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TD-165 Sale

目录号 : GC62600

TD-165 is a PROTAC-based cereblon (CRBN) degrader. TD-165 comprises a cereblon (CRBN) ligand binding group, a linker and an von Hippel-Landau (VHL) binding group.

TD-165 Chemical Structure

Cas No.:2305936-56-3

规格 价格 库存 购买数量
10mM (in 1mL DMSO)
¥4,995.00
现货
5 mg
¥3,150.00
现货
10 mg
¥5,220.00
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25 mg
¥9,900.00
现货
50 mg
¥15,300.00
现货
100 mg
¥22,500.00
现货

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Sample solution is provided at 25 µL, 10mM.

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产品描述

TD-165 is a PROTAC-based cereblon (CRBN) degrader. TD-165 comprises a cereblon (CRBN) ligand binding group, a linker and an von Hippel-Landau (VHL) binding group.

Treatment with TD-165 causes a concentration-dependent decrease in the level of CRBN proteins by Western blot analysis.[1]

TD-165 do not affect CRBN levels in the spleen, peripheral blood mononuclear cells (PBMCs), or liver of mice by immunoblotting, which might be attributable to the high plasma protein binding of TD-165. [1]

[1] Kim K, et al. Sci Rep. 2019 Dec 23;9(1):19654.

Chemical Properties

Cas No. 2305936-56-3 SDF
分子式 C46H59N7O8S 分子量 870.07
溶解度 DMSO : 50 mg/mL (57.47 mM; Need ultrasonic) 储存条件 -20°C, protect from light
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溶解性数据

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1 mg 5 mg 10 mg
1 mM 1.1493 mL 5.7467 mL 11.4933 mL
5 mM 0.2299 mL 1.1493 mL 2.2987 mL
10 mM 0.1149 mL 0.5747 mL 1.1493 mL
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Research Update

Cereblon contributes to cardiac dysfunction by degrading Cav1.2α

Eur Heart J 2022 May 21;43(20):1973-1989.PMID:35190817DOI:10.1093/eurheartj/ehac072

Aims: Cereblon (CRBN) is a substrate receptor of the E3 ubiquitin ligase complex that was reported to target ion channel proteins. L-type voltage-dependent Ca2+ channel (LTCC) density and dysfunction is a critical player in heart failure with reduced ejection fraction (HFrEF). However, the underlying cellular mechanisms by which CRBN regulates LTCC subtype Cav1.2α during cardiac dysfunction remain unclear. Here, we explored the role of CRBN in HFrEF by investigating the direct regulatory role of CRBN in Cav1.2α activity and examining how it can serve as a target to address myocardial dysfunction. Methods and results: Cardiac tissues from HFrEF patients exhibited increased levels of CRBN compared with controls. In vivo and ex vivo studies demonstrated that whole-body CRBN knockout (CRBN-/-) and cardiac-specific knockout mice (Crbnfl/fl/Myh6Cre+) exhibited enhanced cardiac contractility with increased LTCC current (ICaL) compared with their respective controls, which was modulated by the direct interaction of CRBN with Cav1.2α. Mechanistically, the Lon domain of CRBN directly interacted with the N-terminal of Cav1.2α. Increasing CRBN levels enhanced the ubiquitination and proteasomal degradation of Cav1.2α and decreased ICaL. In contrast, genetic or pharmacological depletion of CRBN via TD-165, a novel PROTAC-based CRBN degrader, increased surface expression of Cav1.2α and enhanced ICaL. Low CRBN levels protected the heart against cardiomyopathy in vivo. Conclusion: Cereblon selectively degrades Cav1.2α, which in turn facilitates cardiac dysfunction. A targeted approach or an efficient method of reducing CRBN levels could serve as a promising strategy for HFrEF therapeutics.