新型隐球菌的细胞壁组成依赖于培养基,并改变宿主反应,诱导保护性免疫。

IF 2.1 Q3 MYCOLOGY Frontiers in fungal biology Pub Date : 2023-01-01 DOI:10.3389/ffunb.2023.1183291
Rajendra Upadhya, Woei C Lam, Camaron R Hole, Joseph G Vasselli, Jennifer K Lodge
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引用次数: 1

摘要

简介:新型隐球菌是一种担子菌真菌,可引起脑膜脑炎,特别是免疫功能低下的患者。隐球菌在许多不同的培养基中生长,尽管很少有人注意到生长条件对隐球菌细胞壁或毒力的作用。目的:研究不同培养基如何影响细胞壁中几丁质和壳聚糖的含量,从而影响细胞壁结构和宿主反应。方法:酵母提取液、蛋白胨和葡萄糖(YPD)和酵母氮碱(YNB)是隐球菌体外或体内实验前常用的两种培养基。结果,新生C. formans在YPD或YNB中生长,YPD或YNB要么没有缓冲,要么用MOPS缓冲到pH 7。然后用细胞壁特异性荧光探针标记这些细胞,以确定各种细胞壁成分的量。此外,这些细胞还被用于小鼠吸入感染模型的动物毒力研究。结果:我们观察到野生型新形态C. KN99在生长过程中显著改变了无缓冲培养基的pH值。当生长在无缓冲的YPD中时,pH值升高到8.0,而在无缓冲的YNB (YNB- u)中,pH值降低到2.0。重要的是,细胞壁的组成受到不同培养基生长的实质性影响。与YPD中生长的细胞相比,YNB-U中生长的细胞显示出90%的壳聚糖(几丁质的去乙酰化形式)减少。与YPD或pH为7的YNB- u培养的细胞相比,pH和壳聚糖的降低与YNB- u培养的细胞表面一些病原体相关分子模式的显著增加有关。当使用小鼠感染模型进行测试时,这种改变的细胞壁结构导致毒力显著降低。此外,当使用热杀伤细胞作为接种物时,在YNB-U中生长的KN99细胞引起肺部异常的高炎症反应,导致动物快速死亡。相比之下,在pH为7的YNB中生长的热杀死的KN99细胞在宿主肺部几乎没有引起炎症反应,但是,当用作疫苗时,它们对毒性KN99细胞的后续攻击感染具有强大的保护反应。结论:这些发现强调了生长过程中培养基和pH值在塑造新形态C.细胞壁的内容和组织中的重要性,以及它们对真菌毒力和宿主反应的影响。
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Cell wall composition in Cryptococcus neoformans is media dependent and alters host response, inducing protective immunity.

Introduction: Cryptococcus neoformans is a basidiomycete fungus that can cause meningoencephalitis, especially in immunocompromised patients. Cryptococcus grows in many different media, although little attention has been paid to the role of growth conditions on the cryptococcal cell wall or on virulence.

Objective: The purpose of this study was to determine how different media influenced the amount of chitin and chitosan in the cell wall, which in turn impacted the cell wall architecture and host response.

Methods: Yeast extract, peptone, and dextrose (YPD) and yeast nitrogen base (YNB) are two commonly used media for growing Cryptococcus before use in in vitro or in vivo experiments. As a result, C. neoformans was grown in either YPD or YNB, which were either left unbuffered or buffered to pH 7 with MOPS. These cells were then labeled with cell wall-specific fluorescent probes to determine the amounts of various cell wall components. In addition, these cells were employed in animal virulence studies using the murine inhalation model of infection.

Results: We observed that the growth of wild-type C. neoformans KN99 significantly changes the pH of unbuffered media during growth. It raises the pH to 8.0 when grown in unbuffered YPD but lowers the pH to 2.0 when grown in unbuffered YNB (YNB-U). Importantly, the composition of the cell wall was substantially impacted by growth in different media. Cells grown in YNB-U exhibited a 90% reduction in chitosan, the deacetylated form of chitin, compared with cells grown in YPD. The decrease in pH and chitosan in the YNB-U-grown cells was associated with a significant increase in some pathogen-associated molecular patterns on the surface of cells compared with cells grown in YPD or YNB, pH 7. This altered cell wall architecture resulted in a significant reduction in virulence when tested using a murine model of infection. Furthermore, when heat-killed cells were used as the inoculum, KN99 cells grown in YNB-U caused an aberrant hyper-inflammatory response in the lungs, resulting in rapid animal death. In contrast, heat-killed KN99 cells grown in YNB, pH 7, caused little to no inflammatory response in the host lung, but, when used as a vaccine, they conferred a robust protective response against a subsequent challenge infection with the virulent KN99 cells.

Conclusion: These findings emphasize the importance of culture media and pH during growth in shaping the content and organization of the C. neoformans cell wall, as well as their impact on fungal virulence and the host response.

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