Generation of large numbers of fully mature and stable dendritic cells from leukapheresis products for clinical application

白细胞清除术 单采 CD14型 树突状细胞 浅黄色外套 CD86 人口 免疫学 单核细胞 启动(农业) 男科 化学 外周血单个核细胞 生物 医学 体外 细胞生物学 T细胞 免疫系统 血小板 川地34 生物化学 发芽 环境卫生 植物 干细胞
作者
Beatrice Thurner,Claudia Röder,Detlef Dieckmann,Marion Heuer,Monika Kruse,Anke Glaser,Petra Keikavoussi,Eckhart Kämpgen,Armin Bender,Gerold Schuler
出处
期刊:Journal of Immunological Methods [Elsevier BV]
卷期号:223 (1): 1-15 被引量:465
标识
DOI:10.1016/s0022-1759(98)00208-7
摘要

Dendritic Cell (DC)-based vaccination approaches in man require a reproducible DC generation method that can be performed in conformity with GMP (Good Manufacturing Practice) guidelines and that circumvents the need for multiple blood drawings to generate DC. To this end we modified our previously described method to generate mature DC from CD14 + monocytes by a two step method (priming in GM-SF + IL-4 followed by maturation in monocyte conditioned medium) for use with leukapheresis products as a starting population. Several adaptations were necessary. We established, for example, a modified adherence step to reliably enrich CD14 + DC precursors from apheresis mononuclear cells. The addition of GM-CSF + IL-4 at the onset of culture proved disadvantageous and was, therefore, delayed for 24 h. DC development from apheresis cells occurred faster than from fresh blood or buffy coat, and was complete after 7 days. Monocyte conditioned medium when added on day 6 resulted in fully mature and stable DC (veiled, highly migratory and T cell sensitizing cells with a characteristic phenotype such as 85% CD83 + , p55/fascin + , CD115/M-CSF-R - , CD86 + ) already after 24 h. The mature DC progeny were shown to remain stable and viable if cultured for another 1-2 days in the absence of cytokines, and to be resistant to inhibitory effects of IL-10. Freezing conditions were established to generate DC from frozen aliquots of PBMC or to freeze mature DC themselves for later use. The approach yields large numbers of standardized DC (5-10 x 10(8) mature CD83 + DC/leukapheresis) that are suitable for performing sound DC-based vaccination trials that can be compared with each other.
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