Peters Godefridus J, van Gemert Frank P A, Kathmann Ietje, Reddy Guru, Cillessen Saskia A G M, Jansen Gerrit
Department of Medical Oncology, Amsterdam UMC, VU University Medical Center Amsterdam, Amsterdam, Netherlands.
Department of Biochemistry, Medical University of Gdańsk, Gdańsk, Poland.
Front Cell Dev Biol. 2020 Oct 9;8:577215. doi: 10.3389/fcell.2020.577215. eCollection 2020.
Pralatrexate (Folotyn; PLX) and belinostat (Beleodaq; BLS) are registered for the treatment of patients with peripheral T-cell lymphoma (PTCL) and are being considered for other lymphomas. In this study we investigated whether BLS had the ability to potentiate the cytotoxicity of PLX. A panel of lymphoma cell lines was used for the combination studies: the B-cell SUDHL-4, SUDHL-5, HT, Jeko-1 and T-cell Karpas-299 and Hut-78. Uptake of PLX was mediated by the reduced folate carrier (RFC). PLX showed a 6-fold better RFC substrate affinity compared to methotrexate, and 2-fold better than levoleucovorin (l-LV). Sensitivity expressed as the concentration that resulted in 50% growth inhibition (IC50) after 72 hr exposure to PLX varied from 2.8 to 20 nM and for BLS from 72 to 233 nM, independent of the background of the cell lines. The interaction between BLS and PLX was studied using the median-drug effect analysis. At a fixed molar ratio between the drugs based on the IC50 concentration the average combination index (CI) for all cell lines showed additivity (CI: around 1.0). In three selected cell lines (SUDHL-4, SUDHL-5, and HT) sequential exposure (24 h pretreatment with BLS, followed by 48 h to PLX + BLS), did not improve interaction (CI: 0.9-1.4). As an alternative approach a non-fixed ratio was used by exposing SUDHL-4, SUDHL-5, and HT cells to IC25 concentrations of either BLS or PLX in combination with the other drug. Exposure to IC25 of PLX did not decrease the IC50 for BLS (CI from 0.6-1.2), but exposure to IC25 of BLS markedly increased PLX sensitivity (low CIs from 0.40 to 0.66). Mechanistic studies focused on induction of apoptosis, and showed cleavage of predominantly caspase-9 in HT and SUDHL-4 cells for both drugs at their IC50s, being similar in the combination setting. Moreover, at these concentrations, the drugs were shown to confer an S-phase arrest. In conclusion, the combination of PLX and BLS showed additivity in various lymphoma cell lines, with a schedule-dependent synergism in B-cell lymphoma. Based on these data, proficient inhibition of HDAC activity by BLS holds promise in sensitization of tumor cells to PLX.
普拉曲沙(Folotyn;PLX)和贝利司他(Beleodaq;BLS)已获批用于治疗外周T细胞淋巴瘤(PTCL)患者,并且正在考虑用于其他淋巴瘤的治疗。在本研究中,我们调查了BLS是否具有增强PLX细胞毒性的能力。一组淋巴瘤细胞系用于联合研究:B细胞系SUDHL-4、SUDHL-5、HT、Jeko-1以及T细胞系Karpas-299和Hut-78。PLX的摄取由还原型叶酸载体(RFC)介导。与甲氨蝶呤相比,PLX对RFC底物的亲和力高6倍,比亚叶酸(l-LV)高2倍。以72小时暴露于PLX后导致50%生长抑制的浓度(IC50)表示的敏感性在2.8至20 nM之间,BLS的敏感性在72至233 nM之间,与细胞系背景无关。使用中位药物效应分析研究了BLS与PLX之间的相互作用。在基于IC50浓度的药物固定摩尔比下,所有细胞系的平均联合指数(CI)显示为相加作用(CI:约为1.0)。在三个选定的细胞系(SUDHL-4、SUDHL-5和HT)中,序贯暴露(先用BLS预处理24小时,然后用PLX + BLS处理48小时)并未改善相互作用(CI:0.9 - 1.4)。作为另一种方法,通过将SUDHL-4、SUDHL-5和HT细胞暴露于IC25浓度的BLS或PLX与另一种药物的组合中,使用非固定比例。暴露于PLX的IC25浓度并未降低BLS的IC50(CI为0.6 - 1.2),但暴露于BLS的IC25浓度显著增加了PLX的敏感性(低CI为0.40至0.66)。机制研究集中在凋亡诱导方面,结果显示在HT和SUDHL-4细胞中,两种药物在其IC50浓度下主要诱导caspase-9裂解,在联合用药时情况相似。此外,在这些浓度下,药物显示可导致S期阻滞。总之,PLX和BLS的联合在各种淋巴瘤细胞系中显示出相加作用,在B细胞淋巴瘤中存在时间依赖性协同作用。基于这些数据,BLS对HDAC活性的有效抑制有望使肿瘤细胞对PLX敏感。
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