Su Guomiao, Wang Juan, Liu Shiyue, Fu Xiaonan, Li Yanxi, Pan Guoqing
Department of Pathology, The First Affiliated Hospital of Kunming Medical University, Kunming, Yun Nan, People's Republic of China.
Clinical Laboratory, Yunnan Province Third People's Hospital, Kunming, Yun Nan, People's Republic of China.
Int J Gen Med. 2024 Dec 30;17:6567-6584. doi: 10.2147/IJGM.S496006. eCollection 2024.
To identify the epithelial cell centre regulatory transcription factors in the gastric cancer (GC) microenvironment and provide a new strategy for the diagnosis and treatment of GC.
The GC single-cell dataset was downloaded from the Gene Expression Omnibus (GEO) database. The regulatory mechanisms of transcription factors in both pan-cancer and GC microenvironments were analysed using the Cancer Genome Atlas (TGCA) database. Real-time quantitative PCR (RT-qPCR) was used to determine the mRNA expression levels of Prospero homeobox gene 1 (PROX1) and Endothelial PAS domain-containing protein 1 (EPAS1) in the human gastric mucosal normal epithelial cell line (GES-1) and the GC cell line (AGS). Immunohistochemistry (IHC) was used to determine the amounts of PROX1 and EPAS1 protein expression in GC and adjacent tissues. GC patients' overall survival (OS) was tracked through outpatient, Inpatient case inquiry, or phone follow-up.
The single-cell data from GSE184198 was re-annotated, resulting in nine cell subsets: T cells (13364), NK cells (606), B cells (2525), Epithelial cells (2497), DC cells (1167), Fibroblast cells (372), Endothelial cells (271), Neutrophils cells (246) and Macrophage cells (420). Analysis of cell subgroup signalling pathways revealed that communication intensity between epithelial cells and smooth muscle cells was highest. Transcription factors and were notably active in epithelial cells. Cell communication analysis indicated that IFNG may interact with IFNGR1/2 and LIF with IL6ST and LIFR to regulate the downstream and and were upregulated and negatively correlated with tumour mutation burden (TMB). also exhibited high positive correlations with immune checkpoints CTLA4 and PDCD1LG2, as well as with chemokines CCL24 and CXCL12 and their receptors CCR3 and CCR4. Additionally, and were positively correlated with immunosuppressive factors ADORA2A, CD160, IL10, TGFBR1, KDR and CSF1R, as well as with immunostimulators CD276, PVR, TNFRSF25, ULBP1, CXCL12 and ENTPD1. In GC tissues and AGS, PROX1 and EPAS1 were both substantially expressed. In the meantime, they showed a positive correlation with clinicopathological features such TNM stage and degree of differentiation. In GC patients, the up-regulated group's PROX1 and EPAS1 prognosis was noticeably poorer than the down-regulated group's.
and are likely central regulatory transcription factors in the epithelial cells of the GC environment, regulated by IFNG and LIF. They may contribute to GC progression by modulating the tumour's immune microenvironment.
鉴定胃癌(GC)微环境中的上皮细胞中心调节转录因子,为GC的诊断和治疗提供新策略。
从基因表达综合数据库(GEO)下载GC单细胞数据集。利用癌症基因组图谱(TGCA)数据库分析泛癌和GC微环境中转录因子的调控机制。采用实时定量聚合酶链反应(RT-qPCR)检测人胃黏膜正常上皮细胞系(GES-1)和GC细胞系(AGS)中Prospero同源框基因1(PROX1)和含内皮PAS结构域蛋白1(EPAS1)的mRNA表达水平。采用免疫组织化学(IHC)检测GC及癌旁组织中PROX1和EPAS1蛋白表达量。通过门诊、住院病例查询或电话随访追踪GC患者的总生存期(OS)。
对GSE184198的单细胞数据进行重新注释,得到9个细胞亚群:T细胞(13364个)、自然杀伤细胞(NK细胞,606个)、B细胞(2525个)、上皮细胞(2497个)、树突状细胞(DC细胞,1167个)、成纤维细胞(372个)、内皮细胞(271个)、中性粒细胞(246个)和巨噬细胞(420个)。细胞亚群信号通路分析显示上皮细胞与平滑肌细胞之间的通讯强度最高。转录因子[具体转录因子未给出名称]在上皮细胞中显著活跃。细胞通讯分析表明,IFNG可能与IFNGR1/2相互作用,LIF与IL6ST和LIFR相互作用,以调节下游[具体内容未给出],[具体转录因子未给出名称]上调且与肿瘤突变负荷(TMB)呈负相关。[具体转录因子未给出名称]还与免疫检查点CTLA4和PDCD1LG2以及趋化因子CCL24和CXCL12及其受体CCR3和CCR4呈高度正相关。此外,[具体转录因子未给出名称]与免疫抑制因子ADORA2A、CD160、IL10、TGFBR1、KDR和CSF1R以及免疫刺激因子CD276、PVR、TNFRSF25、ULBP1、CXCL12和ENTPD1呈正相关。在GC组织和AGS中,PROX1和EPAS1均大量表达。同时,它们与TNM分期和分化程度等临床病理特征呈正相关。在GC患者中,PROX1和EPAS1上调组的预后明显比下调组差。
[具体转录因子未给出名称]可能是GC环境上皮细胞中的核心调节转录因子,受IFNG和LIF调控。它们可能通过调节肿瘤免疫微环境促进GC进展。
