Histone Modifier Differentially Regulates Gene Expression and Unravels Survival Role of MicroRNA-494 in Jurkat Leukemia.

MicroRNA (Shariqah, United Arab Emirates) Pub Date : 2021-01-01 DOI:10.2174/2211536610666210412153322

Arathi Jayaraman, Tong Zhou, Sundararajan Jayaraman

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引用次数: 2

Abstract

Background: Although the protein-coding genes are subject to histone hyperacetylation- mediated regulation, it is unclear whether microRNAs are similarly regulated in the T cell leukemia Jurkat.

Objective: To determine whether treatment with the histone modifier Trichostatin A could concurrently alter the expression profiles of microRNAs and protein-coding genes.

Methods: Changes in histone hyperacetylation and viability in response to drug treatment were analyzed, respectively, using western blotting and flow cytometry. Paired global expression profiling of microRNAs and coding genes was performed and highly regulated genes have been validated by qRT-PCR. The interrelationships between the drug-induced miR-494 upregulation, the expression of putative target genes, and T cell receptor-mediated apoptosis were evaluated using qRT-PCR, flow cytometry, and western blotting following lipid-mediated transfection with specific anti-microRNA inhibitors.

Results: Treatment of Jurkat cells with Trichostatin A resulted in histone hyperacetylation and apoptosis. Global expression profiling indicated prominent upregulation of miR-494 in contrast to differential regulation of many protein-coding and non-coding genes validated by qRT-PCR. Although transfection with synthetic anti-miR-494 inhibitors failed to block drug-induced apoptosis or miR-494 upregulation, it induced the transcriptional repression of the PVRIG gene. Surprisingly, miR-494 inhibition in conjunction with low doses of Trichostatin A enhanced the weak T cell receptor- mediated apoptosis, indicating a subtle pro-survival role of miR-494. Interestingly, this prosurvival effect was overwhelmed by mitogen-mediated T cell activation and higher drug doses, which mediated caspase-dependent apoptosis.

Conclusion: Our results unravel a pro-survival function of miR-494 and its putative interaction with the PVRIG gene and the apoptotic machinery in Jurkat cells.

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组蛋白修饰因子差异调控Jurkat白血病MicroRNA-494基因表达及生存作用

背景:虽然蛋白质编码基因受到组蛋白超乙酰化介导的调控，但尚不清楚microrna是否在T细胞白血病Jurkat中受到类似的调控。目的:探讨组蛋白修饰剂曲古霉素A治疗是否能同时改变microrna和蛋白编码基因的表达谱。方法:采用western blotting和流式细胞术分别分析药物治疗后组蛋白超乙酰化和活力的变化。对microrna和编码基因进行了配对的全球表达谱分析，并通过qRT-PCR验证了高度调控的基因。在脂质介导转染特异性抗microrna抑制剂后，使用qRT-PCR、流式细胞术和western blotting评估药物诱导的miR-494上调、推测靶基因表达和T细胞受体介导的凋亡之间的相互关系。结果:曲古抑素A处理Jurkat细胞导致组蛋白超乙酰化和细胞凋亡。全球表达谱显示miR-494显著上调，而qRT-PCR证实了许多蛋白质编码和非编码基因的差异调控。虽然转染合成的抗miR-494抑制剂不能阻断药物诱导的细胞凋亡或miR-494上调，但可以诱导PVRIG基因的转录抑制。令人惊讶的是，miR-494抑制与低剂量曲古抑素A联合可增强弱T细胞受体介导的细胞凋亡，表明miR-494具有微妙的促生存作用。有趣的是，这种促进生存的作用被丝裂原介导的T细胞活化和更高的药物剂量所掩盖，后者介导了caspase依赖性的细胞凋亡。结论:我们的研究结果揭示了miR-494的促存活功能及其与PVRIG基因和Jurkat细胞凋亡机制的相互作用。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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MicroRNA (Shariqah, United Arab Emirates) Medicine-Medicine (all)

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