2021
DOI: 10.3389/fimmu.2021.694588
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Therapeutic Vaccination of Hematopoietic Cell Transplantation Recipients Improves Protective CD8 T-Cell Immunotherapy of Cytomegalovirus Infection

Abstract: Reactivation of latent cytomegalovirus (CMV) endangers the therapeutic success of hematopoietic cell transplantation (HCT) in tumor patients due to cytopathogenic virus spread that leads to organ manifestations of CMV disease, to interstitial pneumonia in particular. In cases of virus variants that are refractory to standard antiviral pharmacotherapy, immunotherapy by adoptive cell transfer (ACT) of virus-specific CD8+ T cells is the last resort to bridge the “protection gap” between hematoablative conditionin… Show more

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Cited by 8 publications
(16 citation statements)
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“…From the very low numbers of viral epitope-specific cells required in AT for control of infection in various organs it becomes intuitively clear that protection is not accomplished by an instant effector function of the few initially transferred cells. Instead, protection must result from the effector function of the progeny cell population generated by in vivo clonal expansion of the transferred cells [33,78]. As we have shown previously [78], as well as here (Fig 3), AT of unseparated memory cells leads to CD8 T-cell tissue infiltrates that are not randomly distributed but accumulate at infected cells in a micro-anatomical structure, the NIF.…”
Section: Resultssupporting
confidence: 58%
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“…From the very low numbers of viral epitope-specific cells required in AT for control of infection in various organs it becomes intuitively clear that protection is not accomplished by an instant effector function of the few initially transferred cells. Instead, protection must result from the effector function of the progeny cell population generated by in vivo clonal expansion of the transferred cells [33,78]. As we have shown previously [78], as well as here (Fig 3), AT of unseparated memory cells leads to CD8 T-cell tissue infiltrates that are not randomly distributed but accumulate at infected cells in a micro-anatomical structure, the NIF.…”
Section: Resultssupporting
confidence: 58%
“…Standard assays for in vivo proliferation are based on loss of a fluorescent reporter dye with every cell division [81,82], but this approach requires AT of high cell numbers, and the resolution is limited to few cell divisions until fluorescence intensity falls below the detection limit. To overcome such technical limitations, we used here our previously described approach of a quantitative ‘input-output’ comparison of the number of initially transferred viral epitope-specific CD8 T cells with the absolute number of progeny cells present in a host organ at defined times after AT [33,78]. CD8 T cells in the stage of cell division were detected in situ by 2C-IHC specific for the CD8 molecule, which localizes to the cytoplasm and cell membrane, and the intra-nuclear ‘proliferating cell nuclear antigen’ PCNA (Fig 7A, images).…”
Section: Resultsmentioning
confidence: 99%
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“…Furthermore, the pattern of immunoreconstitution was not analyzed due to insufficient data on the dynamic monitoring of lymphocyte subsets. Because our retrospective study focused on recipients after haplo-HCT with an ATG-contained regimen, the impact of serotherapy should be taken into account in further studies ( Lindemans et al., 2015 ; Storek, 2015 ; Willemsen et al., 2015 ; Gergely et al., 2021 ; Keogh et al., 2021 ). Hence, our findings need to be validated by large-scale real-world studies and laboratory investigations in the future.…”
Section: Discussionmentioning
confidence: 99%