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RNA 剪接因子 Rbm25 是小鼠异质性前白血病克隆扩增的基础。

RNA splicing factor Rbm25 underlies heterogeneous preleukemic clonal expansion in mice.

机构信息

Department of Stem Cell Biology and Regenerative Medicine, Eli and Edythe Broad Center for Regenerative Medicine and Stem Cell Research, Keck School of Medicine, University of Southern California, Los Angeles, CA.

出版信息

Blood. 2023 Jun 15;141(24):2961-2972. doi: 10.1182/blood.2023019620.

Abstract

Clonal expansion sets the stage for cancer genesis by allowing for the accumulation of molecular alterations. Although genetic mutations such as Tet2 that induce clonal expansion and malignancy have been identified, these mutations are also frequently found in healthy individuals. Here, we tracked preleukemic clonal expansion using genetic barcoding in an inducible Tet2 knockout mouse model and found that only a small fraction of hematopoietic stem cells (HSCs) expanded excessively upon Tet2 knockout. These overexpanded HSCs expressed significantly lower levels of genes associated with leukemia and RNA splicing than nonoverexpanded Tet2 knockout HSCs. Knocking down Rbm25, an identified RNA splicing factor, accelerated the expansion of Tet2-knockout hematopoietic cells in vitro and in vivo. Our data suggest that mutations of an epigenetic factor Tet2 induce variability in the expression of an RNA splicing factor Rbm25, which subsequently drives heterogeneous preleukemic clonal expansion. This heterogeneous clonal expansion could contribute to the variable disease risks across individuals.

摘要

克隆扩增为癌症发生奠定了基础,允许分子改变的积累。虽然已经确定了 Tet2 等诱导克隆扩增和恶性肿瘤的基因突变,但这些突变也经常在健康个体中发现。在这里,我们使用遗传条形码在诱导型 Tet2 敲除小鼠模型中跟踪白血病前克隆扩增,发现只有一小部分造血干细胞 (HSC) 在 Tet2 敲除后过度扩增。与非过度扩增的 Tet2 敲除 HSC 相比,这些过度扩增的 HSC 表达与白血病和 RNA 剪接相关的基因水平明显降低。敲低鉴定出的 RNA 剪接因子 Rbm25 可加速 Tet2 敲除造血细胞在体外和体内的扩增。我们的数据表明,表观遗传因子 Tet2 的突变诱导 RNA 剪接因子 Rbm25 的表达变异性,随后驱动异质性白血病前克隆扩增。这种异质性克隆扩增可能导致个体间疾病风险的变化。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/92f9/10315624/537c4a519ae9/BLOOD_BLD-2023-019620-fx1.jpg

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