Single-cell transcriptome conservation in cryopreserved cells and tissues

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作者
Amy Guillaumet-Adkins
Gustavo Rodríguez-Esteban
Elisabetta Mereu
Maria Mendez-Lago
Diego A. Jaitin
Alberto Villanueva
August Vidal
Alex Martinez-Marti
Enriqueta Felip
Ana Vivancos
Hadas Keren-Shaul
Simon Heath
Marta Gut
Ido Amit
Ivo Gut
Holger Heyn
机构
[1] CNAG-CRG,Department of Immunology
[2] Centre for Genomic Regulation (CRG),Chemoresistance and Predictive Factors Laboratory, Program Against Cancer Therapeutic Resistance (ProCURE)
[3] Barcelona Institute of Science and Technology (BIST),Department of Pathology
[4] Universitat Pompeu Fabra (UPF),undefined
[5] Weizmann Institute,undefined
[6] Catalan Institute of Oncology (ICO),undefined
[7] Bellvitge Institute for Biomedical Research (IDIBELL),undefined
[8] Xenopat S.L.,undefined
[9] Business Bioincubator,undefined
[10] University Hospital of Bellvitge (IDIBELL),undefined
[11] Vall d’Hebron University Hospital,undefined
[12] Universitat Autònoma de Barcelona (UAB),undefined
[13] Vall d’Hebron Institute of Oncology (VHIO),undefined
来源
关键词
Single-cell genomics; RNA sequencing; Transcriptomics; MARS-Seq; Smart-seq2; Cryopreservation; Conservation; Peripheral blood mononuclear cells; PBMC; Patient-derived orthotopic xenograft; PDOX;
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摘要
A variety of single-cell RNA preparation procedures have been described. So far, protocols require fresh material, which hinders complex study designs. We describe a sample preservation method that maintains transcripts in viable single cells, allowing one to disconnect time and place of sampling from subsequent processing steps. We sequence single-cell transcriptomes from >1000 fresh and cryopreserved cells using 3'-end and full-length RNA preparation methods. Our results confirm that the conservation process did not alter transcriptional profiles. This substantially broadens the scope of applications in single-cell transcriptomics and could lead to a paradigm shift in future study designs.
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