CYB-5067
CYB-5067 is a FGFR molecular glue degrader with a DC50 of 27 nM against FGFR2. CYB-5067 inhibits FGFR1, FGFR3, FGFR4 and downstream FGFR signaling pathways, induces antiproliferative activity in vitro, and exhibits sustained target protein inhibition in vivo without obvious hook effect. CYB-5067 shows significant tumor growth inhibitory activity in the ETV6-FGFR2 fusion Ba/F3 xenograft model. CYB-5067 can be used for the research of FGFR-driven cancers.
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- 화학식: C26H27Br2Cl2N7O4
- 분자량:732.25
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보관:
Please store the product under the recommended conditions in the Certificate of Analysis.
Biological Activity
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FGFR2 27 nM (DC50) |
FGFR1 430 nM (DC50) |
FGFR3 314 nM (DC50) |
FGFR4 596 nM (DC50) |
CYB-5067 (1.5-10000 nM, 0.123-3.3 μM; 24 h) potently and rapidly degrades FGFR2 in KATO III cells with a DC50 of 27 nM and 96% maximum degradation, achieving sustained target suppression following washout[1].
CYB-5067 (0.0001-10 μM; 72 h) inhibits KATO III cell proliferation with an IC50 of 3.8 nM, showing greater potency than Infigratinib (HY-13311)[1].
CYB-5067 can covalently recruit RNF213 in KATO III and HEK293T cells, forming a ternary complex with FGFR2. This mediates RNF213-dependent FGFR2 ubiquitination and proteasome degradation, independent of NEDD8-mediated E3 ligase activation and lysosomal pathways[1].
CYB-5067 covalently engages RNF213 at the solvent-exposed C1748 residue, which is required for productive recruitment of RNF213[1].
CYB-5067 (0.123-10 μM; 16 h, 0.0001-10 μM; 72 h) acts as a pan-FGFR degrader, potently degrading FGFR1-4 in subtype-specific and multi-subtype cell models with subtype-dependent potency[1].
CYB-5067 (0.5 μM; 12 h) specifically downregulates FGFR2 in KATO III cells at the proteome level, with other observed protein changes being target-driven downstream effects[1].
CYB-5067 (0.123-10 μM; 16 h, 0.0001-10 μM; 72 h) potently degrades FGFR2 and inhibits proliferation in SNU-16 and Ba/F3-ETV6-FGFR2 cells, with high potency in the FGFR2 fusion-positive Ba/F3 model[1].
MedChemExpress (MCE) has not independently confirmed the accuracy of these methods. They are for reference only.
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Cell Line:gastric cancer KATO III cells
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Concentration:1.5, 4.3, 13, 41, 123, 370, 1111, 3333, 10000 nM
0.123, 0.37, 1.1, 3.3 μM -
Incubation Time:24 h
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Result:Induced 86% degradation of FGFR2 after 24 h treatment with 100 nM.
Achieved a half-maximal degradation concentration (DC50) of 27 nM and a maximum degradation (Dmax) of 96% after 24 h with no observed hook effect.
Caused ~43% FGFR2 degradation within 3 h, and 91% degradation after 24 h in time-course analysis.
Demonstrated sustained FGFR2 suppression for up to 24 h after compound removal, with no substantial recovery of protein levels in washout experiments.
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Cell Line:Molt 4, H3255, Huh7, Kelly
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Concentration:0.123, 0.37, 1.1, 3.3, 10 μM
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Incubation Time:72 h
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Result:Exhibiting broad pan-FGFR subtype degradation capacity, CYB-5067 degraded distinct FGFR isoforms in multiple cell lines with single FGFR overexpression: FGFR1 was depleted in Molt 4 cells, FGFR3 was depleted in H3255 cells, and FGFR4 was depleted in Huh7 cells.
MedChemExpress (MCE) has not independently confirmed the accuracy of these methods. They are for reference only.
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Animal Model:BALB/c nude (female)[1]
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Dosage:15 mg/kg; 30 mg/kg
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Administration:i.p.; daily; 12 days
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Result:Achieved 68.1% tumor growth inhibition (TGI).
Achieved 94.6% tumor growth inhibition (TGI).
Showed no significant body weight loss.
Confirmed robust degradation of FGFR2 in tumor tissues at 15 mg/kg dose.
Chemical Information
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분자량 732.25
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화학식 C26H27Br2Cl2N7O4
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SMILES
BrC(Br)C(N(CC1)CCN1C2=CC=C(NC3=NC=NC(N(C)C(NC4=C(Cl)C(OC)=CC(OC)=C4Cl)=O)=C3)C=C2)=O
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선적
Room temperature in continental US; may vary elsewhere.
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보관
Please store the product under the recommended conditions in the Certificate of Analysis.
순도&문서
References
Calculators
Concentration (start) × Volume (start) = Concentration (final) × Volume (final)