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Treatment with G-CSF reduces acute myeloid leukemia blast viability in the presence of bone marrow stroma

机译:在骨髓基质存在的情况下,使用G-CSF进行治疗可降低急性髓样白血病胚细胞的生存能力

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The resulting clinical impact of the combined use of G-CSF with chemotherapy as a chemosensitizing strategy for treatment of acute myeloid leukemia (AML) patients is still controversial. In this study, the effect of ex vivo treatment with G-CSF on AML primary blasts was studied. Peripheral blood mononuclear cells from AML patients were treated with G-CSF at increasing doses, alone or in co-culture with HS-5 stromal cells. Cell viability and surface phenotype was determined by flow cytometry 72?h after treatment. For clonogenicity assays, AML primary samples were treated for 18?h with G-CSF at increasing concentrations and cultured in methyl-cellulose for 14?days. Colonies were counted based on cellularity and morphology criteria. The presence of G-CSF reduced the overall viability of AML cells co-cultured with bone marrow stroma; whereas, in absence of stroma, a negligible effect was observed. Moreover, clonogenic capacity of AML cells was significantly reduced upon treatment with G-CSF. Interestingly, reduction in the AML clonogenic capacity correlated with the sensitivity to chemotherapy observed in vivo. These ex vivo results would provide a biological basis to data available from studies showing a clinical benefit with the use of G-CSF as a priming agent in patients with a chemosensitive AML and would support implementation of further studies exploring new strategies of chemotherapy priming in AML.
机译:联合使用G-CSF与化学疗法作为治疗急性髓细胞性白血病(AML)的化学增敏策略所产生的临床影响仍存在争议。在这项研究中,研究了G-CSF体外治疗对AML原代细胞的影响。将来自AML患者的外周血单核细胞单独或与HS-5基质细胞一起用G-CSF递增剂量治疗。处理后72小时,通过流式细胞仪测定细胞活力和表面表型。为了进行克隆形成性分析,将AML原始样品用浓度递增的G-CSF处理18分钟,并在甲基纤维素中培养14天。根据细胞性和形态学标准对菌落进行计数。 G-CSF的存在降低了与骨髓基质共培养的AML细胞的整体生存能力;而在没有基质的情况下,观察到的影响可忽略不计。此外,用G-CSF治疗后,AML细胞的克隆能力明显降低。有趣的是,AML克隆形成能力的降低与体内观察到的化疗敏感性相关。这些离体研究结果将为可从研究中获得的数据提供生物学基础,这些研究表明使用G-CSF作为化学敏感性AML患者的引发剂具有临床益处,并将支持进一步研究的开展,以探索针对AML进行化学疗法引发的新策略。

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