A soluble activator that favors the ex vivo expansion of CD8+CD27+ T cells
Esther I. Matus, Amanda Sparkes, Jean Gariépy
Esther I. Matus, Amanda Sparkes, Jean Gariépy
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Resource and Technical Advance Therapeutics

A soluble activator that favors the ex vivo expansion of CD8+CD27+ T cells

Abstract

Adoptive cell therapy involves the infusion of tumor-reactive T cells into patients with cancer to provide antitumor immunity. The ex vivo expansion and differentiation of such T cells are key parameters that affect their therapeutic potential. Human T cells are presently expanded in culture through the use of anti-CD3 and anti-CD28 mAbs immobilized on beads, expressed on cells, or assembled in the context of soluble antibody complexes. Here we report the design of a small, bispecific single-chain variable fragment construct agonizing both CD3 and CD28 pathways. This soluble T cell expansion protein, termed T-CEP, activates, expands, and differentiates human T cells ex vivo at concentrations in the femtomolar range. Importantly, T-CEP promotes the preferential growth of human CD8+ T cells over the course of 12 days in comparison with methods involving immobilized anti-CD3 mAb/soluble anti-CD28 mAb or soluble anti-CD3/CD28 mAb complexes. The differentiation profile of the resulting human T cell population is also singularly affected by T-CEP, favoring the expansion of a preferred CD8+CD27+ T cell phenotype. The activity profile of T-CEP on human T cells ex vivo suggests its use in generating human T cell populations that are more suited for adoptive cell therapy.

Authors

Esther I. Matus, Amanda Sparkes, Jean Gariépy

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Figure 5

Human T cell activation following stimulation over a 12-day ex vivo expansion period.

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Human T cell activation following stimulation over a 12-day ex vivo expa...
The presence of surface markers on human T cells from 5 donors was analyzed by flow cytometry. (A) The surface expression of activation markers CD25 and CD38 exposed to specific stimulation conditions. The increase in median fluorescence intensities (MFIs) for the activation markers was calculated by subtracting MFI values at day 0 before stimulation. MFI values of both activation markers decreased to baseline values by day 12 for all 3 donors. T-CEP–stimulated T cells showed the highest average expression of both activation markers. The MFI of CD25, significantly increased when stimulated with T-CEP as compared with i αCD3 and i αCD3 with s αCD28 in CD4+ T cells, and compared with i αCD3 in CD8+ T cells. There was no significant difference in peak CD38 MFI values between specific stimulation methods. By day 12 the MFI of both activation markers returned to pretreatment levels in all stimulation methods (n = 5, 1-way repeated measures ANOVA with a Tukey’s multiple-comparison test). (B) The coexpression of PD-1 and LAG-3 markers on human T cells peaked by day 3 and returned to pretreatment levels by day 12. In both CD4+ and CD8+ T cells, the expression of these markers was significantly increased on day 3 in T-CEP–stimulated cells but returned to baseline values as in the case of other activation methods by day 9. (n = 5, 1-way repeated measures ANOVA with a Tukey’s multiple-comparison test.) TACs, tetrameric antibody complexes; i αCD3, immobilized anti-CD3; s αCD28, soluble anti-CD28. *P < 0.05; ***P < 0.001; ☐, T-CEP; ○, TACs; ◇, i αCD3 + s αCD28; △, i αCD3.