Retroviral gene therapy with an immunoglobulin-antigen fusion construct protects from experimental autoimmune uveitis
Rajeev K. Agarwal, … , Chi-Chao Chan, Rachel R. Caspi
Rajeev K. Agarwal, … , Chi-Chao Chan, Rachel R. Caspi
Published January 15, 2000
Citation Information: J Clin Invest. 2000;106(2):245-252. https://doi.org/10.1172/JCI9168.
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Article

Retroviral gene therapy with an immunoglobulin-antigen fusion construct protects from experimental autoimmune uveitis

Abstract

Immunoglobulins can serve as tolerogenic carriers for antigens, and B cells can function as tolerogenic antigen-presenting cells. We used this principle to design a strategy for gene therapy of experimental autoimmune uveitis, a cell-mediated autoimmune disease model for human uveitis induced with the uveitogenic interphotoreceptor retinoid-binding protein (IRBP). A retroviral vector was constructed containing a major uveitogenic IRBP epitope in frame with mouse IgG1 heavy chain. This construct was used to transduce peripheral B cells, which were infused into syngeneic recipients. A single infusion of transduced cells, 10 days before uveitogenic challenge, protected mice from clinical disease induced with the epitope or with the native IRBP protein. Protected mice had reduced antigen-specific responses, but showed no evidence for a classic Th1/Th2 response shift or for generalized anergy. Protection was not transferable, arguing against a mechanism dependent on regulatory cells. Importantly, the treatment was protective when initiated 7 days after uveitogenic immunization or concurrently with adoptive transfer of primed uveitogenic T cells. We suggest that this form of gene therapy can induce epitope-specific protection not only in naive, but also in already primed recipients, thus providing a protocol for treatment of established autoimmunity.

Authors

Rajeev K. Agarwal, Yubin Kang, Elias Zambidis, David W. Scott, Chi-Chao Chan, Rachel R. Caspi

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IL-2, IFN-γ, and IL-10 production by spleen cells of tolerized mice to 3...
IL-2, IFN-γ, and IL-10 production by spleen cells of tolerized mice to 30 μM peptide. Shown are IFN-γ and IL-10 production as assayed 21 days after immunization (average of three experiments) and IL-2 as assayed only 10 days after immunization (single experiment). Values are normalized against the mock control (100%). Lower level of detectability in picograms per milliliter was 26 for IL-2, 30 for IFN-γ, and 10 for IL-10. Actual 100% values in picograms per milliliter were 3,600 for IL-2, 910 for IFN-γ, and 56 for IL-10. The pattern of IFN-γ and IL-10 responses on day 10 was the same as on day 21, though the absolute amounts secreted were higher. Lymph node cytokine responses were essentially identical to spleen responses.