Monocyte derived dendritic cells generated by IFN-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis

BACKGROUND: Dendritic cell (DC) vaccines can induce antitumor immune responses in patients with malignant diseases, while the most suitable DC culture conditions have not been established yet. In this study we compared monocyte derived human DC from conventional cultures containing GM-CSF and IL-4/T...

Descripción completa

Detalles Bibliográficos
Autores principales: Korthals, Mark, Safaian, Nancy, Kronenwett, Ralf, Maihöfer, Dagmar, Schott, Matthias, Papewalis, Claudia, Diaz Blanco, Elena, Winter, Meike, Czibere, Akos, Haas, Rainer, Kobbe, Guido, Fenk, Roland
Formato: Texto
Lenguaje:English
Publicado: BioMed Central|1 2007
Materias:
Research
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2064912/
https://www.ncbi.nlm.nih.gov/pubmed/17894866
http://dx.doi.org/10.1186/1479-5876-5-46
_version_ 1782137636950900736
author Korthals, Mark
Safaian, Nancy
Kronenwett, Ralf
Maihöfer, Dagmar
Schott, Matthias
Papewalis, Claudia
Diaz Blanco, Elena
Winter, Meike
Czibere, Akos
Haas, Rainer
Kobbe, Guido
Fenk, Roland
author_facet Korthals, Mark
Safaian, Nancy
Kronenwett, Ralf
Maihöfer, Dagmar
Schott, Matthias
Papewalis, Claudia
Diaz Blanco, Elena
Winter, Meike
Czibere, Akos
Haas, Rainer
Kobbe, Guido
Fenk, Roland
author_sort Korthals, Mark
collection PubMed
description BACKGROUND: Dendritic cell (DC) vaccines can induce antitumor immune responses in patients with malignant diseases, while the most suitable DC culture conditions have not been established yet. In this study we compared monocyte derived human DC from conventional cultures containing GM-CSF and IL-4/TNF-α (IL-4/TNF-DC) with DC generated by the novel protocol using GM-CSF and IFN-α (IFN-DC). METHODS: To characterise the molecular differences of both DC preparations, gene expression profiling was performed using Affymetrix microarrays. The data were conformed on a protein level by immunophenotyping, and functional tests for T cell stimulation, migration and cytolytic activity were performed. RESULTS: Both methods resulted in CD11c+ CD86+ HLA-DR+ cells with a typical DC morphology that could efficiently stimulate T cells. But gene expression profiling revealed two distinct DC populations. Whereas IL-4/TNF-DC showed a higher expression of genes envolved in phagocytosis IFN-DC had higher RNA levels for markers of DC maturity and migration to the lymph nodes like DCLAMP, CCR7 and CD49d. This different orientation of both DC populations was confined by a 2.3 fold greater migration in transwell experiments (p = 0.01). Most interestingly, IFN-DC also showed higher RNA levels for markers of NK cells such as TRAIL, granzymes, KLRs and other NK cell receptors. On a protein level, intracytoplasmatic TRAIL and granzyme B were observed in 90% of IFN-DC. This translated into a cytolytic activity against K562 cells with a median specific lysis of 26% at high effector cell numbers as determined by propidium iodide uptake, whereas IL-4/TNF-DC did not induce any tumor cell lysis (p = 0.006). Thus, IFN-DC combined characteristics of mature DC and natural killer cells. CONCLUSION: Our results suggest that IFN-DC not only stimulate adaptive but also mediate innate antitumor immune responses. Therefore, IFN-DC should be evaluated in clinical vaccination trials. In particular, this could be relevant for patients with diseases responsive to a treatment with IFN-α such as Non-Hodgkin lymphoma or chronic myeloid leukemia.
format Text
id pubmed-2064912
institution National Center for Biotechnology Information
language English
publishDate 2007
publisher BioMed Central|1
record_format MEDLINE/PubMed
spelling pubmed-20649122007-11-07 Monocyte derived dendritic cells generated by IFN-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis Korthals, Mark Safaian, Nancy Kronenwett, Ralf Maihöfer, Dagmar Schott, Matthias Papewalis, Claudia Diaz Blanco, Elena Winter, Meike Czibere, Akos Haas, Rainer Kobbe, Guido Fenk, Roland J Transl Med Research BACKGROUND: Dendritic cell (DC) vaccines can induce antitumor immune responses in patients with malignant diseases, while the most suitable DC culture conditions have not been established yet. In this study we compared monocyte derived human DC from conventional cultures containing GM-CSF and IL-4/TNF-α (IL-4/TNF-DC) with DC generated by the novel protocol using GM-CSF and IFN-α (IFN-DC). METHODS: To characterise the molecular differences of both DC preparations, gene expression profiling was performed using Affymetrix microarrays. The data were conformed on a protein level by immunophenotyping, and functional tests for T cell stimulation, migration and cytolytic activity were performed. RESULTS: Both methods resulted in CD11c+ CD86+ HLA-DR+ cells with a typical DC morphology that could efficiently stimulate T cells. But gene expression profiling revealed two distinct DC populations. Whereas IL-4/TNF-DC showed a higher expression of genes envolved in phagocytosis IFN-DC had higher RNA levels for markers of DC maturity and migration to the lymph nodes like DCLAMP, CCR7 and CD49d. This different orientation of both DC populations was confined by a 2.3 fold greater migration in transwell experiments (p = 0.01). Most interestingly, IFN-DC also showed higher RNA levels for markers of NK cells such as TRAIL, granzymes, KLRs and other NK cell receptors. On a protein level, intracytoplasmatic TRAIL and granzyme B were observed in 90% of IFN-DC. This translated into a cytolytic activity against K562 cells with a median specific lysis of 26% at high effector cell numbers as determined by propidium iodide uptake, whereas IL-4/TNF-DC did not induce any tumor cell lysis (p = 0.006). Thus, IFN-DC combined characteristics of mature DC and natural killer cells. CONCLUSION: Our results suggest that IFN-DC not only stimulate adaptive but also mediate innate antitumor immune responses. Therefore, IFN-DC should be evaluated in clinical vaccination trials. In particular, this could be relevant for patients with diseases responsive to a treatment with IFN-α such as Non-Hodgkin lymphoma or chronic myeloid leukemia. BioMed Central|1 2007-09-25 /pmc/articles/PMC2064912/ /pubmed/17894866 http://dx.doi.org/10.1186/1479-5876-5-46 Text en Copyright © 2007 Korthals et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License ( (http://creativecommons.org/licenses/by/2.0) ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research
Korthals, Mark
Safaian, Nancy
Kronenwett, Ralf
Maihöfer, Dagmar
Schott, Matthias
Papewalis, Claudia
Diaz Blanco, Elena
Winter, Meike
Czibere, Akos
Haas, Rainer
Kobbe, Guido
Fenk, Roland
Monocyte derived dendritic cells generated by IFN-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis
title Monocyte derived dendritic cells generated by IFN-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis
title_full Monocyte derived dendritic cells generated by IFN-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis
title_fullStr Monocyte derived dendritic cells generated by IFN-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis
title_full_unstemmed Monocyte derived dendritic cells generated by IFN-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis
title_short Monocyte derived dendritic cells generated by IFN-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis
title_sort monocyte derived dendritic cells generated by ifn-α acquire mature dendritic and natural killer cell properties as shown by gene expression analysis
topic Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2064912/
https://www.ncbi.nlm.nih.gov/pubmed/17894866
http://dx.doi.org/10.1186/1479-5876-5-46
work_keys_str_mv AT korthalsmark monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT safaiannancy monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT kronenwettralf monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT maihoferdagmar monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT schottmatthias monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT papewalisclaudia monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT diazblancoelena monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT wintermeike monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT czibereakos monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT haasrainer monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT kobbeguido monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis
AT fenkroland monocytederiveddendriticcellsgeneratedbyifnaacquirematuredendriticandnaturalkillercellpropertiesasshownbygeneexpressionanalysis

Ejemplares similares