Frenkel Deborah, Zhang Fengqiu, Guirnalda Patrick, Haynes Carole, Bockstal Viki, Radwanska Magdalena, Magez Stefan, Black Samuel J
Department of Veterinary and Animal Sciences, University of Massachusetts Amherst, Amherst, Massachusetts, United States of America.
Laboratory for Cellular and Molecular Immunology, Vrije Universiteit Brussel, Brussels, Belgium.
PLoS Pathog. 2016 Jul 12;12(7):e1005733. doi: 10.1371/journal.ppat.1005733. eCollection 2016 Jul.
After infection with T. brucei AnTat 1.1, C57BL/6 mice lost splenic B2 B cells and lymphoid follicles, developed poor parasite-specific antibody responses, lost weight, became anemic and died with fulminating parasitemia within 35 days. In contrast, infected C57BL/6 mice lacking the cytotoxic granule pore-forming protein perforin (Prf1-/-) retained splenic B2 B cells and lymphoid follicles, developed high-titer antibody responses against many trypanosome polypeptides, rapidly suppressed parasitemia and did not develop anemia or lose weight for at least 60 days. Several lines of evidence show that T. brucei infection-induced splenic B cell depletion results from natural killer (NK) cell-mediated cytotoxicity: i) B2 B cells were depleted from the spleens of infected intact, T cell deficient (TCR-/-) and FcγRIIIa deficient (CD16-/-) C57BL/6 mice excluding a requirement for T cells, NKT cell, or antibody-dependent cell-mediated cytotoxicity; ii) administration of NK1.1 specific IgG2a (mAb PK136) but not irrelevant IgG2a (myeloma M9144) prevented infection-induced B cell depletion consistent with a requirement for NK cells; iii) splenic NK cells but not T cells or NKT cells degranulated in infected C57BL/6 mice co-incident with B cell depletion evidenced by increased surface expression of CD107a; iv) purified NK cells from naïve C57BL/6 mice killed purified splenic B cells from T. brucei infected but not uninfected mice in vitro indicating acquisition of an NK cell activating phenotype by the post-infection B cells; v) adoptively transferred C57BL/6 NK cells prevented infection-induced B cell population growth in infected Prf1-/- mice consistent with in vivo B cell killing; vi) degranulated NK cells in infected mice had altered gene and differentiation antigen expression and lost cytotoxic activity consistent with functional exhaustion, but increased in number as infection progressed indicating continued generation. We conclude that NK cells in T. brucei infected mice kill B cells, suppress humoral immunity and expedite early mortality.
感染布氏锥虫AnTat 1.1后,C57BL/6小鼠脾脏中的B2 B细胞和淋巴滤泡消失,寄生虫特异性抗体反应不佳,体重减轻,出现贫血,并在35天内死于暴发性寄生虫血症。相比之下,缺乏细胞毒性颗粒穿孔蛋白穿孔素(Prf1-/-)的受感染C57BL/6小鼠保留了脾脏B2 B细胞和淋巴滤泡,产生了针对多种锥虫多肽的高滴度抗体反应,迅速抑制了寄生虫血症,并且至少60天内没有出现贫血或体重减轻。多项证据表明,布氏锥虫感染诱导的脾脏B细胞耗竭是由自然杀伤(NK)细胞介导的细胞毒性所致:i)在受感染的完整、T细胞缺陷(TCR-/-)和FcγRIIIa缺陷(CD16-/-)的C57BL/6小鼠脾脏中,B2 B细胞被耗尽,排除了对T细胞、NKT细胞或抗体依赖性细胞介导的细胞毒性的需求;ii)给予NK1.1特异性IgG2a(单克隆抗体PK136)而非无关的IgG2a(骨髓瘤M9144)可预防感染诱导的B细胞耗竭,这与对NK细胞的需求一致;iii)在受感染的C57BL/6小鼠中,脾脏NK细胞而非T细胞或NKT细胞脱颗粒,同时B细胞耗竭,CD107a表面表达增加证明了这一点;iv)从幼稚C57BL/6小鼠中纯化的NK细胞在体外杀死了来自布氏锥虫感染但未感染小鼠的纯化脾脏B细胞,表明感染后的B细胞获得了NK细胞激活表型;v)过继转移的C57BL/6 NK细胞阻止了感染的Prf1-/-小鼠中感染诱导的B细胞群体生长,这与体内B细胞杀伤一致;vi)感染小鼠中脱颗粒的NK细胞基因和分化抗原表达发生改变,细胞毒性活性丧失,与功能耗竭一致,但随着感染进展数量增加,表明持续生成。我们得出结论,布氏锥虫感染小鼠中的NK细胞杀死B细胞,抑制体液免疫并加速早期死亡。
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