CD4+ CD25+ 调节性T细胞在脓毒症免疫抑制中的作用。
The contribution of CD4+ CD25+ T-regulatory-cells to immune suppression in sepsis.
作者信息
Wisnoski Nicholas, Chung Chun-Shiang, Chen Yaping, Huang Xin, Ayala Alfred
机构信息
Shock-Trauma Research Laboratories in the Division of Surgical Research, Department of Surgery, Rhode Island Hospital and Brown University School of Medicine, Providence, Rhode Island 02903, USA.
出版信息
Shock. 2007 Mar;27(3):251-7. doi: 10.1097/01.shk.0000239780.33398.e4.
Studies have indicated that there is a development of generalized immune dysfunction after septic insult. However, the mechanisms responsible for these changes remain unclear. Recently, accumulating evidence shows that several lymphocyte subpopulations such as NKT-, CD4(+)-Th2-T-, CD8(+)-T-, gammadelta-T-, and CD4+ CD25+ T regulatory cells are capable of actively contributing to the induction of septic immune suppression. Thus, our aim was to investigate the contribution of CD4+ CD25+ cells to the immune dysfunction seen in sepsis. To study this, C57BL/6J, C57BL/6-Il6(tm1Kopf) (interleukin [IL] 6 -/-), and C57BL/6-Il10(tm1Cgn) (IL-10 -/-) mice were subjected to cecal ligation and puncture (CLP) or sham operations. Twenty-four hours later, blood was collected, and splenocytes were isolated. Phenotypic expression of CD4/CD25 (by fluorescence-activated cell sorter), cell proliferation (presented as proliferation index = [with anti-CD3]/[without anti-CD3]), and immune suppressive capacity (by in vitro add-back experiments) were assessed. The results indicate a marked elevation in CD4+ CD25+ cell levels and their proliferation index after sepsis in background mice. CD4+ CD25- cells from sham and CLP mice proliferated equally. However, coculture of CD4+ CD25- with CD4+ CD25+ cells suppressed their proliferation in both sham and CLP mice. Depletion of CD25+ cells in vivo before CLP markedly restored CD4+ CD25- proliferative capacity and Th1 cytokine release while not altering plasma proinflammatory cytokine levels. Subsequently, IL-6 -/- and IL-10 -/- mice were used to elucidate the possible mediator(s) regulating the changes seen after sepsis. Although CD4+ CD25+ cells increased after septic insult in both C57BL/6J and IL-6 -/- mice, this was not observed in IL-10 -/- mice. Similarly, in vitro proliferation studies showed that proliferation index increased in CD4+ CD25+ cells from septic C57BL/6J and IL6 -/- mice, but it remained the same in IL-10 -/- mice. Surprisingly, depletion of CD25+ cells before inducing sepsis did not alter septic mortality. Together, these findings suggest that although CD4+ CD25+ T regulatory cells induced by IL-10 seem to contribute to aspects of sepsis-induced lymphoid immune suppression, the oblation of CD25+ cells does not provide a survival advantage or disadvantage.
研究表明,脓毒症损伤后会出现全身性免疫功能障碍。然而,导致这些变化的机制仍不清楚。最近,越来越多的证据表明,一些淋巴细胞亚群,如自然杀伤T细胞、CD4(+)辅助性T细胞2型、CD8(+)T细胞、γδT细胞和CD4+CD25+调节性T细胞,能够积极促成脓毒症免疫抑制的诱导。因此,我们的目的是研究CD4+CD25+细胞在脓毒症中出现的免疫功能障碍中的作用。为了研究这一点,将C57BL/6J、C57BL/6-Il6(tm1Kopf)(白细胞介素[IL]-6基因敲除)和C57BL/6-Il10(tm1Cgn)(IL-10基因敲除)小鼠进行盲肠结扎和穿刺(CLP)或假手术。24小时后,采集血液并分离脾细胞。评估CD4/CD25的表型表达(通过荧光激活细胞分选仪)、细胞增殖(以增殖指数表示 = [抗CD3刺激后]/[无抗CD3刺激])和免疫抑制能力(通过体外回补实验)。结果表明,背景小鼠在脓毒症后CD4+CD25+细胞水平及其增殖指数显著升高。假手术和CLP小鼠的CD4+CD2-细胞增殖情况相同。然而,在假手术和CLP小鼠中,CD4+CD2-细胞与CD4+CD25+细胞共培养均会抑制其增殖。CLP前体内清除CD25+细胞可显著恢复CD4+CD2-细胞的增殖能力和Th1细胞因子释放,而不改变血浆促炎细胞因子水平。随后,使用IL-6基因敲除和IL-10基因敲除小鼠来阐明可能调节脓毒症后所见变化的介质。尽管在C57BL/6J和IL-6基因敲除小鼠中,脓毒症损伤后CD4+CD25+细胞均增加,但在IL-10基因敲除小鼠中未观察到这种情况。同样,体外增殖研究表明,脓毒症C57BL/6J和IL-6基因敲除小鼠的CD4+CD25+细胞增殖指数增加,但在IL-10基因敲除小鼠中保持不变。令人惊讶的是,诱导脓毒症前清除CD25+细胞并未改变脓毒症死亡率。总之,这些发现表明,尽管IL-10诱导的CD4+CD25+调节性T细胞似乎在脓毒症诱导的淋巴细胞免疫抑制方面发挥作用,但清除CD25+细胞并不会带来生存优势或劣势。
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