Elgehama Ahmed M, Yang Qian, He Zaoke, Ruegg Lauryn, You Sungyong, Yang Wei
bioRxiv. 2025 May 5:2025.04.30.651490. doi: 10.1101/2025.04.30.651490.
Receptor-interacting protein kinase 2 (RIPK2) has emerged as a promising drug target in various cancers, including prostate cancer (PC). However, the absence of reliable biomarkers to assess RIPK2 activity limits both patient selection for anti-RIPK2 therapies and treatment monitoring. To address this gap, we performed RNA-Seq analysis on PC cell lines (22Rv1, DU145, and PC3) with CRISPR/Cas9-mediated knockout ( -KO) using two independent guide RNAs. This analysis identified 13 candidate RIPK2-regulated genes, of which eight were validated by reverse transcription quantitative PCR (RT-qPCR). Furthermore, treatment with two distinct RIPK2 inhibitors significantly reduced RIPK2 signature scores in five independent PC cell lines in a dose- and/or time-dependent manner. Clinical association analyses revealed that high RIPK2 signature scores correlate with metastasis and worse biochemical recurrence-free, progression-free, disease-free, and overall survival, outperforming RIPK2 mRNA levels as a prognostic biomarker. This study establishes, for the first time, a RIPK2-regulated gene signature as a potential biomarker for RIPK2 activity and PC prognosis, warranting further validation in clinical specimens to provide a much-needed tool for patient stratification and response monitoring in RIPK2-targeted therapies.
受体相互作用蛋白激酶2(RIPK2)已成为包括前列腺癌(PC)在内的多种癌症中一个有前景的药物靶点。然而,缺乏可靠的生物标志物来评估RIPK2活性限制了抗RIPK2疗法的患者选择和治疗监测。为了填补这一空白,我们使用两个独立的引导RNA,对经CRISPR/Cas9介导敲除(-KO)的前列腺癌细胞系(22Rv1、DU145和PC3)进行了RNA测序分析。该分析确定了13个RIPK2调控的候选基因,其中8个通过逆转录定量PCR(RT-qPCR)得到验证。此外,用两种不同的RIPK2抑制剂处理以剂量和/或时间依赖性方式显著降低了五个独立前列腺癌细胞系中的RIPK2特征评分。临床关联分析显示,高RIPK2特征评分与转移以及更差的生化无复发生存、无进展生存、无病生存和总生存相关,作为一种预后生物标志物,其表现优于RIPK2 mRNA水平。本研究首次建立了RIPK2调控的基因特征作为RIPK2活性和前列腺癌预后的潜在生物标志物,需要在临床标本中进一步验证,以为RIPK2靶向治疗中的患者分层和反应监测提供急需的工具。
