An Extended Flow Cytometry Evaluation of ex Vivo Expanded NK Cells Using K562.Clone1, a Feeder Cell Line Manufactured in Brazil

IF 3.6 3区 医学 Q2 HEMATOLOGY Transplantation and Cellular Therapy Pub Date : 2024-11-01 DOI:10.1016/j.jtct.2024.07.004
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Abstract

Natural killer (NK) cells play a crucial role in the immune system's response against cancer. However, the challenge of obtaining the required quantity of NK cells for effective therapeutic response necessitates the development of strategies for their ex vivo expansion. This study aimed to develop a novel feeder cell line, K562.Clone1, capable of promoting the ex vivo expansion of NK cells while preserving their cytotoxic potential. he K562 leukemic cell line was transduced with mbIL-21 and 4-1BBL proteins to generate K562.Clone1 cells. NK cells were then co-cultured with these feeder cells, and their expansion rate was monitored over 14 days. The cytotoxic potential of the expanded NK cells was evaluated against acute myeloid leukemia blasts and tumor cell lines of leukemia and glial origin. Statistical analysis was performed to determine the significance of the results. The K562.Clone1 co-cultured with peripheral NK showed a significant increase in cell count, with an approximate 94-fold expansion over 14 days. Expanded NK cells demonstrated cytotoxicity against the tested tumor cell lines, indicating preservation of their cytotoxic characteristics. Additionally, the CD56, CD16, inhibitory KIRs, and activation receptors were conserved and present in a well-balanced manner. The study successfully developed a feeder cell line, K562.Clone1, that effectively promotes the expansion of NK cells ex vivo while maintaining their cytotoxic potential. This development could significantly contribute to the advancement of NK cell therapy, especially in Brazil.
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使用巴西生产的馈源细胞系 K562.Clone1 对体内外扩增的 NK 细胞进行扩展流式细胞仪评估。
背景:自然杀伤细胞(NK)在免疫系统抗癌反应中发挥着至关重要的作用。然而,要获得有效治疗反应所需的 NK 细胞数量是一项挑战,因此有必要开发体内外扩增 NK 细胞的策略:本研究旨在开发一种新型饲养细胞系 K562.Clone1,这种细胞系能够促进 NK 细胞的体内外扩增,同时保留其细胞毒性潜能:研究设计:用mbIL-21和4-1BBL蛋白转导K562白血病细胞系,生成K562.Clone1细胞。研究设计:用 mbIL-21 和 4-1BBL 蛋白转导 K562 白血病细胞系,生成 K562.Clone1 细胞,然后将 NK 细胞与这些饲养细胞共培养,并在 14 天内监测其扩增速度。评估了扩增的 NK 细胞对急性髓性白血病血块以及白血病和胶质源肿瘤细胞系的细胞毒性潜力。对结果的显著性进行了统计分析:结果:与外周 NK 共同培养的 K562.Clone1 细胞数量显著增加,14 天内扩增了约 94 倍。扩增后的 NK 细胞对测试的肿瘤细胞系具有细胞毒性,表明其细胞毒性特性得以保留。此外,CD56、CD16、抑制性 KIR 和活化受体都是保守的,并以良好的平衡方式存在:该研究成功开发了一种饲养细胞系 K562.Clone1,它能有效促进体内 NK 细胞的扩增,同时保持其细胞毒性潜能。这项研究成果将极大地推动 NK 细胞疗法的发展,尤其是在巴西。
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来源期刊
CiteScore
7.00
自引率
15.60%
发文量
1061
审稿时长
51 days
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