Key Laboratory of Genomic and Precision Medicine, Collaborative Innovation Center of Genetics and Development, Beijing Institute of Genomics, Chinese Academy of Sciences, Beijing, China.
Division of Pathology and Experimental Hematology and Cancer Biology, Cincinnati Children's Hospital Medical Center, Cincinnati, OH, USA.
Leukemia. 2018 Apr;32(4):890-899. doi: 10.1038/leu.2017.339. Epub 2017 Nov 29.
Previously, we identified SETD2 loss-of-function mutations in 22% of MLL-rearranged (MLLr) acute leukemia patients, implicating a mechanism for cooperativity between SETD2 mutations and MLL fusions. However, the detailed mechanism of how SETD2-H3K36me3 downregulation accelerates MLLr leukemia remains unclear. Here, we show that in MLLr leukemia, both H3K79me2 and H3K36me3 are aberrantly elevated and co-enriched in a group of genes. SETD2 inactivation leads to a global reduction of H3K36me3 and a further elevation of H3K79me2, but does not change the expression of known MLL fusion target genes. Instead, this pattern of histone changes is associated with transcriptional deregulation of a novel set of genes; downregulating tumor suppressors (for example, ASXL1) and upregulating oncogenes (for example, ERG). Taken together, our findings reveal a global crosstalk between the oncogenic DOT1L-H3K79me2 axis and the tumor suppressive SETD2-H3K36me3 axis in gene regulation, provide molecular insights into how SETD2 mutations accelerate MLLr leukemogenesis through differential regulation of additional tumor suppressors and oncogenes.
此前,我们在 22%的 MLL 重排(MLLr)急性白血病患者中发现 SETD2 功能丧失突变,提示 SETD2 突变与 MLL 融合之间存在协同作用的机制。然而,SETD2-H3K36me3 下调如何加速 MLLr 白血病的确切机制仍不清楚。在这里,我们表明在 MLLr 白血病中,H3K79me2 和 H3K36me3 都异常升高,并在一组基因中共富集。SETD2 失活导致 H3K36me3 的全面减少和 H3K79me2 的进一步升高,但不改变已知 MLL 融合靶基因的表达。相反,这种组蛋白变化模式与一组新的基因转录失调相关;下调肿瘤抑制因子(例如,ASXL1)和上调癌基因(例如,ERG)。总之,我们的研究结果揭示了致癌 DOT1L-H3K79me2 轴与肿瘤抑制 SETD2-H3K36me3 轴在基因调控中的全局串扰,为 SETD2 突变如何通过对其他肿瘤抑制因子和癌基因的差异调节加速 MLLr 白血病发生提供了分子见解。