Kim Min-Ah, Kim Banseok, Jeon Jihyeon, Lee Jonghyun, Jang Hyeji, Baek Minjae, Seo Sang-Uk, Shin Dongkwan, Dutta Anindya, Lee Kyung Yong
Research Institute, National Cancer Center, Goyang-Si, Gyeonggi-Do, 10408, Republic of Korea.
Department of Microbiology, College of Medicine, The Catholic University of Korea, Seoul, 06591, Republic of Korea.
Mol Med. 2025 Jan 22;31(1):18. doi: 10.1186/s10020-025-01066-z.
Double-strand breaks (DSBs) are primarily repaired through non-homologous end joining (NHEJ) and homologous recombination (HR). Given that DSBs are highly cytotoxic, PARP inhibitors (PARPi), a prominent class of anticancer drugs, are designed to target tumors with HR deficiency (HRD), such as those harboring BRCA mutations. However, many tumor cells acquire resistance to PARPi, often by restoring HR in HRD cells through the inactivation of NHEJ. Therefore, identifying novel regulators of NHEJ could provide valuable insights into the mechanisms underlying PARPi resistance.
Cellular DSBs were assessed using neutral comet assays and phospho-H2AX immunoblotting. Fluorescence-based reporter assays quantified repair via NHEJ or HR. The recruitment of proteins that promote NHEJ and HR to DSBs was analyzed using immunostaining, live-cell imaging following laser-induced microirradiation, and FokI-inducible single DSB generation. Loss-of-function experiments were performed in multiple human cancer cell lines using siRNA-mediated knockdown or CRISPR-Cas9 gene knockout. Cell viability assays were conducted to evaluate resistance to PARP inhibitors. Additionally, bioinformatic analyses of public databases were performed to investigate the association between TLK expression and BRCA1 status.
We demonstrate that human tousled-like kinase (TLK) orthologs are essential for NHEJ-mediated repair of DSBs and for PARPi sensitivity in cells with BRCA1 mutation. TLK1 and TLK2 exhibit redundant roles in promoting NHEJ, and their deficiency results in a significant accumulation of DSBs. TLKs are required for the proper localization of 53BP1, a key factor in promoting the NHEJ pathway. Consequently, TLK deficiency induces PARPi resistance in triple-negative breast cancer (TNBC) and ovarian cancer (OVCA) cell lines with BRCA1 deficiency, as TLK deficiency in BRCA1-depleted cells, impairs 53BP1 recruitment to DSBs and reduces NHEJ efficiency, while restoring HR.
We have identified TLK proteins as novel regulators of NHEJ repair and PARPi sensitivity in BRCA1-depleted cells, suggesting that TLK repression may represent a previously unrecognized mechanism by which BRCA1 mutant cancers acquire PARPi resistance.
双链断裂(DSB)主要通过非同源末端连接(NHEJ)和同源重组(HR)进行修复。鉴于DSB具有高度细胞毒性,聚(ADP-核糖)聚合酶抑制剂(PARPi)作为一类重要的抗癌药物,旨在靶向具有HR缺陷(HRD)的肿瘤,例如那些携带BRCA突变的肿瘤。然而,许多肿瘤细胞会对PARPi产生耐药性,通常是通过使NHEJ失活来恢复HRD细胞中的HR。因此,鉴定NHEJ的新型调节因子可以为PARPi耐药的潜在机制提供有价值的见解。
使用中性彗星试验和磷酸化H2AX免疫印迹评估细胞DSB。基于荧光的报告基因试验定量通过NHEJ或HR的修复。使用免疫染色、激光诱导微辐射后的活细胞成像以及FokI诱导的单个DSB生成,分析促进NHEJ和HR的蛋白质向DSB的募集。在多种人类癌细胞系中使用siRNA介导的敲低或CRISPR-Cas9基因敲除进行功能丧失实验。进行细胞活力试验以评估对PARP抑制剂的耐药性。此外,对公共数据库进行生物信息学分析,以研究TLK表达与BRCA1状态之间的关联。
我们证明人类类紊乱激酶(TLK)直系同源物对于NHEJ介导的DSB修复以及对具有BRCA1突变的细胞中的PARPi敏感性至关重要。TLK1和TLK2在促进NHEJ方面表现出冗余作用,它们的缺陷导致DSB的显著积累。TLK是促进NHEJ途径的关键因子53BP1正确定位所必需的。因此,TLK缺陷会在具有BRCA1缺陷的三阴性乳腺癌(TNBC)和卵巢癌(OVCA)细胞系中诱导PARPi耐药性,因为BRCA1缺失细胞中的TLK缺陷会损害53BP1向DSB的募集并降低NHEJ效率,同时恢复HR。
我们已将TLK蛋白鉴定为BRCA1缺失细胞中NHEJ修复和PARPi敏感性的新型调节因子,表明TLK抑制可能代表BRCA1突变癌症获得PARPi耐药性的一种先前未被认识的机制。
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