de Repentigny L, Petitbois S, Boushira M, Michaliszyn E, Sénéchal S, Gendron N, Montplaisir S
Department of Microbiology and Immunology, Faculty of Medicine, University of Montreal, Quebec, Canada.
Infect Immun. 1993 Sep;61(9):3791-802. doi: 10.1128/iai.61.9.3791-3802.1993.
A number of studies have substantiated the pivotal role of innate defense mechanisms in protection against invasive aspergillosis. However, experiments demonstrating increased resistance to lethal intravenous (i.v.) infection with Aspergillus fumigatus conidia in cortisone-treated or untreated mice preinfected with a sublethal dose of conidia and protection of turkeys inoculated subcutaneously with a killed A. fumigatus germling vaccine against subsequent aerosol challenge led us to speculate that acquired immunity may also contribute to host defense against Aspergillus infection. Five-week-old male BALB/c mice were inoculated i.v. with 1.0 x 10(4) viable conidia or saline and challenged i.v. with 1.0 x 10(6) conidia after 7, 15, or 21 days. No protection against challenge was found after 7 days. However, significant and reproducible protection was observed after 15 and 21 days. Mortality was reduced from 90% in control mice to 53% in preinfected mice 40 days after challenge (P = 0.0002). Increased survival was correlated with decreased content of chitin in lungs, liver, and kidneys 4 and 7 days after challenge (P < 0.05). Mice were again inoculated with 1.0 x 10(4) conidia or saline, and after 21 days, 1.0 x 10(8) or 2.0 x 10(8) splenocytes were transferred to naive syngeneic recipients; 2.0 x 10(8) immune splenocytes conferred significant protection (P = 0.0001) against i.v. challenge with 1.0 x 10(6) conidia, and mortality decreased from 83 to 48% 40 days after challenge. Transfer of immune serum offered no protection despite the presence of antibody against a hyphal homogenate of A. fumigatus, which was absent in the sera of control mice. Protection by immune splenocytes was maintained after selective depletion of T cells but was abolished after removal of plastic-adherent splenocytes. Adherent cells were characterized as macrophages by using morphological criteria, nonspecific esterase, and MAC-1 monoclonal antibody. Production of hydrogen peroxide by peritoneal and splenic macrophages from preinfected mice was the same as and lower than, respectively, that from uninfected controls. However, phagocytosis of conidia by peritoneal or splenic macrophages from mice preinfected i.v. or intratracheally was significantly increased after 2 and 3 h of coculture compared with that from uninfected animals, whereas in vitro killing of conidia by splenic macrophages was unaltered. Peritoneal or splenic macrophages from control or preinfected mice failed to kill hyphae in vitro. Killing of hyphae by polymorphonuclear leukocytes was not significantly different between mice preinfected i.v. and uninfected controls. Taken together, the results indicate that acquired immunity mediated by activated macrophages can be demonstrated in experimental murine aspergillosis.(ABSTRACT TRUNCATED AT 400 WORDS)
多项研究证实了固有防御机制在抵御侵袭性曲霉病中的关键作用。然而,有实验表明,在经可的松处理或未经处理的小鼠中,预先感染亚致死剂量分生孢子后,对致死性静脉注射烟曲霉分生孢子感染的抵抗力增强;用灭活的烟曲霉菌丝体疫苗皮下接种火鸡,可使其免受后续气溶胶攻击。这些实验使我们推测,获得性免疫也可能有助于宿主抵御曲霉感染。将1.0×10⁴个活的分生孢子或生理盐水静脉接种于5周龄雄性BALB/c小鼠,7、15或21天后再静脉注射1.0×10⁶个分生孢子进行攻毒。7天后未发现对攻毒的保护作用。然而,在15天和21天后观察到显著且可重复的保护作用。攻毒40天后,对照小鼠的死亡率为90%,而预先感染小鼠的死亡率降至53%(P = 0.0002)。存活时间延长与攻毒后4天和7天肺、肝和肾中几丁质含量降低相关(P < 0.05)。再次将1.0×10⁴个分生孢子或生理盐水接种小鼠,21天后,将1.0×10⁸或2.0×10⁸个脾细胞转移至同基因未感染受体;2.0×10⁸个免疫脾细胞对静脉注射1.0×10⁶个分生孢子的攻毒具有显著保护作用(P = 0.0001),攻毒40天后死亡率从83%降至48%。尽管免疫血清中存在针对烟曲霉菌丝匀浆的抗体(对照小鼠血清中不存在),但免疫血清并未提供保护作用。选择性清除T细胞后,免疫脾细胞的保护作用得以维持,但去除贴壁脾细胞后保护作用消失。通过形态学标准、非特异性酯酶和MAC-1单克隆抗体将贴壁细胞鉴定为巨噬细胞。预先感染小鼠的腹腔和脾巨噬细胞产生过氧化氢的量分别与未感染对照相同且低于未感染对照。然而,与未感染动物相比,预先经静脉或气管内感染小鼠的腹腔或脾巨噬细胞在共培养2小时和3小时后对分生孢子的吞噬作用显著增强,而脾巨噬细胞对分生孢子的体外杀伤作用未改变。对照或预先感染小鼠的腹腔或脾巨噬细胞在体外均不能杀死菌丝。预先经静脉感染小鼠的多形核白细胞对菌丝的杀伤作用与未感染对照无显著差异。综上所述,结果表明在实验性小鼠曲霉病中可证明由活化巨噬细胞介导的获得性免疫。(摘要截短至400字)
Zotero 插件