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首页> 外文期刊>Transfusion: The Journal of the American Association of Blood Banks >Evaluating maturation and genetic modification of human dendritic cells in a new polyolefin cell culture bag system.
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Evaluating maturation and genetic modification of human dendritic cells in a new polyolefin cell culture bag system.

机译:在新的聚烯烃细胞培养袋系统中评估人树突状细胞的成熟和遗传修饰。

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摘要

BACKGROUND: Dendritic cells (DCs) are applied worldwide in several clinical studies of immune therapy of malignancies, autoimmune diseases, and transplantations. Most legislative bodies are demanding high standards for cultivation and transduction of cells. Closed-cell cultivating systems like cell culture bags would simplify and greatly improve the ability to reach these cultivation standards. We investigated if a new polyolefin cell culture bag enables maturation and adenoviral modification of human DCs in a closed system and compare the results with standard polystyrene flasks. STUDY DESIGN AND METHODS: Mononuclear cells were isolated from HLA-A*0201-positive blood donors by leukapheresis. A commercially available separation system (CliniMACS, Miltenyi Biotec) was used to isolate monocytes by positive selection using CD14-specific immunomagnetic beads. The essentially homogenous starting cell population was cultivated in the presence of granulocyte-macrophage-colony-stimulating factor and interleukin-4 in a closed-bag system in parallel to the standard flask cultivation system. Genetic modification was performed on Day 4. After induction of maturation on Day 5, mature DCs could be harvested and cryopreserved on Day 7. During the cultivation period comparative quality control was performed using flow cytometry, gene expression profiling, and functional assays. RESULTS: Both flasks and bags generated mature genetically modified DCs in similar yields. Surface membrane markers, expression profiles, and functional testing results were comparable. The use of a closed-bag system facilitated clinical applicability of genetically modified DCs. CONCLUSIONS: The polyolefin bag-based culture system yields DCs qualitatively and quantitatively comparable to the standard flask preparation. All steps including cryopreservation can be performed in a closed system facilitating standardized, safe, and reproducible preparation of therapeutic cells.
机译:背景:树突状细胞(DC)在世界范围内广泛用于恶性肿瘤,自身免疫性疾病和移植物免疫治疗的一些临床研究中。大多数立法机构都对细胞的培养和转导提出了很高的要求。像细胞培养袋这样的闭孔培养系统将简化并大大提高达到这些培养标准的能力。我们调查了一个新的聚烯烃细胞培养袋是否可以在封闭系统中使人DC的成熟和腺病毒修饰,并将结果与​​标准聚苯乙烯烧瓶进行比较。研究设计和方法:通过白细胞分离术从HLA-A * 0201阳性献血者中分离出单核细胞。使用市售的分离系统(CliniMACS,Miltenyi Biotec)通过使用CD14特异性免疫磁珠的阳性选择分离单核细胞。在与标准烧瓶培养系统平行的密闭袋系统中,在粒细胞-巨噬细胞-集落刺激因子和白细胞介素-4的存在下培养基本均质的起始细胞群。在第4天进行遗传修饰。在第5天诱导成熟后,可以在第7天收获成熟的DC并冷冻保存。在培养期间,使用流式细胞术,基因表达谱和功能测定进行比较质量控制。结果:烧瓶和袋子都以相似的产量产生了成熟的转基因DC。表面膜标记物,表达谱和功能测试结果可比。封闭袋系统的使用促进了转基因DC的临床适用性。结论:基于聚烯烃袋的培养系统在质和量上可产生与标准烧瓶制备品相当的DC。包括冷冻保存在内的所有步骤均可在封闭系统中进行,以促进治疗细胞的标准化,安全和可重复制备。

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