3D Centrifugation‐Enabled Priming of Synaptic Activation Promotes Primary T Cell Expansion

Author:

Jiang Ruoyu1ORCID,Chen Yu‐Hsi1ORCID,Parajuli Ritesh2,Agrawal Anshu3,Lee Abraham P.14ORCID

Affiliation:

1. Biomedical Engineering University of California Irvine CA 92697 USA

2. Department of Medicine Division of Hematology Oncology University of California Irvine CA 92697 USA

3. Department of Medicine Division of Basic and Clinical Immunology University of California Irvine CA 92697 USA

4. Mechanical and Aerospace Engineering University of California Irvine CA 92697 USA

Abstract

AbstractAutologous cell therapy depends on T lymphocyte expansion efficiency and is hindered by suboptimal interactions between T cell receptors (TCR) and peptide‐MHC molecules. Various artificial antigen presenting cell systems that enhance these interactions are often labor‐intensive, fabrication costly, highly variable, and potentially unscalable toward clinical setting. Here, 3D centrifugation‐enabled priming of T cell immune‐synapse junctions is performed to generate tight T cell–Dynabead aggregates at a rate 200‐fold faster than that of conventional 24‐h bulk shaking. Furthermore, by forming T cell–Dynabead aggregates in the starting culture, two‐ to sixfold greater T cell expansion is achieved over conventional T cell expansion for cancer patient‐derived primary T cells while limiting over‐activation. Creating 3D T cell–Dynabead aggregates as the “booster” material enables highly efficient polyclonal T cell expansion without the need for complex surface modification of artificial antigen‐presenting cells (APCs). This method can be modularly adapted to existing T cell expansion processes for various applications, including adoptive cell therapies (ACTs).

Funder

National Cancer Institute

Publisher

Wiley

Subject

Pharmacology (medical),Biochemistry (medical),Genetics (clinical),Pharmaceutical Science,Pharmacology,Medicine (miscellaneous)

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