Facultad de Química, Universidad Nacional Autónoma de México , México D.F. 04510, Mexico.
J Nat Prod. 2013 Aug 23;76(8):1454-60. doi: 10.1021/np4002477. Epub 2013 Jul 22.
Bioassay-guided fractionation of an extract prepared from the culture medium and mycelium of Purpureocillium lilacinum allowed the isolation of two calmodulin (CaM) inhibitors, namely, acremoxanthone C (1) and acremonidin A (2). The absolute configuration of 1 was established as 2R, 3R, 1'S, 11'S, and 14'R through extensive NMR spectroscopy and molecular modeling calculations at the DFT B3LYP/DGDZVP level, which included the comparison between theoretical and experimental specific rotation, ³J(C,H), and ³J(H,H) values. Compounds 1 and 2 bind to the human calmodulin (hCaM) biosensor hCaM M124C-mBBr, with dissociation constants (Kd) of 18.25 and 19.40 nM, respectively, 70-fold higher than that of chlorpromazine (Kd = 1.24 μM), used as positive control. Docking analysis using AutoDock 4.2 predicted that 1 and 2 bind to CaM at a similar site to that which KAR-2 binds, which is unusual. Furthermore, a novel, sensible, and specific fluorescent biosensor of hCaM, i.e., hCaM T110C-mBBr, was constructed; this device is labeled at a site where classical inhibitors do not interact and was successfully applied to measure the interaction of 1 with CaM. This is the first report of xanthone-anthraquinone heterodimers in species of Paecilomyces or Purpureocillium genera.
从培养介质和Purpureocillium lilacinum 菌丝体中提取的提取物进行生物测定指导分离,得到了两种钙调蛋白(CaM)抑制剂,分别是 acremoxanthone C(1)和 acremonidin A(2)。通过广泛的 NMR 光谱和在 DFT B3LYP/DGDZVP 水平上的分子建模计算,确定 1 的绝对构型为 2R、3R、1'S、11'S 和 14'R,包括理论和实验比旋光度、³J(C,H)和 ³J(H,H)值的比较。化合物 1 和 2 与人类钙调蛋白(hCaM)生物传感器 hCaM M124C-mBBr 结合,解离常数(Kd)分别为 18.25 和 19.40 nM,分别比阳性对照氯丙嗪(Kd = 1.24 μM)高 70 倍。使用 AutoDock 4.2 进行的对接分析预测,1 和 2 在与 KAR-2 结合的相似部位与 CaM 结合,这是不寻常的。此外,构建了一种新颖、灵敏和特异性的 hCaM 荧光生物传感器,即 hCaM T110C-mBBr;该装置标记在经典抑制剂不相互作用的位点上,并成功应用于测量 1 与 CaM 的相互作用。这是首次在 Paecilomyces 或 Purpureocillium 属的物种中报道黄烷酮-蒽醌杂二聚体。
