在ETV6/RUNX1阳性淋巴白血病细胞中使用组蛋白去乙酰化酶抑制剂鉴定淋巴细胞生成中(ETV6)/RUNX1调控的基因。
The identification of (ETV6)/RUNX1-regulated genes in lymphopoiesis using histone deacetylase inhibitors in ETV6/RUNX1-positive lymphoid leukemic cells.
作者信息
Starkova Julia, Madzo Jozef, Cario Gunnar, Kalina Tomas, Ford Anthony, Zaliova Marketa, Hrusak Ondrej, Trka Jan
机构信息
Childhood Leukaemia Investigation Prague, Department of Paediatric Haematology/Oncology, 2nd Medical School, Charles University Prague, Prague, Czech Republic.
出版信息
Clin Cancer Res. 2007 Mar 15;13(6):1726-35. doi: 10.1158/1078-0432.CCR-06-2569. Epub 2007 Feb 26.
PURPOSE
Chimeric transcription factor ETV6/RUNX1 (TEL/AML1) is believed to cause pathologic block in lymphoid cell development via interaction with corepressor complex and histone deacetylase. We wanted to show the regulatory effect of ETV6/RUNX1 and its reversibility by histone deacetylase inhibitors (HDACi), as well as to identify potential ETV6/RUNX1-regulated genes.
EXPERIMENTAL DESIGN
We used luciferase assay to show the interaction of ETV6/RUNX1 protein, ETV6/RUNX1-regulated gene, and HDACi. To identify ETV6/RUNX1-regulated genes, we used expression profiling and HDACi in lymphoid cells. Next, using the flow cytometry and quantitative reverse transcription-PCR, we measured differentiation changes in gene and protein expression after HDACi treatment.
RESULTS
Luciferase assay showed repression of granzyme B expression by ETV6/RUNX1 protein and the reversibility of this effect by HDACi. Proving this regulatory role of ETV6/RUNX1, we identified, using complex statistical analysis, 25 genes that are potentially regulated by ETV6/RUNX1 protein. In four selected genes with known role in the cell cycle regulation (JunD, ACK1, PDGFRB, and TCF4), we confirmed expression changes after HDACi by quantitative analysis. After HDACi treatment, ETV6/RUNX1-positive cells showed immunophenotype changes resembling differentiation process compared with other leukemic cells (BCR/ABL, ETV6/PDGFRB positive). Moreover, ETV6/RUNX1-positive leukemic cells accumulated in G(1)-G(0) phase after HDACi whereas other B-lineage leukemic cell lines showed rather unspecific changes including induction of apoptosis and decreased proliferation.
CONCLUSIONS
Presented data support the hypothesis that HDACi affect ETV6/RUNX1-positive cells via direct interaction with ETV6/RUNX1 protein and that treatment with HDACi may release aberrant transcription activity caused by ETV6/RUNX1 chimeric transcription factor.
目的
嵌合转录因子ETV6/RUNX1(TEL/AML1)被认为通过与共抑制复合物和组蛋白去乙酰化酶相互作用导致淋巴细胞发育的病理性阻滞。我们想要展示ETV6/RUNX1的调节作用及其通过组蛋白去乙酰化酶抑制剂(HDACi)的可逆性,同时鉴定潜在的ETV6/RUNX1调节基因。
实验设计
我们使用荧光素酶测定法来展示ETV6/RUNX1蛋白、ETV6/RUNX1调节基因和HDACi之间的相互作用。为了鉴定ETV6/RUNX1调节基因,我们在淋巴细胞中使用了表达谱分析和HDACi。接下来,通过流式细胞术和定量逆转录PCR,我们测量了HDACi处理后基因和蛋白表达的分化变化。
结果
荧光素酶测定显示ETV6/RUNX1蛋白对颗粒酶B表达有抑制作用,且HDACi可使这种作用逆转。通过复杂的统计分析,我们鉴定出25个可能受ETV6/RUNX1蛋白调节来证明ETV6/RUNX1的这种调节作用。在四个选定的在细胞周期调节中具有已知作用的基因(JunD、ACK1、PDGFRB和TCF4)中,我们通过定量分析证实了HDACi处理后的表达变化。HDACi处理后,与其他白血病细胞(BCR/ABL、ETV6/PDGFRB阳性)相比,ETV6/RUNX1阳性细胞显示出类似于分化过程的免疫表型变化。此外,HDACi处理后,ETV6/RUNX1阳性白血病细胞在G(1)-G(0)期积累,而其他B系白血病细胞系则表现出相当非特异性的变化,包括诱导凋亡和增殖减少。
结论
现有数据支持以下假设,即HDACi通过与ETV6/RUNX1蛋白直接相互作用影响ETV6/RUNX1阳性细胞,并且用HDACi治疗可能释放由ETV6/RUNX1嵌合转录因子引起的异常转录活性。
Zotero 插件