Multivalent 4-1BB binding aptamers costimulate CD8+ T cells and inhibit tumor growth in mice
James O. McNamara II, … , Bruce Sullenger, Eli Gilboa
James O. McNamara II, … , Bruce Sullenger, Eli Gilboa
Published December 3, 2007
Citation Information: J Clin Invest. 2008;118(1):376-386. https://doi.org/10.1172/JCI33365.
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Research Article Technical Advance Oncology

Multivalent 4-1BB binding aptamers costimulate CD8+ T cells and inhibit tumor growth in mice

Abstract

4-1BB is a major costimulatory receptor that promotes the survival and expansion of activated T cells. Administration of agonistic anti–4-1BB Abs has been previously shown to enhance tumor immunity in mice. Abs are cell-based products posing significant cost, manufacturing, and regulatory challenges. Aptamers are oligonucleotide-based ligands that exhibit specificity and avidity comparable to, or exceeding, that of Abs. To date, various aptamers have been shown to inhibit the function of their cognate target. Here, we have described the development of an aptamer that binds 4-1BB expressed on the surface of activated mouse T cells and shown that multivalent configurations of the aptamer costimulated T cell activation in vitro and mediated tumor rejection in mice. Because aptamers can be chemically synthesized, manufacturing and the regulatory approval process should be substantially simpler and less costly than for Abs. Agonistic aptamers could therefore represent a superior alternative to Abs for the therapeutic manipulation of the immune system.

Authors

James O. McNamara II, Despina Kolonias, Fernando Pastor, Robert S. Mittler, Lieping Chen, Paloma H. Giangrande, Bruce Sullenger, Eli Gilboa

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Figure 2

Characterization of M12-23 and mutM12-23 aptamers.

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Characterization of M12-23 and mutM12-23 aptamers. (A) Sequence and comp...
(A) Sequence and computer-predicted secondary structure. Arrows show the nucleotide changes introduced into the M12-23 sequence to generate mutM12-23. (B) CFSE proliferation assay of suboptimally activated CD8+ T cells incubated with bead-multimerized 4-1BB aptamers. CD8+ T cells isolated from the spleens and lymph nodes of Balb/c mice were labeled with CFSE and cultured in the absence or presence of either 1 μg/ml anti-CD3 or isotype-matched hamster IgG control Ab. At 16 hours after plating, the following reagents were added, as indicated: 5 μg/ml anti–4-1BB Ab or isotype-matched rat IgG2a Ab, or 100 nM M12-23 aptamer (monomer), bead-coupled M12-23 aptamer, or bead-coupled mutM12-23 aptamer. Cellular fluorescence was measured with flow cytometry 72 hours after plating. Percentages within each panel indicate the fraction of cells that underwent proliferation. See Methods for additional details.