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Your search keyword '"Cerundolo, V."' showing total 10 results
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10 results on '"Cerundolo, V."'

2. Cross-presentation of tumour antigens by human induced pluripotent stem cell-derived CD141+XCR1+ dendritic cells.

Author

Silk, K M, Silk, J D, Ichiryu, N, Davies, T J, Nolan, K F, Leishman, A J, Carpenter, L, Watt, S M, Cerundolo, V, and Fairchild, P J

Subjects
TUMOR antigens, INDUCED pluripotent stem cells, DENDRITIC cells, MONOCYTES, CANCER immunotherapy, T cells, CYTOTOXIC T cells
Abstract

Monocyte-derived dendritic cells (moDC) have been widely used in cancer immunotherapy but show significant donor-to-donor variability and low capacity for the cross-presentation of tumour-associated antigens (TAA) to CD8+ T cells, greatly limiting the success of this approach. Given recent developments in induced pluripotency and the relative ease with which induced pluripotent stem (iPS) cell lines may be generated from individuals, we have succeeded in differentiating dendritic cells (DC) from human leukocyte antigen (HLA)-A*0201+ iPS cells (iPS cell-derived DC (ipDC)), using protocols compliant with their subsequent clinical application. Unlike moDC, a subset of ipDC was found to coexpress CD141 and XCR1 that have been shown previously to define the human equivalent of mouse CD8α+ DC, in which the capacity for cross-presentation has been shown to reside. Accordingly, ipDC were able to cross-present the TAA, Melan A, to a CD8+ T-cell clone and stimulate primary Melan A-specific responses among naïve T cells from an HLA-A*0201+ donor. Given that CD141+XCR1+ DC are present in peripheral blood in trace numbers that preclude their clinical application, the ability to generate a potentially unlimited source from iPS cells offers the possibility of harnessing their capacity for cross-priming of cytotoxic T lymphocytes for the induction of tumour-specific immune responses. [ABSTRACT FROM AUTHOR]

Published
2012
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3. Glykosphingolipide Gb3 und iGb3.

Author

Porubsky, S., Luckow, B., Bonrouhi, M., Speak, A., Cerundolo, V., Platt, F., and Gröne, H.-J.

Abstract

Copyright of Der Pathologe is the property of Springer Nature and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published
2008
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4. Malignant melanoma and bone resorption.

Author

Lau, Y. S., Sabokbar, A., Giele, H., Cerundolo, V., Hofstetter, W., and Athanasou, N. A.

Subjects
BONE metastasis, MELANOMA, BONE cancer, BONE resorption, OSTEOCLASTS, CYTOKINES, CANCER cells, ANTINEOPLASTIC agents, CARRIER proteins, CELL culture, CELL differentiation, CELL receptors, COMPARATIVE studies, CULTURE media (Biology), FIBROBLASTS, GLYCOPROTEINS, INTERLEUKIN-1, MACROPHAGES, RESEARCH methodology, MEDICAL cooperation, MEMBRANE proteins, METASTASIS, POLYMERASE chain reaction, RESEARCH, SKIN tumors, TUMOR necrosis factors, EVALUATION research, REVERSE transcriptase polymerase chain reaction, MEMBRANE glycoproteins, PHARMACODYNAMICS
Abstract

The cellular and humoral mechanisms accounting for osteolysis in skeletal metastases of malignant melanoma are uncertain. Osteoclasts, the specialised multinucleated cells that carry out bone resorption, are derived from monocyte/macrophage precursors. We isolated tumour-associated macrophages (TAMs) from metastatic (lymph node/skin) melanomas and cultured them in the presence and absence of osteoclastogenic cytokines and growth factors. The effect of tumour-derived fibroblasts and melanoma cells on osteoclast formation and resorption was also analysed. Melanoma TAMs (CD14+/CD51-) differentiated into osteoclasts (CD14-/CD51+) in the presence of receptor activator for nuclear factor kappaB ligand (RANKL) and macrophage-colony stimulating factor. Tumour-associated macrophage-osteoclast differentiation also occurred via a RANKL-independent pathway when TAMs were cultured with tumour necrosis factor-alpha and interleukin (IL)-1alpha. RT-PCR showed that fibroblasts isolated from metastatic melanomas expressed RANKL messenger RNA and the conditioned medium of cultured melanoma fibroblasts was found to be capable of inducing osteoclast formation in the absence of RANKL; this effect was inhibited by the addition of osteoprotegerin (OPG). We also found that cultured human SK-Mel-29 melanoma cells produce a soluble factor that induces osteoclast differentiation; this effect was not inhibited by OPG. Our findings indicate that TAMs in metastatic melanomas can differentiate into osteoclasts and that melanoma fibroblasts and melanoma tumour cells can induce osteoclast formation by RANKL-dependent and RANKL-independent mechanisms, respectively. [ABSTRACT FROM AUTHOR]

Published
2006
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5. Sensitization of tumour cells to lysis by virus-specific CTL using antibody-targeted MHC class I/peptide complexes.

Author

Ogg, G S, Dunbar, P R, Cerundolo, V, McMichael, A J, Lemoine, N R, and Savage, P

Subjects
IMMUNOTHERAPY, MONOCLONAL antibodies, CANCER, HLA histocompatibility antigens
Abstract

A number of cell surface molecules with specificity to tumour cells have been identified and monoclonal antibodies (mAb) to some of these antigens have been used for targeting tumour cells in vivo. We have sought to link the powerful effector mechanisms of cytotoxic T-cells with the specificity of mAb, by targeting recombinant HLA class I molecules to tumour cells using an antibody delivery system. Soluble recombinant MHC class I/peptide complexes including HLA-A2.1 refolded around an immunodominant peptide from the HIV gag protein (HLA-A2/gag) were synthesized, and the stability of these complexes at 37 °C was confirmed by enzyme-linked immunosorbent assay using a conformation-specific antibody. MHC class I-negative lymphoma cells (Daudi) were labelled with a biotinylated mAb specific for a cell surface protein (anti-CD20) then linked to soluble biotinylated HLA-A2/gag complexes using an avidin bridge. Flow cytometry revealed strong labelling of lymphoma cells with HLA-A2/gag complexes (80-fold increase in mean channel fluorescence). CTL specific for HLA-A2/gag efficiently lysed complex-targeted cells, while control CTL (specific for an HLA-A2.1-restricted epitope of melan-A) did not. Similarly, SK-mel-29 melanoma cells were also efficiently lysed by HLA-A2/gag-specific CTL when HLA-A2/gag complexes were linked to their surface via the HMW-MAA specific anti-melanoma antibody 225.28s. With further consideration to the in vivo stability of the MHC class I/peptide complexes, this system could prove a new strategy for the immunological therapy of cancer. [ABSTRACT FROM AUTHOR]

Published
2000
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9. Presentation of viral antigen by MHC class I molecules is dependent on a putative peptide...

Author

Spies, T. and Cerundolo, V.

Subjects
*VIRUSES
Abstract

States that major histocompatibility complex (MHC) class I molecules present peptides derived from the endogenous protein pool to cytotoxic T lymphocytes, which can thus recognize intracellular antigen. Shows that PSF1 is necessary for the efficient assembly of class I molecules and enables them to present a peptide epitope derived from endogenously synthesized viral antigen.

Published
1992
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10. Results and harmonization guidelines from two large-scale international Elispot proficiency panels conducted by the Cancer Vaccine Consortium (CVC/SVI)

Author

Sylvia, Janetzki, Katherine S, Panageas, Leah, Ben-Porat, Jean, Boyer, Cedrik M, Britten, Timothy M, Clay, Michael, Kalos, Holden T, Maecker, Pedro, Romero, Jianda, Yuan, W Martin, Kast, Axel, Hoos, Jedd, Wolchok, Elispot Proficiency Panel of the CVC Immune Assay Working Group, Anderson, R., Bercovici, N., Boyer, J., Britten, C., Brockstedt, D., Caterini, J., Cerundolo, V., Chen, W., Clay, T., Darnell, R., Dubey, S., Ermak, T., Gnjatic, S., Harrop, R., Healey, D., Houghton, A., Jaeger, E., Janssen, W., Jones, L., Kast, WM., Kaufman, J., Knuth, A., Konur, A., Kos, F., Kunle, O., Manson, K., Matijevic, M., Miyahara, Y., Musselli, C., Olson, W., Panicali, D., Parida, S., Parker, J., Pohla, H., Pride, M., Rappaport, R., Reay, P., Rivoltini, L., Romero, P., Schiltz, P., Shiku, H., Slingluff, C., Smith, J., Speiser, D., Swanlund, D., Vajdy, M., Van der Aa, A., Weber, J., Woelfel, T., and Wolchok, J.

Subjects
Quality Control, medicine.medical_specialty, Cancer Research, Standardization, Cell Survival, International Cooperation, Immunology, Harmonization, Enzyme-Linked Immunosorbent Assay, Audit, Certification, Cancer Vaccines, Sensitivity and Specificity, Interlaboratory testing, Leukocyte Count, Validation, Medicine, Humans, Immunology and Allergy, Medical physics, Immune monitoring, Protocol (science), Proficiency panel, business.industry, Clinical Laboratory Techniques, ELISPOT, Reproducibility of Results, Guideline, Reference Standards, Health Surveys, Cancer Vaccines/immunology, Cell Survival/immunology, Clinical Laboratory Techniques/standards, Clinical Laboratory Techniques/statistics & numerical data, Enzyme-Linked Immunosorbent Assay/standards, Laboratories/standards, Leukocytes, Mononuclear/immunology, Peptides/immunology, Societies, Oncology, Scale (social sciences), Leukocytes, Mononuclear, Original Article, business, Laboratories, Peptides, Tetramer
Abstract

The interpretation of the results obtained from immunomonitoring of clinical trials is a difficult task due to the variety of methods and protocols available to detect vaccine-specific T-cell responses. This heterogeneity as well as the lack of standards has led to significant scepticism towards published results. In February 2005, a working group was therefore founded under the aegis of the Association for Immunotherapy of Cancer (“CIMT”) in order to compare techniques and protocols applied for the enumeration of antigen-specific T-cell responses. Here we present the results from two consecutive phases of an international inter-laboratory testing project referred to as the “CIMT monitoring panel”. A total of 13 centers from six European countries participated in the study in which pre-tested PBMC samples, synthetic peptides and PE-conjugated HLA-tetramers were prepared centrally and distributed to participants. All were asked to determine the number of antigen-specific T-cells in each sample using tetramer staining and one functional assay. The results of the first testing round revealed that the total number of cells analyzed was the most important determinant for the sensitive detection of antigen-specific CD8+ T-cells by tetramer staining. Analysis by ELISPOT was influenced by a combination of cell number and a resting phase after thawing of peripheral blood mononuclear cells. Therefore, the experiments were repeated in a second phase but now the participants were asked to change their protocols according to the new guidelines distilled from the results of the first phase. The recommendations improved the number of antigen-specific T-cell responses that were detected and decreased the variability between the laboratories. We conclude that a two-step approach in inter-laboratory testing allows the identification of distinct variables that influence the sensitivity of different T-cell assays and to formally show that a defined correction to the protocols successfully increases the sensitivity and reduces the inter-center variability. Such “two-step” inter-laboratory projects could define rational bases for accepted international guidelines and thereby lead to the harmonization of the techniques used for immune monitoring. Electronic supplementary material The online version of this article (doi:10.1007/s00262-007-0378-0) contains supplementary material, which is available to authorized users.

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