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Differentiation of natural killer cells from induced pluripotent stem cells under defined, serum- and feeder-free conditions

脱颗粒 NKG2D公司 诱导多能干细胞 细胞生物学 免疫学 生物 胚胎干细胞 重编程 细胞 细胞毒性 体外 生物化学 受体 遗传学 基因
作者
Kyle B. Lupo,Jung-Il Moon,Andrea M. Chambers,Sandro Matosevic
出处
期刊:Cytotherapy [Elsevier BV]
卷期号:23 (10): 939-952 被引量:36
标识
DOI:10.1016/j.jcyt.2021.05.001
摘要

Background aims Traditionally, natural killer (NK) cells are sourced from the peripheral blood of donors―a laborious and highly donor-specific process. Processes for generating NK cells from induced pluripotent stem cells (iPSCs) have demonstrated that it is possible to successfully generate renewable alloreactive NK cells that are not only functional in vivo but can also be genetically engineered for enhanced function. However, poor standardization and cumbersome differentiation procedures suggest that further improvements in the control of the differentiation process are necessary. Methods Here the authors evaluated the potential of differentiating NK cells from centrally authenticated iPSCs under entirely chemically defined and serum-free conditions as well as their immunotherapeutic potential, after expansion in feeder-free media, against solid tumors targets. To address limitations of current differentiation approaches, the authors did not utilize feeder or stromal cell layers, TrypLE adaptation or peripheral blood during the differentiation process. The authors also evaluated the feasibility of utilizing centrally authenticated iPSC lines, thus circumventing protocol- and donor-induced variability associated with reprogramming approaches, and characterized these iPSC-NK cells in terms of cytotoxicity, cytokine production and degranulation potential against solid tumor cell lines and patient-derived targets. Results Differentiation of iPSCs generated NK cells that were predominantly CD56+/CD16+/CD3− and expressed NK activation markers NKG2D, NKp30, NKp44, NKp46 and DNAM-1. These iPSC-NK cells mediated effector functions, including cytotoxicity, degranulation and IFN-γ production, in response to solid tumor targets, including patient-derived cancer cells, and could be cryopreserved and expanded in culture. Conclusions The ability to produce NK cells under defined conditions and the functional responses elicited by these iPSC-NK cells suggest that they could represent promising effectors in clinical adoptive transfer settings as a renewable source of donor-independent NK cells for immunotherapy of solid tumors.
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