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Molecular heterogeneity unravelled by single‐cell transcriptomics in patients with essential thrombocythaemia

人口 生物 转录组 遗传学 索引 遗传异质性 表型 医学 计算生物学 基因 单核苷酸多态性 基因型 基因表达 环境卫生
作者
Chia‐Chen Hsu,Ying‐Ju Chen,Cih‐En Huang,Yuying Wu,Ming-Chung Wang,Sung‐Nan Pei,Chun‐Kai Liao,Chang‐Hsien Lu,Ping‐Tsung Chen,Hsing-Yi Tsou,Chian-Pei Li,Wei-Hsuan Chuang,Ching-Kai Chuang,Cheng‐Yu Yang,Yi-Hua Lai,Yi‐Hsuan Lin,Chih‐Cheng Chen
出处
期刊:British Journal of Haematology [Wiley]
卷期号:188 (5): 707-722 被引量:2
标识
DOI:10.1111/bjh.16225
摘要

Summary Significant phenotypic heterogeneity exists in patients with all subtypes of myeloproliferative neoplasms (MPN), including essential thrombocythaemia (ET). Single‐cell RNA sequencing (scRNA‐Seq) holds the promise of unravelling the biology of MPN at an unprecedented level of resolution. Herein we employed this approach to dissect the transcriptomes in the CD34 + cells from the peripheral blood of seven previously untreated ET patients and one healthy adult. The mutational profiles in these patients were as follows: JAK2 V617F in two, CALR in three (one type I and two type II) and triple‐negative (TN) in two. Our results reveal substantial heterogeneity within this enrolled cohort of patients. Activation of JAK/STAT signalling was recognized in discrepant progenitor lineages among different samples. Significantly disparate molecular profiling was identified in the comparison between ET patients and the control, between patients with different driver mutations ( JAK2 V617F and CALR exon 9 indel), and even between patients harbouring the same driver. Intra‐individual clonal diversity was also found in the CD34 + progenitor population of a patient, possibly indicating the presence of multiple clones in this case. Estimation of subpopulation size based on cellular immunophenotyping suggested differentiation bias in all analysed samples. Furthermore, combining the transcriptomic information with data from targeted sequencing enabled us to unravel key somatic mutations that are molecularly relevant. To conclude, we demonstrated that scRNA‐Seq extended our knowledge of clonal diversity and inter‐individual heterogeneity in patients with ET. The obtained information could potentially leapfrog our efforts in the elucidation of the pathogenesis of the disease.
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