Department of Medicine/Hematology-Oncology Division, Weill Medical College of Cornell University, New York, NY 10065, USA.
Cancer Discov. 2012 Nov;2(11):1004-23. doi: 10.1158/2159-8290.CD-12-0208. Epub 2012 Oct 29.
Genetic lesions such as BCR-ABL1, E2A-PBX1, and MLL rearrangements (MLLr) are associated with unfavorable outcomes in adult B-cell precursor acute lymphoblastic leukemia (B-ALL). Leukemia oncoproteins may directly or indirectly disrupt cytosine methylation patterning to mediate the malignant phenotype. We postulated that DNA methylation signatures in these aggressive B-ALLs would point toward disease mechanisms and useful biomarkers and therapeutic targets. We therefore conducted DNA methylation and gene expression profiling on a cohort of 215 adult patients with B-ALL enrolled in a single phase III clinical trial (ECOG E2993) and normal control B cells. In BCR-ABL1-positive B-ALLs, aberrant cytosine methylation patterning centered around a cytokine network defined by hypomethylation and overexpression of IL2RA(CD25). The E2993 trial clinical data showed that CD25 expression was strongly associated with a poor outcome in patients with ALL regardless of BCR-ABL1 status, suggesting CD25 as a novel prognostic biomarker for risk stratification in B-ALLs. In E2A-PBX1-positive B-ALLs, aberrant DNA methylation patterning was strongly associated with direct fusion protein binding as shown by the E2A-PBX1 chromatin immunoprecipitation (ChIP) sequencing (ChIP-seq), suggesting that E2A-PBX1 fusion protein directly remodels the epigenome to impose an aggressive B-ALL phenotype. MLLr B-ALL featured prominent cytosine hypomethylation, which was linked with MLL fusion protein binding, H3K79 dimethylation, and transcriptional upregulation, affecting a set of known and newly identified MLL fusion direct targets with oncogenic activity such as FLT3 and BCL6. Notably, BCL6 blockade or loss of function suppressed proliferation and survival of MLLr leukemia cells, suggesting BCL6-targeted therapy as a new therapeutic strategy for MLLr B-ALLs.
We conducted the first integrative epigenomic study in adult B-ALLs, as a correlative study to the ECOG E2993 phase III clinical trial. This study links for the first time the direct actions of oncogenic fusion proteins with disruption of epigenetic regulation mediated by cytosine methylation. We identify a novel clinically actionable biomarker in B-ALLs: IL2RA (CD25), which is linked with BCR-ABL1 and an inflammatory signaling network associated with chemotherapy resistance. We show that BCL6 is a novel MLL fusion protein target that is required to maintain the proliferation and survival of primary human adult MLLr cells and provide the basis for a clinical trial with BCL6 inhibitors for patients with MLLr.
遗传病变,如 BCR-ABL1、E2A-PBX1 和 MLL 重排(MLLr),与成人 B 细胞前体急性淋巴细胞白血病(B-ALL)的不良预后相关。白血病致癌蛋白可能直接或间接地破坏胞嘧啶甲基化模式,从而介导恶性表型。我们推测,这些侵袭性 B-ALL 中的 DNA 甲基化特征将指向疾病机制,并提供有用的生物标志物和治疗靶点。因此,我们对 215 名成年 B-ALL 患者进行了 DNA 甲基化和基因表达谱分析,这些患者均参与了一项单阶段 III 临床试验(ECOG E2993)和正常对照 B 细胞。在 BCR-ABL1 阳性的 B-ALL 中,异常的胞嘧啶甲基化模式以细胞因子网络为中心,其特征是 IL2RA(CD25)低甲基化和过表达。E2993 试验的临床数据表明,无论 BCR-ABL1 状态如何,CD25 表达与 ALL 患者的不良预后密切相关,提示 CD25 可作为 B-ALL 危险分层的新型预后生物标志物。在 E2A-PBX1 阳性的 B-ALL 中,异常的 DNA 甲基化模式与直接融合蛋白结合密切相关,这可以通过 E2A-PBX1 染色质免疫沉淀(ChIP)测序(ChIP-seq)显示出来,表明 E2A-PBX1 融合蛋白直接重塑表观基因组以施加侵袭性 B-ALL 表型。MLLr B-ALL 的特征是明显的胞嘧啶低甲基化,这与 MLL 融合蛋白结合、H3K79 二甲基化和转录上调有关,影响了一组已知和新发现的具有致癌活性的 MLL 融合直接靶标,如 FLT3 和 BCL6。值得注意的是,BCL6 阻断或功能丧失抑制了 MLLr 白血病细胞的增殖和存活,这表明 BCL6 靶向治疗是 MLLr B-ALL 的一种新的治疗策略。
我们对成人 B-ALL 进行了首次综合表观基因组学研究,这是 ECOG E2993 三期临床试验的一项相关性研究。该研究首次将致癌融合蛋白的直接作用与胞嘧啶甲基化介导的表观遗传调控的破坏联系起来。我们在 B-ALL 中确定了一个新的具有临床可操作性的生物标志物:IL2RA(CD25),它与 BCR-ABL1 相关,与化疗耐药相关的炎症信号网络相关。我们表明,BCL6 是一个新的 MLL 融合蛋白靶点,需要它来维持原代人成年 MLLr 细胞的增殖和存活,并为 MLLr 患者提供 BCL6 抑制剂临床试验的基础。
