Johnston Paul A, Sen Malabika, Hua Yun, Camarco Daniel P, Shun Tong Ying, Lazo John S, Wilson Gabriela Mustata, Resnick Lynn O, LaPorte Matthew G, Wipf Peter, Huryn Donna M, Grandis Jennifer R
1 Department of Pharmaceutical Sciences, School of Pharmacy, University of Pittsburgh , Pittsburgh, Pennsylvania.
2 University of Pittsburgh Cancer Institute , Pittsburgh, Pennsylvania.
Assay Drug Dev Technol. 2015 Sep;13(7):356-76. doi: 10.1089/adt.2015.663.
Signal transducer and activator of transcription factor 3 (STAT3) is hyperactivated in head and neck squamous cell carcinomas (HNSCC). Cumulative evidence indicates that IL-6 production by HNSCC cells and/or stromal cells in the tumor microenvironment activates STAT3 and contributes to tumor progression and drug resistance. A library of 94,491 compounds from the Molecular Library Screening Center Network (MLSCN) was screened for the ability to inhibit interleukin-6 (IL-6)-induced pSTAT3 activation. For contractual reasons, the primary high-content screening (HCS) campaign was conducted over several months in 3 distinct phases; 1,068 (1.1%) primary HCS actives remained after cytotoxic or fluorescent outliers were eliminated. One thousand one hundred eighty-seven compounds were cherry-picked for confirmation; actives identified in the primary HCS and compounds selected by a structural similarity search of the remaining MLSCN library using hits identified in phases I and II of the screen. Actives were confirmed in pSTAT3 IC50 assays, and an IFNγ-induced pSTAT1 activation assay was used to prioritize selective inhibitors of STAT3 activation that would not inhibit STAT1 tumor suppressor functions. Two hundred three concentration-dependent inhibitors of IL-6-induced pSTAT3 activation were identified and 89 of these also produced IC50s against IFN-γ-induced pSTAT1 activation. Forty-nine compounds met our hit criteria: they reproducibly inhibited IL-6-induced pSTAT3 activation by ≥70% at 20 μM; their pSTAT3 activation IC50s were ≤25 μM; they were ≥2-fold selective for pSTAT3 inhibition over pSTAT1 inhibition; a cross target query of PubChem indicated that they were not biologically promiscuous; and they were ≥90% pure. Twenty-six chemically tractable hits that passed filters for nuisance compounds and had acceptable drug-like and ADME-Tox properties by computational evaluation were purchased for characterization. The hit structures were distributed among 5 clusters and 8 singletons. Twenty-four compounds inhibited IL-6-induced pSTAT3 activation with IC50s ≤20 μM and 13 were ≥3-fold selective versus inhibition of pSTAT1 activation. Eighteen hits inhibited the growth of HNSCC cell lines with average IC50s ≤ 20 μM. Four chemical series were progressed into lead optimization: the guanidinoquinazolines, the triazolothiadiazines, the amino alcohols, and an oxazole-piperazine singleton.
信号转导与转录激活因子3(STAT3)在头颈部鳞状细胞癌(HNSCC)中高度活化。越来越多的证据表明,肿瘤微环境中HNSCC细胞和/或基质细胞产生的白细胞介素-6(IL-6)激活STAT3,并促进肿瘤进展和耐药性。对来自分子库筛选中心网络(MLSCN)的94491种化合物文库进行筛选,以检测其抑制白细胞介素-6(IL-6)诱导的pSTAT3活化的能力。由于合同原因,主要的高内涵筛选(HCS)活动分三个不同阶段在几个月内进行;在去除细胞毒性或荧光异常值后,剩下1068种(1.1%)主要的HCS活性物质。挑选了1187种化合物进行确认;包括在主要HCS中鉴定出的活性物质,以及通过使用筛选第一阶段和第二阶段鉴定出的命中物对剩余MLSCN文库进行结构相似性搜索而选择的化合物。在pSTAT3 IC50测定中确认活性物质,并使用IFNγ诱导的pSTAT1活化测定来对不会抑制STAT1肿瘤抑制功能的STAT3活化选择性抑制剂进行优先排序。鉴定出203种IL-6诱导的pSTAT3活化的浓度依赖性抑制剂,其中89种对IFN-γ诱导的pSTAT1活化也产生了IC50值。49种化合物符合我们的命中标准:它们在20μM时可重复抑制IL-6诱导的pSTAT3活化≥70%;它们的pSTAT3活化IC50值≤25μM;它们对pSTAT3抑制的选择性比对pSTAT1抑制高≥2倍;对PubChem的交叉靶点查询表明它们没有生物学上的混杂性;并且它们的纯度≥90%。购买了26种通过了有害化合物筛选且通过计算评估具有可接受的类药和ADME-Tox特性的化学上易于处理的命中物进行表征。命中结构分布在5个簇和8个单例中。24种化合物以IC50值≤20μM抑制IL-6诱导的pSTAT3活化,其中13种对pSTAT1活化的抑制具有≥3倍的选择性。18种命中物抑制HNSCC细胞系的生长,平均IC50值≤20μM。四个化学系列进入先导优化阶段:胍基喹唑啉类、三唑并噻二嗪类、氨基醇类和一个恶唑-哌嗪单例。
