一个RNA结合蛋白组对调节肝细胞癌中RSPO-LGR4/5-ZNRF3/RNF43模块及免疫微环境的影响

The impact of an RNA-binding protein group on regulating the RSPO-LGR4/5-ZNRF3/RNF43 module and the immune microenvironment in hepatocellular carcinoma.

作者信息

Xie Zhengyao, Dai Zhiyan, Liu Ziyao, Chen Yiqiang, Huang Shuting, Liu Siyuan, Li Jingjing, Shen Jie

机构信息

Department of Precision Medicine, Affiliated Hospital of Medical School, Nanjing Drum Tower Hospital, Nanjing University, Nanjing, China.

Comprehensive Cancer Centre, Department of Oncology, Affiliated Hospital of Medical School, Nanjing Drum Tower Hospital, Nanjing University, Nanjing, China.

出版信息

BMC Cancer. 2025 Apr 22;25(1):751. doi: 10.1186/s12885-025-13874-x.

DOI:10.1186/s12885-025-13874-x

PMID:40264052

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12012940/

Abstract

BACKGROUND

Hepatocellular carcinoma (HCC) is a leading cause of cancer mortality. RNA-binding proteins (RBPs) are potential therapeutic targets because of their role in tumor progression. This study investigated the interactions between specific HCC progression-associated RBPs (HPARBPs), namely, ILF3, PTBP1, U2AF2, NCBP2, RPS3, and SSB, in HCC and their downstream targets, as well as their impact on the immune microenvironment and their clinical value.

METHODS

Tissue samples from human HCC, collected from 28 patients who experienced recurrence following postoperative adjuvant therapy were examined. The mRNA levels of RBPs and their prospective targets were quantified through RNA isolation and quantitative real-time PCR. Data from two public datasets were scrutinized for both expression and clinical relevance. Through Student's t test and logistic regression, HPARBPs were identified. Enhanced cross-linking immunoprecipitation (eCLIP) experiments revealed RBP-RNA interactions in HepG2 cells. For functional enrichment, Metascape was used, whereas CIBERSORT was used to characterize the immune microenvironment.

RESULTS

Public database analysis confirmed widespread RBP expression abnormalities in HCC (false discovery rate < 0.00001 and fold change ≥ 1.15 or ≤ 0.85), leading to the identification of 42 HPARBPs and core modules. eCLIP data analysis revealed the specificity of downstream target genes and binding site features for core HPARBPs (signal value > 3, P value < 0.01). Four core HPARBPs may bind to RNAs of genes in the RSPO-LGR4/5-ZNRF3/RNF43 module, affecting the Wnt pathway and HCC progression. Immunoinfiltration analysis revealed changes in the HCC immune microenvironment due to altered expression of relevant genes.

CONCLUSION

In our study, we identified core HPARBPs that might contribute to HCC progression by binding to RNAs in the RSPO-LGR4/5-ZNRF3/RNF43 module. Changes in the expression of HPARBPs affect the HCC immune microenvironment. Our findings offer novel insights into the regulatory network of Wnt pathway-related RBPs and their potential clinical value in HCC.

摘要

背景

肝细胞癌（HCC）是癌症死亡的主要原因。RNA结合蛋白（RBPs）因其在肿瘤进展中的作用而成为潜在的治疗靶点。本研究调查了特定的与HCC进展相关的RBPs（HPARBPs），即白细胞介素增强子结合因子3（ILF3）、多嘧啶结合蛋白1（PTBP1）、U2辅助因子2（U2AF2）、核帽结合蛋白2（NCBP2）、核糖体蛋白S3（RPS3）和小核糖体蛋白B（SSB），在HCC中的相互作用及其下游靶点，以及它们对免疫微环境的影响及其临床价值。

方法

对28例术后辅助治疗后复发的患者的人HCC组织样本进行检查。通过RNA分离和定量实时PCR对RBPs及其潜在靶点的mRNA水平进行定量。对两个公共数据集的数据进行表达和临床相关性审查。通过学生t检验和逻辑回归，确定HPARBPs。增强交联免疫沉淀（eCLIP）实验揭示了HepG2细胞中的RBP-RNA相互作用。使用Metascape进行功能富集，而使用CIBERSORT来表征免疫微环境。

结果

公共数据库分析证实HCC中广泛存在RBP表达异常（错误发现率<0.00001，倍数变化≥1.15或≤0.85），从而确定了42个HPARBPs和核心模块。eCLIP数据分析揭示了核心HPARBPs下游靶基因的特异性和结合位点特征（信号值>3，P值<0.01）。四个核心HPARBPs可能与RSPO-LGR4/5-ZNRF3/RNF43模块中的基因RNA结合，影响Wnt通路和HCC进展。免疫浸润分析揭示了由于相关基因表达改变导致的HCC免疫微环境变化。