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通过稳定表达小鼠吲哚胺2,3-双加氧酶建立抗弓形虫状态。

Establishment of an antitoxoplasma state by stable expression of mouse indoleamine 2,3-dioxygenase.

作者信息

Habara-Ohkubo A, Shirahata T, Takikawa O, Yoshida R

机构信息

Department of Cell Biology, Osaka Bioscience Institute, Suita, Japan.

出版信息

Infect Immun. 1993 May;61(5):1810-3. doi: 10.1128/iai.61.5.1810-1813.1993.

Abstract

Indoleamine 2,3-dioxygenase (IDO), a tryptophan-degrading enzyme, is inducible by various interferons (IFNs). IDO-mediated tryptophan degradation, but not the formation of IDO-catalyzed tryptophan metabolites, has been suggested as a mechanism for the antiparasitic action of IFN-gamma. To determine whether the IFN-gamma-induced IDO alone is sufficient for establishing the antiparasitic state, we constructed a mouse IDO expression plasmid containing a heavy metal-responsive metallothionein promoter and obtained a stable transformant (C6) by transfection of this plasmid into mouse rectal cancer (CMT-93) cells. In the presence of 100 microM ZnSO4, C6 cells yielded a high level of IDO; and after a 2-day culture period, the enzyme induction resulted in complete depletion of tryptophan from the culture medium. Under these conditions, the growth of Toxoplasma gondii in C6 cells infected with the organisms on day 3 after enzyme induction was completely blocked. In the absence of ZnSO4, however, IDO induction was negligible in C6 cells, and T. gondii continued to grow. Furthermore, in a transformant (CC10) carrying an antisense mouse IDO plasmid or in parental CMT-93 cells, IDO was not induced at all even in the presence of 100 microM ZnSO4, and T. gondii continued to grow in these cells as well. These results taken together indicate that complete depletion of tryptophan from the culture by IDO alone is sufficient to establish the antitoxoplasma state in mouse cells.

摘要

吲哚胺2,3-双加氧酶(IDO)是一种色氨酸降解酶,可被多种干扰素(IFN)诱导。IDO介导的色氨酸降解,而非IDO催化的色氨酸代谢产物的形成,被认为是IFN-γ抗寄生虫作用的一种机制。为了确定单独由IFN-γ诱导的IDO是否足以建立抗寄生虫状态,我们构建了一个含有重金属响应金属硫蛋白启动子的小鼠IDO表达质粒,并通过将该质粒转染到小鼠直肠癌(CMT-93)细胞中获得了一个稳定的转化体(C6)。在存在100μM硫酸锌的情况下,C6细胞产生高水平的IDO;经过2天的培养期后,酶诱导导致培养基中的色氨酸完全耗尽。在这些条件下,酶诱导后第3天感染弓形虫的C6细胞中弓形虫的生长被完全阻断。然而,在不存在硫酸锌的情况下,C6细胞中的IDO诱导可以忽略不计,并且弓形虫继续生长。此外,在携带反义小鼠IDO质粒的转化体(CC10)或亲本CMT-93细胞中,即使在存在100μM硫酸锌的情况下,IDO也根本不被诱导,并且弓形虫在这些细胞中也继续生长。综合这些结果表明,仅由IDO使培养基中的色氨酸完全耗尽就足以在小鼠细胞中建立抗弓形虫状态。

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