The cell-mediated immune response to ectromelia virus infection. Secondary response in vitro: specificity, nature of effector and responder cells and requirements for induction of antigenic changes in stimulator cells.

T Pang, R V Blanden
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Abstract

An in vitro culture method was used to study secondary cell-mediated responses to ectromelia virus infection in mice. Infected, syngeneic spleen cells or peritoneal cells were efficient "stimulator" cells when cultured with "responder" cells obtained from mice infected with ectromelia 4-6 weeks previously. The kinetics of generation of cytotoxic cells in cultures were determined; a peak occurred on days 4-5. A separation procedure performed on the cytotoxic cells showed that activity was associated mainly with the Ig-negative subpopulation (T cell-rich) and that H-2 compatibility between cytotoxic cells and target cells was required. The secondary response was virus-specific, at the level of both induction and target cell lysis, at least so far as ectromelia and lymphocytic choriomeningitis (LCM) viruses are concerned. Seperation of responder cells prior to culture showed that a potent secondary response was generated with the Ig-negative (T cell-rich) subpopulation and only a weak response was observed when the responder cells were Ig-positive (rich in B cells). Infected stimulator cells did not appear to secrete significant amounts of soluble antigen into the medium over 4 days of culture. Thus, antigenic patterns effective in memory T cell stimulation may be largely associated with the surfaces of infected cells.Pretreatment of ectromelia virus with UV- or gamma-irradiation did not impair its ability to induce antigenic changes in stimulator cells. Stimulator cells treated with UV-or gamma-irradiated virus for 1 h and then immediately with pactamycin to inhibit further viral protein synthesis and replication were efficient stimulators, thus indicating that antigenic changes are induced very rapidly on the surface of stimulator cells after uptake of virus. These treatments are being used to further characterize the cellular requirements in the stimulator population.

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细胞介导的免疫应答对疣病毒感染的影响。体外二次反应:特异性、效应细胞和应答细胞的性质以及诱导刺激细胞抗原变化的要求。
采用体外培养的方法研究了小鼠继发性细胞介导的对嗜电性贫血病毒感染的反应。感染的同系脾细胞或腹膜细胞与4-6周前感染鼠患的“应答”细胞一起培养时,是有效的“刺激”细胞。测定培养物中细胞毒性细胞生成动力学;发病高峰出现在第4-5天。对细胞毒性细胞进行的分离程序表明,活性主要与igg阴性亚群(T细胞丰富)相关,并且细胞毒性细胞和靶细胞之间需要H-2相容性。在诱导和靶细胞裂解水平上,继发性反应是病毒特异性的,至少就嗜电性和淋巴细胞性脉络丛脑膜炎(LCM)病毒而言是如此。在培养前分离的应答细胞表明,在igg阴性(富含T细胞)的亚群中产生了强有力的二次应答,而当应答细胞为igg阳性(富含B细胞)时,只观察到微弱的应答。感染的刺激细胞在培养的4天内似乎没有分泌大量的可溶性抗原到培养基中。因此,在记忆T细胞刺激中有效的抗原模式可能在很大程度上与感染细胞的表面有关。用紫外或γ辐照预处理嗜电性贫血病毒不影响其在刺激细胞中诱导抗原变化的能力。用紫外线或γ辐照的病毒处理刺激细胞1小时,然后立即用帕塔霉素抑制病毒蛋白的进一步合成和复制,这是有效的刺激细胞,这表明在摄取病毒后,刺激细胞表面的抗原变化是非常迅速地诱导的。这些治疗方法正被用于进一步表征刺激器群体的细胞需求。
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