<i>Ex vivo</i> generation of human cytomegalovirus‐specific cytotoxic T cells by peptide‐pulsed dendritic cells

Kleihauer, Annette; Grigoleit, Ulrich; Hebart, Holger; Moris, Arnaud; Brossart, Peter; Muhm, Alexandra; Stevanović, Stefan; Rammensee, Hans Georg; Sinzger, Christian; Riegler, Susanne; Jahn, Gerhard; Kanz, Lothar; Einsele, Hermann

doi:10.1046/j.1365-2141.2001.02681.x

Cited by 68 publications

(43 citation statements)

References 40 publications

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“…Peptide pulsing of DC proved highly efficient for the selective stimulation and expansion of peptide-specific CTL in eight out of nine donors with pre-existing CD8 + cells against the peptide. This is in contrast to the findings of Kleihauer et al (2001), who reported a variable success of expanding CMV-directed CD8 + T cells. The expanded CTL specifically lysed T2 target cells pulsed with the cognate peptide, as also shown by others (Solache et al, 1999;Kleihauer et al, 2001).…”

Section: Discussioncontrasting

confidence: 55%

“…This is in contrast to the findings of Kleihauer et al (2001), who reported a variable success of expanding CMV-directed CD8 + T cells. The expanded CTL specifically lysed T2 target cells pulsed with the cognate peptide, as also shown by others (Solache et al, 1999;Kleihauer et al, 2001). MHC class I tetramers can be used for the direct isolation of CMV-specific T cells from leukapheresis products.…”

Section: Discussioncontrasting

confidence: 55%

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Ex vivo stimulation of cytomegalovirus (CMV)‐specific T cells using CMV pp65‐modified dendritic cells as stimulators

et al. 2003

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Summary. Cytomegalovirus (CMV) infection is a dangerous complication in immunosuppressed individuals such as allogeneic stem cell transplant patients. CMV disease can be prevented by the early post-transplant transfer of donorderived, CMV-directed, T cells. Fast and cost efficient methods to generate CMV-specific T cells are, therefore, warranted. The current study utilized peptide-pulsed and adenovirus-transduced dendritic cells (DC) to generate CMV-restricted T cells. After one stimulation with CMV pp65 495)503 peptide-pulsed DC and three re-stimulations with peptide-pulsed monocytes, virtually all T cells were CD8 + , expressed the relevant T cell receptor and exhibited high peptide-specific lytic activity. After only one stimulation, pp65 495)503 -restricted T cells could be sorted to a purity of higher than 95% and expanded up to 1000-fold in 2 weeks. This technique may prove useful for the rapid generation of large quantities of specific cytolytic T lymphocytes (CTL) for cell therapy. DC transduced with an adenoviral vector encoding the full-length pp65 protein (Adpp65) were able to simultaneously expand CTL against multiple epitopes of pp65. In addition, they activated CMVspecific CD4 + T-helper cells. This approach would stimulate multiple-epitope populations of pp65-specific T cells and could be made available to patients of any human leucocyte antigen (HLA) haplotype. DC transduced with adenoviral vectors to express full-length antigens may prove to be potent vaccines against viral pathogens and cancer.

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Section: Discussioncontrasting

confidence: 55%

Section: Discussioncontrasting

confidence: 55%

Ex vivo stimulation of cytomegalovirus (CMV)‐specific T cells using CMV pp65‐modified dendritic cells as stimulators

et al. 2003

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“…For example, infusion of CMVspecific CD8 ϩ T cell clones to hemopoietic stem cell recipients resulted in the restoration of CMV-specific immunity (12,19). Various combinations of APC and CMV Ags have been developed for the generation of CMV-specific T cell responses including CMV-infected fibroblasts (20); CMV-infected MoDC (21,22); MoDC pulsed with pp65 peptides (23,24); MoDC pulsed with recombinant pp65 protein (25); adenovirus vector-infected MoDC (26); vaccinia virus vector-infected MoDC (27); LCL transfected with pp65 gene (28); and retrovirus vector-infected LCL (29). All of the methods described to date have limitations.…”

Section: Discussionmentioning

confidence: 99%

“…The results, however, do not necessarily preclude the possibility of priming naive T cells with CD40-B/pp65 cells. Kleihauer et al (23) showed that cytotoxic T cell lines were generated from CMV-seronegative donors only in 2 of 11 donors starting with 3 ϫ 10 6 PBMC, even after stimulating with pp65 peptidepulsed MoDC. Szmania et al (24) also reported that only 2 of 10 CTL lines were pp65 specific, when 2 ϫ 10 6 PBMC were stimulated with MoDC.…”

Section: Discussionmentioning

confidence: 99%

Efficient Generation of Antigen-Specific Cytotoxic T Cells Using Retrovirally Transduced CD40-Activated B Cells

Kondo

Topp²,

Kiem

et al. 2002

The Journal of Immunology

107

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The development of rapid, efficient, and safe methods for generating Ag-specific T cells is necessary for the clinical application of adoptive immunotherapy. We show that B cells stimulated with CD40 ligand and IL-4 (CD40-B cells) can be efficiently transduced with retroviral vectors encoding a model Ag, CMV tegument protein pp65 gene, and maintain high levels of costimulatory molecules after gene transfer. CTL lines specific for pp65 were readily generated in all four healthy CMV-seropositive donors by stimulating autologous CD8+ T cells with these transduced CD40-B cells, both of which were derived from 10 ml peripheral blood. ELISPOT assays revealed that the CTL lines used multiple HLA alleles as restricting elements. Thus, CD40-B cells transduced retrovirally with Ag-encoding cDNA can be potent APC and facilitate to generate Ag-specific CTL in vitro.

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“…Remarkably, with a small proportion of CMV-seronegative donors it has been possible to generate CMV-specific T cells by in vitro priming (45)(46)(47). However, we expect it to be very difficult to translate these observations into feasible clinical procedures, because the precursor frequency of naive CMV-specific CD8 ϩ T cells in CMV-seronegative individuals, estimated from general considerations on TCR diversity (48), is unlikely to be above 1 in 10 6 naive T cells.…”

Section: Cd8mentioning

confidence: 99%

CMV-Specific TCR-Transgenic T Cells for Immunotherapy

Schub

Schuster

Hammerschmidt

et al. 2009

The Journal of Immunology

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Reactivation of CMV can cause severe disease after allogeneic hemopoietic stem cell transplantation. Adoptive T cell therapy was successfully used for patients who had received transplants from CMV-positive donors. However, patients with transplants from CMV-negative donors are at highest risk, and an adoptive therapy is missing because CMV-specific T cells are not available from such donors. To address this problem, we used retroviral transfer of CMV-specific TCR genes. We generated CMV-specific T cell clones of several HLA restrictions recognizing the endogenously processed Ag pp65. The genes of four TCRs were cloned and transferred to primary T cells from CMV-negative donors. These CMV-TCR-transgenic T cells displayed a broad spectrum of important effector functions (secretion of IFN-γ and IL-2, cytotoxicity, proliferation) in response to endogenously processed pp65 and could be enriched and expanded by strictly Ag-specific stimulation. Expansion of engineered T cells was accompanied by an increase in specific effector functions, indicating that the transferred specificity is stable and fully functional. Hence, we expect these CMV-TCR-transgenic T cells to be effective in controlling acute CMV disease and establishing an antiviral memory.

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Ex vivo generation of human cytomegalovirus‐specific cytotoxic T cells by peptide‐pulsed dendritic cells

Cited by 68 publications

References 40 publications

Ex vivo stimulation of cytomegalovirus (CMV)‐specific T cells using CMV pp65‐modified dendritic cells as stimulators

Ex vivo stimulation of cytomegalovirus (CMV)‐specific T cells using CMV pp65‐modified dendritic cells as stimulators

Efficient Generation of Antigen-Specific Cytotoxic T Cells Using Retrovirally Transduced CD40-Activated B Cells

CMV-Specific TCR-Transgenic T Cells for Immunotherapy

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