Efficient short-term expansion of human peripheral blood regulatory T cells for co-culture suppression assay

Korawit Kanjana, K. Paisooksantivatana, P. Matangkasombut, Parawee Chevaisrakul, P. Lumjiaktase
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引用次数: 4

Abstract

ABSTRACT Regulatory T cells (Tregs) are a small population of CD4+ lymphocytes and play a key role as suppressors of the immune system, a role that can be identified by employing a co-culture suppression assay. Conventional protocol requires a long period of in vitro expansion of Treg numbers; hence, this study describes an establishment of a co-culture suppression assay using a short-term expansion of peripheral blood (PB) Tregs and autologous T cells (Tconvs) IL-2-pre-cultured in parallel for the same length of time, thereby obviating the need of freeze/thawed autologous Tconvs. Tregs and Tconvs were isolated from PB mononuclear cells employing magnetic bead-aided depletion of CD8+ cells followed by cell sorting of CD4+ CD25high+CD127low- (Treg) and CD4+ CD25-CD127+ (Tconv) cell populations. Following a 3-day co-cultivation period under optimized conditions, Treg suppression activity was monitored by comparing using flow cytometry the number of carboxyfluorescein succinimidyl ester-labeled Tconvs to that of Treg-minus control. The assay allowed significant differentiation between Treg suppression activity of patients with active rheumatoid arthritis and those in remission. This method should be more convenient and time-saving than the conventional Treg suppression assay in current use.
人外周血调节性T细胞短期高效扩增共培养抑制实验
调节性T细胞(Regulatory T cells, Tregs)是CD4+淋巴细胞的一个小群体,作为免疫系统的抑制因子发挥着关键作用,这一作用可以通过共培养抑制实验来确定。常规方案需要长时间体外扩增Treg数量;因此,本研究描述了一种共同培养抑制实验的建立,利用外周血(PB) Tregs和自体T细胞(Tconvs) il -2的短期扩增,平行培养相同的时间长度,从而消除了对冷冻/解冻自体Tconvs的需要。从PB单核细胞中分离Tregs和Tconvs,采用磁珠辅助CD8+细胞耗散,然后对CD4+ CD25high+CD127low- (Treg)和CD4+ CD25-CD127+ (Tconv)细胞群进行细胞分选。在优化条件下共培养3天后,通过流式细胞术比较羧基荧光素琥珀酰酰酯标记的Tconvs与Treg阴性对照的数量,监测Treg抑制活性。该实验允许活动期类风湿关节炎患者和缓解期类风湿关节炎患者Treg抑制活性的显著差异。该方法比目前使用的常规Treg抑制法更方便、省时。
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