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利用家蚕感染模型评估处于萌发状态的白色念珠菌的致病性。

Evaluation of pathogenicity of Candida albicans in germination-ready states using a silkworm infection model.

作者信息

Matsumoto Haruhito, Nagao Jun-ichi, Cho Tamaki, Kodama Jun

机构信息

Department of Functional Bioscience, Fukuoka Dental College, Fukuoka, Japan.

出版信息

Med Mycol J. 2013;54(2):131-40. doi: 10.3314/mmj.54.131.

Abstract

We previously developed an N-acetyl-D-glucosamine (GlcNAc) medium which induces Candida albicans to undergo a yeast-to-hyphal transition through a cAMP-PKA pathway. Microarray analysis demonstrated that 18 genes, including ALS3 that encodes a cell wall adhesion, were upregulated by 30-min incubation of yeast cells at 37°C in the GlcNAc medium. To investigate the differences between morphological transition and morphotype in C. albicans as a consequence of infection, this study utilized a silkworm infection model as an invertebrate mini-host. We prepared 3 different conditions of C. albicans cells in vitro by changing the incubation times in the GlcNAc medium: yeast-form cells at 0 min (Y0 cells), yeast-form cells in germination-ready state at 60 min (Y60 cells), and hyphal cells at 120 min (H120 cells), and compared their pathogenicities. We performed the infection study at various temperatures to find temperature-dependent virulence factors in vivo. Y60 cells in germination-ready state in the GlcNAc medium showed higher pathogenicity in vivo compared to Y0 and H120 cells at 30°C. Y60 cells proliferated in silkworms 24 h post-injection at 30°C, whereas the other 2 cell types did not. In vitro analysis demonstrated that Y60 cells, but not Y0 cells, germinated in the silkworm hemolymph at 30°C. However, Y0 and Y60 cells showed a similar degree of germination in the silkworm hemolymph at 37°C, although no significant difference in silkworm survival after infection with each cell type was observed at 37°C. These results suggested that the germination-ready state induced by the GlcNAc medium contributed to virulence in the silkworm.

摘要

我们之前开发了一种N-乙酰-D-葡萄糖胺(GlcNAc)培养基,该培养基可通过cAMP-PKA途径诱导白色念珠菌发生酵母-菌丝转变。微阵列分析表明,包括编码细胞壁黏附蛋白的ALS3在内的18个基因,在37°C条件下于GlcNAc培养基中孵育酵母细胞30分钟后上调。为了研究白色念珠菌在感染过程中形态转变和形态型之间的差异,本研究利用家蚕感染模型作为无脊椎动物微型宿主。我们通过改变在GlcNAc培养基中的孵育时间,在体外制备了3种不同状态的白色念珠菌细胞:0分钟时的酵母型细胞(Y0细胞)、60分钟时处于萌发准备状态的酵母型细胞(Y60细胞)以及120分钟时的菌丝细胞(H120细胞),并比较了它们的致病性。我们在不同温度下进行感染研究,以寻找体内温度依赖性毒力因子。在30°C时,GlcNAc培养基中处于萌发准备状态的Y60细胞在体内显示出比Y0和H120细胞更高的致病性。在30°C注射后24小时,Y60细胞在家蚕体内增殖,而其他两种细胞类型则没有。体外分析表明,在30°C时,Y60细胞而非Y0细胞在家蚕血淋巴中萌发。然而,在37°C时,Y0和Y60细胞在家蚕血淋巴中的萌发程度相似,尽管在37°C用每种细胞类型感染后家蚕存活率没有显著差异。这些结果表明,GlcNAc培养基诱导的萌发准备状态有助于在家蚕体内产生毒力。

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