A serum- and feeder-free system to generate CD4 and regulatory T cells from human iPSCs

被引:0
|
作者
Fong, Helen [1 ,2 ]
Mendel, Matthew [1 ]
Jascur, John [1 ,2 ]
Najmi, Laeya [1 ,3 ]
Kim, Ken [1 ]
Lew, Garrett [1 ]
Garimalla, Swetha [1 ,4 ]
Schock, Suruchi [1 ]
Hu, Jing [1 ]
Villegas, Andres Gordillo [1 ,5 ]
Conway, Anthony [1 ,6 ]
Fontenot, Jason D. [1 ,7 ]
Zompi, Simona [1 ,8 ]
机构
[1] Sangamo Therapeut, Richmond, CA 94804 USA
[2] Proxim Therapeut, San Francisco, CA 94107 USA
[3] BioMarin, Novato, CA 94949 USA
[4] OmniAb, Emeryville, CA 94608 USA
[5] Kodiak Sci, Palo Alto, CA 94304 USA
[6] Replay, San Diego, CA 92121 USA
[7] Stylus Med, Cambridge, MA 02139 USA
[8] CARGO Therapeut, San Carlos, CA 94070 USA
关键词
THYMOCYTE-THYMOCYTE INTERACTION; PLURIPOTENT STEM-CELLS; POSITIVE SELECTION; IN-VITRO; EPIGENETIC CONTROL; FOXP3; EXPRESSION; DIFFERENTIATION; LINEAGE; CD8(+); STIMULATION;
D O I
10.1093/stmcls/sxaf001
中图分类号
Q813 [细胞工程];
学科分类号
摘要
iPSCs can serve as a renewable source of a consistent edited cell product, overcoming limitations of primary cells. While feeder-free generation of clinical grade iPSC-derived CD8 T cells has been achieved, differentiation of iPSC-derived CD4sp and regulatory T cells requires mouse stromal cells in an artificial thymic organoid. Here we report a serum- and feeder-free differentiation process suitable for large-scale production. Using an optimized concentration of PMA/Ionomycin, we generated iPSC-CD4sp T cells at high efficiency and converted them to Tregs using TGF beta and ATRA. Using genetic engineering, we demonstrated high, non-viral, targeted integration of an HLA-A2 CAR in iPSCs. iPSC-Tregs +/- HLA-A2-targeted CAR phenotypically, transcriptionally and functionally resemble primary Tregs and suppress T-cell proliferation in vitro. Our work is the first to demonstrate an iPSC-based platform amenable to manufacturing CD4 T cells to complement iPSC-CD8 oncology products and functional iPSC-Tregs to deliver Treg cell therapies at scale.
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页数:18
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