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Single-cell RNA sequencing of liver fine-needle aspirates captures immune diversity in the blood and liver in chronic hepatitis B patients

免疫系统 医学 免疫学 丙型肝炎病毒 乙型肝炎 乙型肝炎病毒 人口 免疫 病毒 环境卫生
作者
Alex S. Genshaft,Sonu Subudhi,Arlin Keo,Juan D. Sanchez Vasquez,Nádia Conceição-Neto,Deeqa Mahamed,Lauke L. Boeijen,Nadia Alatrakchi,Chris Oetheimer,Mike Vilme,Riley S. Drake,Ira Fleming,Nancy Tran,Constantine N. Tzouanas,Jasmin Joseph-Chazan,Martin Arreola Villanueva,Harmen J.G. van de Werken,Gertine W. van Oord,Zwier M. A. Groothuismink,Boris J.B. Beudeker,Z. Osmani,Shirin Nkongolo,Aman Mehrotra,Kurt Spittaels,Jordan J. Feld,Raymond T. Chung,Robert J. de Knegt,Harry L.A. Janssen,Jeroen Aerssens,Jacques Bollekens,Nir Hacohen,Georg M. Lauer,André Boonstra,Alex K. Shalek,Adam J. Gehring
出处
期刊:Hepatology [Wiley]
卷期号:Publish Ahead of Print 被引量:4
标识
DOI:10.1097/hep.0000000000000438
摘要

Background: Hepatitis B virus (HBV) infection is restricted to the liver where it drives exhaustion of virus-specific T and B cells and pathogenesis through dysregulation of intrahepatic immunity. Our understanding of liver-specific events related to viral control and liver damage have relied almost solely on animal models and we lack useable peripheral biomarkers to quantify intrahepatic immune activation beyond cytokine measurement. Our objective was to overcome practical obstacles of liver sampling using fine-needle aspiration (FNA) and develop an optimized workflow to comprehensively compare the blood and liver compartments within chronic hepatitis B (CHB) patients using single-cell RNA sequencing (scRNAseq). Methods: We developed a workflow that enabled multi-site international studies and centralized scRNAseq. Blood and liver FNAs were collected, and cellular and molecular capture were compared between the Seq-Well S3 picowell-based and the 10x Chromium reverse-emulsion droplet-based scRNAseq technologies. Results: Both technologies captured the cellular diversity of the liver but Seq-Well S3 effectively captured neutrophils, which were absent in the 10x dataset. CD8 T cells and neutrophils displayed distinct transcriptional profiles between blood and liver. In addition, liver FNAs captured a heterogeneous liver macrophage population. Comparison between untreated CHB patients and patients treated with nucleoside analogues showed that myeloid cells were highly sensitive to environmental changes while lymphocytes displayed minimal differences. Conclusion: The ability to electively sample and intensively profile the immune landscape of the liver, and generate high-resolution data, will enable multi-site clinical studies to identify biomarkers for intrahepatic immune activity in HBV and beyond. Export
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