Fan Wenjun, Liu Hester, Stachelek Gregory C, Begum Asma, Davis Catherine E, Dorado Tony E, Ernst Glen, Reinhold William C, Ozbek Busra, Zheng Qizhi, De Marzo Angelo M, Rajeshkumar N V, Barrow James C, Laiho Marikki
bioRxiv. 2024 Aug 16:2024.08.15.608201. doi: 10.1101/2024.08.15.608201.
Ribosome biosynthesis is a cancer vulnerability executed by targeting RNA polymerase I (Pol I) transcription. We developed advanced, specific Pol I inhibitors to identify drivers of this sensitivity. By integrating multi-omics features and drug sensitivity data from a large cancer cell panel, we discovered that frameshift mutation conferred Pol I inhibitor sensitivity in microsatellite instable cancers. Mechanistically, RPL22 directly interacts with 28S rRNA and mRNA splice junctions, functioning as a splicing regulator. RPL22 deficiency, intensified by 28S rRNA sequestration, promoted the splicing of its paralog RPL22L1 and p53 negative regulator MDM4. Chemical and genetic inhibition of rRNA synthesis broadly remodeled mRNA splicing controlling hundreds of targets. Strikingly, RPL22-dependent alternative splicing was reversed by Pol I inhibition revealing a ribotoxic stress-initiated tumor suppressive pathway. We identify a mechanism that robustly connects rRNA synthesis activity to splicing and reveals their coordination by ribosomal protein RPL22.
核糖体生物合成是一种通过靶向RNA聚合酶I(Pol I)转录而产生的癌症脆弱性。我们开发了先进的、特异性的Pol I抑制剂,以确定这种敏感性的驱动因素。通过整合来自大型癌细胞系的多组学特征和药物敏感性数据,我们发现移码突变在微卫星不稳定癌症中赋予了Pol I抑制剂敏感性。从机制上讲,RPL22直接与28S rRNA和mRNA剪接接头相互作用,作为一种剪接调节因子发挥作用。28S rRNA隔离加剧了RPL22缺陷,促进了其旁系同源物RPL22L1和p53负调节因子MDM4的剪接。rRNA合成的化学和基因抑制广泛重塑了控制数百个靶点的mRNA剪接。引人注目的是,Pol I抑制逆转了RPL22依赖性可变剪接,揭示了一种核糖体毒性应激引发的肿瘤抑制途径。我们确定了一种机制,该机制有力地将rRNA合成活性与剪接联系起来,并揭示了核糖体蛋白RPL22对它们的协调作用。
