Stem cell–derived CAR T cells traffic to HIV reservoirs in macaques
Isaac M. Barber-Axthelm, … , Hans-Peter Kiem, Christopher W. Peterson
Isaac M. Barber-Axthelm, … , Hans-Peter Kiem, Christopher W. Peterson
Published January 11, 2021
Citation Information: JCI Insight. 2021;6(1):e141502. https://doi.org/10.1172/jci.insight.141502.
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Research Article AIDS/HIV Stem cells

Stem cell–derived CAR T cells traffic to HIV reservoirs in macaques

Abstract

Allogeneic hematopoietic stem cell transplantation (allo-HSCT) with CCR5– donor cells is the only treatment known to cure HIV-1 in patients with underlying malignancy. This is likely due to a donor cell–mediated graft-versus-host effect targeting HIV reservoirs. Allo-HSCT would not be an acceptable therapy for most people living with HIV due to the transplant-related side effects. Chimeric antigen receptor (CAR) immunotherapies specifically traffic to malignant lymphoid tissues (lymphomas) and, in some settings, are able to replace allo-HSCT. Here, we quantified the engraftment of HSC-derived, virus-directed CAR T cells within HIV reservoirs in a macaque model of HIV infection, using potentially novel IHC assays. HSC-derived CAR cells trafficked to and displayed multilineage engraftment within tissue-associated viral reservoirs, persisting for nearly 2 years in lymphoid germinal centers, the brain, and the gastrointestinal tract. Our findings demonstrate that HSC-derived CAR+ cells reside long-term and proliferate in numerous tissues relevant for HIV infection and cancer.

Authors

Isaac M. Barber-Axthelm, Valerie Barber-Axthelm, Kai Yin Sze, Anjie Zhen, Gajendra W. Suryawanshi, Irvin S.Y. Chen, Jerome A. Zack, Scott G. Kitchen, Hans-Peter Kiem, Christopher W. Peterson

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Figure 2

Anti-CD4 antibody clone SP35 specifically marks CAR+ cells.

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Anti-CD4 antibody clone SP35 specifically marks CAR+ cells. (A and B) Sp...
(A and B) Specific CD4 (SP35) immunoreactivity in germinal centers from mesenteric lymph node sections from macaques that received either CD4CAR (A) or CD4CARΔζ (B); sparse marking in the parafollicular zone was also observed. (C and D) No immunoreactivity was seen in paired adjacent CD4CAR (C) or CD4CARΔζ (D) tissue sections labeled with an isotype control. (E) Positive control: Labeling of human tonsil shows specific immunoreactivity, which is predominately in the parafollicular zone and consistent with CD4+ T cell marking. (F) Negative control: no immunoreactivity is seen in a control mesenteric lymph node section from a macaque that did not receive either CD4CAR or CD4CARΔζ, indicating that the CD4 (SP35) antibody clone does not cross-react with the endogenous pigtail macaque CD4 antigen. Brown, immunoreactivity for human CD4CAR; blue, hematoxylin counterstain. The experiment was repeated twice to confirm the specificity of the CD4 (SP35) antibody for the human-derived CDCAR or CD4CARΔζ. Scale bars: 50 μm.