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建立使用 Epstein-Barr 病毒的 B 细胞系的稳健方法的开发。

Development of a robust method for establishing B cell lines using Epstein-Barr Virus.

机构信息

Cell Engineering Division, RIKEN BioResource Center, Koyadai, Tsukuba, Ibaraki, Japan.

出版信息

In Vitro Cell Dev Biol Anim. 2012 Aug;48(7):393-402. doi: 10.1007/s11626-012-9523-y. Epub 2012 Jul 18.

DOI:10.1007/s11626-012-9523-y
PMID:22806969
Abstract

B lymphoblastoid cell lines (B-LCLs) are generally established from B lymphocytes by infection with Epstein-Barr virus (EBV). As their genomic structure is stable in culture, B-LCLs are a valuable resource for many types of analysis. The efficiency of establishing B-LCLs from freshly obtained blood samples from healthy individuals is almost 100 %; however, for blood samples stored inappropriately after collection or held in long-term storage as peripheral blood mononuclear cells (PBMCs) in liquid nitrogen, the efficiency of B-LCL establishment can be considerably lower. To date, we have established more than 550 B-LCLs from 685 PBMC samples that have been stored in liquid nitrogen for over 20 yr. The PBMCs were prepared from blood samples donated by individuals belonging to native minority ethnic groups in outlying regions of South America and elsewhere. The establishment of B-LCLs from this material is difficult, and failure results in the waste of valuable and rare samples. We sought to improve our success rate for establishing B-LCLs from these difficult and irreplaceable samples by a detailed examination of each step of the process. The analysis showed that two parameters were particularly critical to the success rate: the density of the PBMCs plated after EBV infection and the EBV titer. These observations shed light on cases where establishment of B-LCLs was hard due to the small number of PBMCs or damage to the cells.

摘要

B 淋巴母细胞系 (B-LCL) 通常通过感染 Epstein-Barr 病毒 (EBV) 从 B 淋巴细胞中建立。由于其基因组结构在培养中稳定,B-LCL 是许多类型分析的宝贵资源。从健康个体新获得的血液样本中建立 B-LCL 的效率几乎为 100%;然而,对于收集后储存不当或作为外周血单核细胞 (PBMC) 在液氮中长期储存的血液样本,建立 B-LCL 的效率可能会显著降低。迄今为止,我们已经从超过 20 年储存在液氮中的 685 个 PBMC 样本中建立了超过 550 个 B-LCL。这些 PBMC 是从南美洲和其他地区偏远地区的土著少数民族个体捐献的血液样本中制备的。从这些材料中建立 B-LCL 很困难,失败会导致宝贵和稀有样本的浪费。我们通过详细检查该过程的每一步,旨在提高从这些困难和不可替代的样本中建立 B-LCL 的成功率。分析表明,两个参数对成功率特别关键:EBV 感染后接种 PBMC 的密度和 EBV 滴度。这些观察结果阐明了由于 PBMC 数量少或细胞受损导致 B-LCL 建立困难的情况。

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