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     Quick Explanation


    Core finding
    A recruited “activating” epigenetic bifunctional can activate in a reporter context yet cause rapid transcriptional collapse, chromatin coactivator swapping, and RIPTAC-like degradation in fusion-oncogene cell models—showing induced proximity is not a fixed functional output.



     Long Explanation


    Paper review: An epigenetic bifunctional that toggles between transactivation and repression

    Date in provided record: March 18, 2026 • DOI: 10.64898/2026.03.17.712509
    Mechanistic chromatin toggling Context-dependent proximity outputs RIPTAC-like + degrader-like

    1) Visual map of claims (what the paper argues)

    Evidence basis: reported throughout the paper’s Results/Discussion across reporter, fusion models, and chromatin/ubiquitination readouts.

    2) Quantitative snapshots (from the provided manuscript text)

    These plots summarize numeric values explicitly stated in the provided full text (not inferred).
    Important caution: potency values in different panels/experiments use different units and timepoints, and the plot keeps them separate without converting (only values explicitly stated in the text are used).

    3) Mechanism: what is supported vs. what remains uncertain

    Supported by reported experiments:
    • Induced proximity can be productive: aTAG-2 robustly drives IRF1 reporter transactivation in a FKBP(F36V)-tagged system and shows ternary complex formation evidence in NanoBiT.
    • In fusion-oncogene models, the sign flips: aTAG-2 causes rapid downregulation of EWS/FLI targets and increases repression of genes normally repressed by the fusion program; repression kinetics are fast (within ~0.5–1h; maximal within ~2h).
    • Local cis chromatin changes: ATAC-seq shows consensus loss of accessibility at EWS/FLI sites, motif analysis enriches EWS/FLI sequence, and ChIP-seq indicates CBP gain with p300 loss at fusion-bound loci.
    • Multiple molecular outputs coexist: targeted degradation of FKBP-tagged EWS/FLI is observed, supported by HA loss in ChIP-seq and inhibitor dependence, plus ubiquitination evidence using TUBE2 pull-down; however, repression persists when degradation is pharmacologically blocked, motivating a RIPTAC-like dominant contribution.
    Key uncertainties / open mechanistic questions (critical reading):
    • How general is the “sign flip”? the study uses engineered FKBP(F36V)-tagged transcription factor fusions in specific cancer cell lines; without endogenous targets/in vivo validation, generalization remains uncertain.
    • RIPTAC-like causal chain: the paper infers a dominant RIPTAC-like functional component because repression persists under conditions intended to block degradation. However, “degradation blocked” does not automatically isolate all ternary-complex-mediated steric/function effects, and residual degradation or other pathways could contribute.
    • “p300→CBP exchange” interpretation: ChIP-seq overlap is consistent with substitution, but whether the same factor occupancy kinetics explain all transcriptional outcomes is not conclusively established in the provided excerpt.

    4) Methodological checklist (reproducibility + skepticism)

    Component What the paper did (from provided text) Skeptical note
    Proximity tool FKBP(F36V) binder AP1867 conjugated to multiple activating epigenetic machinery ligands; aTAGs tested in reporter and fusion contexts. Engineered tags and binder occupancy may bias geometry relative to endogenous regulation; “context” may partially reflect tag placement rather than chromatin alone.
    Ternary complex evidence NanoBiT p300/CBP–FKBP reconstitution with dose titration; binders alone inactive; competitor displacement observed. NanoBiT reports proximity in 293T overexpression conditions, which may not equal chromatin-native kinetics.
    Transcriptional outputs Luciferase reporter for IRF1; RNA-seq + GSEA; RT-qPCR time courses for EWS/FLI/NONO/TFE3 targets. Reporter constructs and fusion-tagged systems can constrain downstream programs; transcriptional collapse could include stress pathways—paper argues repression is direct/early.
    Chromatin mapping ATAC-seq for accessibility changes; ChIP-seq for p300/CBP and HA occupancy; motif/GO enrichment on peak sets. Peak-calling and sliding-window peak merging can shift “lost vs stable” peak definitions; the paper uses consensus criteria—robustness across parameterizations isn’t shown in provided text.
    Degradation & ubiquitination HA loss in ChIP-seq; inhibitor tests (E1 TAK-243; proteasome MG-132); ubiquitination smear after TUBE2 pull-down. Inhibitor pleiotropy (E1 or proteasome inhibition) can alter global transcription indirectly; paper uses degradation-block to argue RIPTAC dominance.

    5) Counterpoints / blind spots (what could change the conclusion)

    • Tag-geometry confound: the FKBP(F36V) tag’s position within different fusion proteins could alter whether forced proximity blocks or productive-recruits chromatin coactivators; the paper emphasizes “baseline chromatin state,” but tag placement may also contribute.
    • Alternative explanations for “chromatin rewiring”: CBP/p300 changes could reflect secondary effects of transcriptional collapse or degradation rather than the mechanistic driver; the paper’s early repression kinetics help, but a tighter temporal dissection linking factor exchange → transcriptional switch is not shown in the provided excerpt.
    • Generalization to endogenous (untagged) oncogenic proteins: engineered fusion systems are powerful but may not reproduce the same coactivator saturation, enhancer occupancy, and cofactor stoichiometry found in primary tumors or in vivo microenvironments.
    • Reproducibility across laboratories: the methods are detailed in provided text, but the provided excerpt does not show independent replication in orthogonal systems or different cellular backgrounds.
    All these are framed as uncertainties relative to the evidence described in the paper rather than contradicting the presented data.

    6) Actionable “what BGPT can do next” links

    Citation note: In this response, all paper-specific claims are grounded in the provided manuscript text for DOI 10.64898/2026.03.17.712509.


    Feedback:   

    Updated: April 25, 2026

    BGPT Paper Review


    Study Novelty

    90%

    The work experimentally demonstrates that “activator-recruiting” epigenetic bifunctionals can flip to rapid repression and multiple MOAs (cis coactivator swapping plus ternary-complex-dependent degradation/RIPTAC-like behavior), making induced proximity explicitly context-dependent rather than sign-deterministic.


    Scientific Quality

    80%

    High internal consistency across orthogonal assays (reporter, NanoBiT, RNA-seq/RT-qPCR kinetics, ATAC-seq, ChIP-seq, degradation/ubiquitination inhibitor tests). Skeptical caveats: causal sufficiency of chromatin exchange vs secondary stress remains underdissected in the provided excerpt; RIPTAC-like dominance is inferred from degradation-block persistence without fully quantifying residual degradation.


    Study Generality

    70%

    The conceptual principle (proximity output depends on cellular context) is broadly important, but experimental generalization is still constrained by engineered FKBP(F36V)-tagged fusion models and selected cell lines; endogenous/universal behavior is not established in the provided text.


    Study Usefulness

    90%

    Strong utility for designing/assessing proximity-based transcriptional chemistry: provides a framework of how to measure sign flips, chromatin localization effects, and multi-modal outputs (activation vs repression vs degradation/RIPTAC).


    Study Reproducibility

    70%

    Methods are detailed (constructs, assay types, sequencing pipelines, peak analysis approach), but the provided excerpt does not include raw data accession IDs or explicit deposition details; independent replication across labs is not demonstrated here.


    Explanatory Depth

    90%

    The paper integrates multi-layer evidence (ternary complex, transcription kinetics, accessibility changes, p300/CBP occupancy swapping, and degradation/ubiquitination) into a mechanistic model for context-dependent proximity outputs, exceeding typical single-assay interpretations.


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     Top Data Sources ExportMCP


     Analysis Wizard



    It will parse the paper’s stated gene sets (EWS/FLI targets vs repressed sets), compute a sign-flip summary table (up/down, NES directionality, timepoints), and generate a compact heatmap-ready matrix for comparing conditions.



     Hypothesis Graveyard


    “aTAG-2 simply globally inhibits p300/CBP” is less likely because the paper reports cis-local accessibility loss and selective p300↓/CBP↑ redistribution at fusion-bound sites, and contrasts its RNA-seq signatures with a dual p300/CBP degrader (dCBP-1).


    “Degradation alone causes repression” is weaker because repression persists when proteasome inhibition is used to block degradation components, implying an additional (RIPTAC-like) functional disruption mechanism beyond loss of the tagged protein.

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     Discussion








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