Single-cell genomic and transcriptomic landscapes of primary and metastatic colorectal cancer tumors

癌症研究 克拉斯 桑格测序 结直肠癌 生物 转录组 癌症 癌变 外显子组测序 外显子组 突变 遗传学 基因 基因表达
作者
Rui Wang,Jingyun Li,Xin Zhou,Yunuo Mao,Wendong Wang,Shuai Gao,Wei Wang,Yuan Gao,Kexuan Chen,Shuntai Yu,Xinglong Wu,Lu Wen,Hao Ge,Wei Fu,Fuchou Tang
出处
期刊:Genome Medicine [Springer Nature]
卷期号:14 (1) 被引量:33
标识
DOI:10.1186/s13073-022-01093-z
摘要

Abstract Background Colorectal cancer (CRC) ranks as the second-leading cause of cancer-related death worldwide with metastases being the main cause of cancer-related death. Here, we investigated the genomic and transcriptomic alterations in matching adjacent normal tissues, primary tumors, and metastatic tumors of CRC patients. Methods We performed whole genome sequencing (WGS), multi-region whole exome sequencing (WES), simultaneous single-cell RNA-Seq, and single-cell targeted cDNA Sanger sequencing on matching adjacent normal tissues, primary tumors, and metastatic tumors from 12 metastatic colorectal cancer patients ( n =84 for genomes, n =81 for exomes, n =9120 for single cells). Patient-derived tumor organoids were used to estimate the anti-tumor effects of a PPAR inhibitor, and self-renewal and differentiation ability of stem cell-like tumor cells. Results We found that the PPAR signaling pathway was prevalently and aberrantly activated in CRC tumors. Blocking of PPAR pathway both suppressed the growth and promoted the apoptosis of CRC organoids in vitro, indicating that aberrant activation of the PPAR signaling pathway plays a critical role in CRC tumorigenesis. Using matched samples from the same patient, distinct origins of the metastasized tumors between lymph node and liver were revealed, which was further verified by both copy number variation and mitochondrial mutation profiles at single-cell resolution. By combining single-cell RNA-Seq and single-cell point mutation identification by targeted cDNA Sanger sequencing, we revealed important phenotypic differences between cancer cells with and without critical point mutations ( KRAS and TP53 ) in the same patient in vivo at single-cell resolution. Conclusions Our data provides deep insights into how driver mutations interfere with the transcriptomic state of cancer cells in vivo at a single-cell resolution. Our findings offer novel knowledge on metastatic mechanisms as well as potential markers and therapeutic targets for CRC diagnosis and therapy. The high-precision single-cell RNA-seq dataset of matched adjacent normal tissues, primary tumors, and metastases from CRCs may serve as a rich resource for further studies.
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