Lee Yang-Jin, Kim Jong-Hyun, Jeong Seok-Ryoul, Song Kyoung-Ju, Kim Kyongmin, Park Sun, Park Moon-Sung, Shin Ho-Joon
Department of Microbiology, Molecular Science & Technology, Ajou University School of Medicine, Suwon, 443-721, South Korea.
Parasitol Res. 2007 Oct;101(5):1191-6. doi: 10.1007/s00436-007-0600-1. Epub 2007 Jul 4.
Naegleria fowleri, agent of fatal primary amoebic meningoencephalitis, appears to induce cytotoxicity mechanically through its contact with the cell. The nfa1 gene cloned from a cDNA library of pathogenic N. fowleri by immunoscreening consists of 360 bp and expresses a 13.1-kDa recombinant protein (rNfa1) that demonstrated localization in the pseudopodia when examined using immunocytochemistry. To study the mechanisms involved in N. fowleri cytotoxicity, we developed a large volume of rNfa1-specific monoclonal antibody (McAb) against a 17-kDa His-tag fusion rNfa1 protein using a cell fusion technique. We established eight McAb-producing hybridoma cells. The antibodies were all immunoglobulin G2b and reacted strongly with a 17-kDa band representing the rNfa1 fusion protein in Western blotting, demonstrating immunoreactivity to the Nfa1 protein in pseudopodia (especially in the food cups) of N. fowleri trophozoites. A 51Cr-release assay indicated N. fowleri cytotoxicity by demonstrating that it eliminated 37.8, 60.6, and 98.8% of the target (microglial) cells 6, 12, and 24 h after co-incubation, respectively. When an anti-Nfa1 McAb was added to the coculture system, N. fowleri cytotoxicity decreased to 29.8, 44.1, and 66.3%, respectively.
福氏耐格里阿米巴是致命的原发性阿米巴脑膜脑炎的病原体,它似乎通过与细胞接触机械性地诱导细胞毒性。通过免疫筛选从致病性福氏耐格里阿米巴的cDNA文库中克隆出的nfa1基因由360个碱基对组成,表达一种13.1 kDa的重组蛋白(rNfa1),用免疫细胞化学检测时,该蛋白定位于伪足中。为了研究福氏耐格里阿米巴细胞毒性的相关机制,我们利用细胞融合技术制备了大量针对17 kDa的His标签融合rNfa1蛋白的rNfa1特异性单克隆抗体(McAb)。我们建立了8个产生McAb的杂交瘤细胞。这些抗体均为免疫球蛋白G2b,在蛋白质印迹法中与代表rNfa1融合蛋白的17 kDa条带强烈反应,证明对福氏耐格里阿米巴滋养体伪足(特别是食物泡)中的Nfa1蛋白具有免疫反应性。一项51Cr释放试验通过显示共孵育6、12和24小时后分别清除了37.8%、60.6%和98.8%的靶(小胶质)细胞,表明了福氏耐格里阿米巴的细胞毒性。当向共培养系统中加入抗Nfa1 McAb时,福氏耐格里阿米巴的细胞毒性分别降至29.8%、44.1%和66.3%。
