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Arecoline as a Novel Scaffold Targeting the ATAD2 Bromodomain for Cell Cycle Modulation

Pharmaceutics. 2026-01; 
Ting-Syuan Lin; Jingting Wan; Jingjin He; Shidong Cui; Yun Huang; Bojian Zhang; Hsi-Yuan Huang; Kexin Zhu; Jihang Chen; Tao Zhang; Shangfu Li; Liao Hu; Yongfei Wang; Hsien-Da Huang; Ping Tang; Yang-Chi-Dung Lin
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Protein Electrophoresis and Western Western blotting was performed according to a previous procedure to confirm differential protein expression corresponding to genes [ 20 ]. Using the Genscript eBlot L1 wet transfer system (Genscript, Nanjing, China No. L00686 ), a comparable amount of protein was separated using 8% SDS-PAGE and then transferred according to a previous procedure to confirm differential protein expression corresponding to genes [ 20 ]. Using the Genscript eBlot L1 wet transfer system (Genscript, Nanjing, China No. L00686 ), a comparable amount of protein was separated using 8% SDS-PAGE and then transferred onto polyvinylidene difluoride membranes Get A Quote

Abstract

Background/Objectives : ATPase family AAA domain-containing protein 2 (ATAD2) is an oncogenic chromatin regulator that amplifies E2F/MYC transcriptional programs, yet direct modulators remain scarce. Arecoline (ARE), the primary alkaloid of the areca nut, is a known carcinogen but paradoxically exhibits context-dependent anti-proliferative activities. In this study, we resolve this paradox by defining ARE s anti-cancer mechanism. Methods : Breast cancer cell proliferation and colony formation assays were performed to evaluate the anti-proliferative effects of ARE. Cell-cycle distribution was analyzed to determine phase-specific effects. Transcriptomic profiling was conducted to identify affected gene networks. ... More

Keywords

arecoline, target identification, ATAD2, cell cycle, lead optimization