a genetic-to-transcriptional bridge, which is mechanistically useful because it offers a concrete pathway for combination logic (as tested with IKK-16 in the paperβs system).
4) Skeptical critique (what could mislead, and what would disprove)
Hit calling depends on modeling assumptions: sgRNA enrichment/depletion uses pooled sequencing counts, and deconvolution relies on probabilistic matching without UMI-based ground truth; even with BEquant, residual mis-assignment or mapping errors could distort LFC estimates for lowly represented guides.
Editing β perfect genotyping: base editing creates intended SNVs but can also produce byproducts (e.g., unintended edits within window, context dependence). The paper focuses on sensor editing and predicted transitions; incomplete accounting of bystander edits could blur mapping between specific intended SNVs and resistance phenotype.
Combination inference is conditional: synergy with IKK-16 is measured in specific in vitro dosing and cell models; NF-ΞΊB activation may be necessary in the tested CIC context, but it might not be sufficient or universally targeting the driver.
Publication/reporting risks (general scientific epistemology): the work is strongly mechanistic and includes validation, which reduces random false positives, but the broader resistance landscape still risks over-weighting pathways that are more tractable to validate (e.g., those with available inhibitors).
What would most strongly disprove the central mechanistic claim?
Show that CIC R215Q does not confer RMC-7977 resistance in additional independent genetic backgrounds/allelic contexts beyond those tested, or that NF-ΞΊB inhibition fails to restore sensitivity despite equivalent pathway modulation.
Demonstrate that the KRAS residue-specific resistance patterns (e.g., E63/Y71 region) do not correspond to altered tri-complex formation/binding in direct biochemical assays under experimentally matched conditions.
5) Practical βwhat to do with thisβ guide (researcher-facing)
Resistance atlas use: Treat the KRAS second-site hotspots as candidate resistance alleles that may be inhibitor-mechanism-specific, then test cross-sensitivity by running the same base-editing logic against other KRAS inhibitors (or by targeted editing of top SNVs into additional isogenic lines).
Mechanism prioritization: For hits like CIC R215Q, follow a genotypic driver β pathway transcriptional signature β dependency perturbation chain (the paper provides this as an end-to-end example with RNA-seq and IKK-16 synergy).
6) Links for deeper exploration on BGPT
Author reviews (BGPT)
Note: the BGPT author-review links are generated from the full names explicitly present in the provided TEI author list.
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Updated: April 01, 2026
BGPT Paper Review
Study Novelty
90%
Near-saturation BE tiling across KRAS coding sequence coupled to an explicit, custom LSH-based sensor deconvolution (BEquant) for SpRY self-editing, then applied to three mechanistically distinct KRAS inhibitors with both on-target and non-KRAS bypass mapping and a validated CICβNF-ΞΊB vulnerability link.
Scientific Quality
80%
Strong internal logic: robust screening scale, explicit handling of a known BE analysis failure mode (self-editing), multiple inhibitor contexts, and mechanistic validation including in vivo and transcriptomics with a pathway perturbation (IKK-16). Skeptical caveat: mechanistic tri-complex claims rely partly on computational modeling and the translational scope is limited by the specific genetic background(s) used and potential base-editor platform biases.
Study Generality
70%
The principleβmechanism-stratified BE mapping of resistance and pathway vulnerability discoveryβis generalizable, but the specific drivers (e.g., CIC R215Q and NF-ΞΊB) and KRAS second-site spectra may depend on KRAS allele, model lineage, and co-mutation context; the study validates mainly in mouse KCP lines plus limited human context (Calu-1).
Study Usefulness
90%
High usefulness for hypothesis generation and experimental prioritization: it provides a concrete resistance allele list/spectra and identifies a directly testable signaling vulnerability (NF-ΞΊB/IKK) connected to a specific recurrent genetic event.
Study Reproducibility
80%
Methods are detailed (library sizes, dosing schedule, analysis tools, and data accession for sensor amplicon + RNA-seq fastqs). Remaining reproducibility risk: exact base-editor and guide library construction details are spread across supplements; BEquant requires careful parameter choices (e.g., hashing settings) and the reliance on probabilistic assignment adds sensitivity to implementation details.
Explanatory Depth
80%
Mechanistic depth is strong for the CICβNF-ΞΊBβIKK-16 resensitization chain and for inhibitor-mechanism-specific KRAS variant selection. Depth is somewhat limited where claims depend on indirect modeling rather than direct biochemical measurements of tri-complex stability across mutant genotypes.
It reconstructs a resistance landscape table from the paperβs reported screen outputs (sgRNA IDs, inhibitor arms, timepoints) and produces an interactive Sankey of genotypeβdrugβresistance classes using SRA-derived counts.
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Hypothesis Graveyard
A purely on-target βdrug biophysics onlyβ explanation for CIC R215Q resistance (i.e., CIC alters KRAS tri-complex formation directly) is less favored because the paper emphasizes transcriptomic NF-ΞΊB derepression and functional resensitization by IKK inhibition.
A model in which CIC R215Q resistance is driven mainly by MAPK derepression rather than NF-ΞΊB is weakened by the paperβs reported observation that only a limited set of KRAS signaling genes appear derepressed, while NF-ΞΊB emerges as the specific positively regulated pathway in CIC mutants.
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