Jähne Evelyn A, Eigenmann Daniela E, Culot Maxime, Cecchelli Roméo, Walter Fruzsina R, Deli Mária A, Tremmel Robin, Fricker Gert, Smiesko Martin, Hamburger Matthias, Oufir Mouhssin
Institute of Pharmaceutical Biology, Department of Pharmaceutical Sciences, University of Basel, Klingelbergstrasse 50, CH-4056 Basel, Switzerland.
Université Lille Nord de France, UArtois, BBB Laboratory EA 2465, IMPRT: IFR114, 62307 Lens Cedex, France.
J Pharm Biomed Anal. 2014 Sep;98:235-46. doi: 10.1016/j.jpba.2014.05.026. Epub 2014 May 27.
The compound (E,Z)-3-(4-hydroxy-3,5-dimethoxybenzylidene)indolin-2-one (indolinone) was identified from lipophilic woad extracts (Isatis tinctoria L., Brassicaceae) as a compound possessing potent histamine release inhibitory and anti-inflammatory properties [1]. To further evaluate the potential of indolinone in terms of crossing the blood-brain barrier (BBB), we screened the compound in several in vitro cell-based human and animal BBB models. Therefore, we developed a quantitative LC-MS/MS method for the compound in modified Ringer HEPES buffer (RHB) and validated it according to FDA and EMA guidelines [2,3]. The calibration curve of indolinone in the range between 30.0 and 3000ng/ml was quadratic, and the limit of quantification was 30.0ng/ml. Dilution of samples up to 100-fold did not affect precision and accuracy. The carry-over was within acceptance criteria. Indolinone proved to be stable in RHB for 3h at room temperature (RT), and for three successive freeze/thaw cycles. The processed samples could be stored in the autosampler at 10°C for at least 28h. Moreover, indolinone was stable for at least 16 days in RHB when stored below -65°C. This validation study demonstrates that our method is specific, selective, precise, accurate, and capable to produce reliable results. In the immortalized human BBB mono-culture model, the apparent permeability coefficient from apical to basolateral (PappA→B), and the Papp from basolateral to apical (PappB→A) were 19.2±0.485×10(-6)cm/s and 21.7±0.326×10(-6)cm/s, respectively. For the primary rat/bovine BBB co-culture model a PappA→B of 27.1±1.67×10(-6)cm/s was determined. In the primary rat BBB triple co-culture model, the PappA→B and the PappB→A were 56.2±3.63×10(-6)cm/s and 34.6±1.41×10(-6)cm/s, respectively. The data obtained with the different models showed good correlation and were indicative of a high BBB permeation potential of indolinone confirmed by in silico prediction calculations. P-glycoprotein (P-gp) interaction for indolinone was studied with the aid of a calcein-AM uptake assay, and by calculation of the efflux ratio (ER) from the bidirectional permeability assays. For both bidirectional BBB models an ER below 2 was calculated, indicating that no active mediated transport mechanism is involved for indolinone. In porcine brain capillary endothelial cells (PBCECs), the calcein-AM uptake assay demonstrated that indolinone is neither a P-gp substrate nor a P-gp inhibitor and is accumulated into cells at high extent.
化合物(E,Z)-3-(4-羟基-3,5-二甲氧基亚苄基)吲哚啉-2-酮(吲哚啉酮)是从亲脂性菘蓝提取物(十字花科菘蓝属植物菘蓝)中鉴定出的一种具有强大组胺释放抑制和抗炎特性的化合物[1]。为了进一步评估吲哚啉酮穿越血脑屏障(BBB)的潜力,我们在几种基于细胞的体外人和动物血脑屏障模型中对该化合物进行了筛选。因此,我们开发了一种用于在改良林格氏HEPES缓冲液(RHB)中检测该化合物的定量液相色谱-串联质谱(LC-MS/MS)方法,并根据美国食品药品监督管理局(FDA)和欧洲药品管理局(EMA)的指南对其进行了验证[2,3]。吲哚啉酮在30.0至3000ng/ml范围内的校准曲线为二次曲线,定量限为30.0ng/ml。样品稀释至100倍不影响精密度和准确度。残留量在可接受标准范围内。吲哚啉酮在室温(RT)下于RHB中3小时内稳定,并且在连续三个冻融循环中稳定。处理后的样品可在自动进样器中于10°C下保存至少28小时。此外,当在-65°C以下储存时,吲哚啉酮在RHB中至少16天稳定。这项验证研究表明,我们的方法具有特异性、选择性、精确性、准确性,并且能够产生可靠的结果。在永生化的人血脑屏障单培养模型中,从顶侧到基底外侧的表观渗透系数(PappA→B)和从基底外侧到顶侧的Papp(PappB→A)分别为19.2±0.485×10(-6)cm/s和21.7±0.326×10(-6)cm/s。对于原代大鼠/牛血脑屏障共培养模型,测定的PappA→B为27.1±1.67×10(-6)cm/s。在原代大鼠血脑屏障三重共培养模型中,PappA→B和PappB→A分别为56.2±3.63×10(-6)cm/s和34.6±1.41×10(-6)cm/s。用不同模型获得的数据显示出良好的相关性,并表明通过计算机预测计算证实吲哚啉酮具有高血脑屏障渗透潜力。借助钙黄绿素-AM摄取试验并通过从双向渗透试验计算流出率(ER),研究了吲哚啉酮与P-糖蛋白(P-gp)的相互作用。对于两种双向血脑屏障模型,计算出的ER均低于2,表明吲哚啉酮不涉及主动介导的转运机制。在猪脑微血管内皮细胞(PBCECs)中,钙黄绿素-AM摄取试验表明吲哚啉酮既不是P-gp底物也不是P-gp抑制剂,并且在细胞中大量积累。
