Multiplex immunofluorescence and single‐cell transcriptomic profiling reveal the spatial cell interaction networks in the non‐small cell lung cancer microenvironment

Background Conventional immunohistochemistry technologies were limited by the inability to simultaneously detect multiple markers and the lack of identifying spatial relationships among cells, hindering understanding of the biological processes in cancer immunology. Methods Tissue slices of primary...

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Published in:Clinical and translational medicine 2023-01, Vol.13 (1), p.e1155-n/a
Main Authors: Peng, Haoxin, Wu, Xiangrong, Liu, Shaopeng, He, Miao, Xie, Chao, Zhong, Ran, Liu, Jun, Tang, Chenshuo, Li, Caichen, Xiong, Shan, Zheng, Hongbo, He, Jianxing, Lu, Xu, Liang, Wenhua
Format: Article
Language:English
Subjects:
Antibodies
Cancer therapies
Carcinoma, Non-Small-Cell Lung - genetics
Carcinoma, Non-Small-Cell Lung - pathology
cell interaction networks
Cells
Clinical medicine
Deep learning
deep learning algorithm
Fluorescent Antibody Technique
Humans
Lung cancer
Lung Neoplasms - pathology
multiplex immunofluorescence
Patients
Proteins
single‐cell RNA sequencing
Thoracic surgery
Transcriptome
Tumor Microenvironment - genetics
Tumors
tumour microenvironment
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Summary:Background Conventional immunohistochemistry technologies were limited by the inability to simultaneously detect multiple markers and the lack of identifying spatial relationships among cells, hindering understanding of the biological processes in cancer immunology. Methods Tissue slices of primary tumours from 553 IA∼IIIB non‐small cell lung cancer (NSCLC) cases were stained by multiplex immunofluorescence (mIF) assay for 10 markers, including CD4, CD38, CD20, FOXP3, CD66b, CD8, CD68, PD‐L1, CD133 and CD163, evaluating the amounts of 26 phenotypes of cells in tumour nest and tumour stroma. StarDist depth learning model was utilised to determine the spatial location of cells based on mIF graphs. Single‐cell RNA sequencing (scRNA‐seq) on four primary NSCLC cases was conducted to investigate the putative cell interaction networks. Results Spatial proximity among CD20+ B cells, CD4+ T cells and CD38+ T cells (r2 = 0.41) was observed, whereas the distribution of regulatory T cells was associated with decreased infiltration levels of CD20+ B cells and CD38+ T cells (r2 = −0.45). Univariate Cox analyses identified closer proximity between CD8+ T cells predicted longer disease‐free survival (DFS). In contrast, closer proximity between CD133+ cancer stem cells (CSCs), longer distances between CD4+ T cells and CD20+ B cells, CD4+ T cells and neutrophils, and CD20+ B cells and neutrophils were correlated with dismal DFS. Data from scRNA‐seq further showed that spatially adjacent N1‐like neutrophils could boost the proliferation and activation of T and B lymphocytes, whereas spatially neighbouring M2‐like macrophages showed negative effects. An immune‐related risk score (IRRS) system aggregating robust quantitative and spatial prognosticators showed that high‐IRRS patients had significantly worse DFS than low‐IRRS ones (HR 2.72, 95% CI 1.87–3.94, p 
ISSN:2001-1326
2001-1326
DOI:10.1002/ctm2.1155