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捕食线虫真菌单端孢属细胞的蛋白质组。

Proteome of the nematode-trapping cells of the fungus Monacrosporium haptotylum.

机构信息

Microbial Ecology, Department of Biology, Lund University, Lund, Sweden.

出版信息

Appl Environ Microbiol. 2013 Aug;79(16):4993-5004. doi: 10.1128/AEM.01390-13. Epub 2013 Jun 14.

DOI:10.1128/AEM.01390-13
PMID:23770896
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3754708/
Abstract

Many nematophagous fungi use morphological structures called traps to capture nematodes by adhesion or mechanically. To better understand the cellular functions of adhesive traps, the trap cell proteome of the fungus Monacrosporium haptotylum was characterized. The trap of M. haptotylum consists of a unicellular structure called a knob that develops at the apex of a hypha. Proteins extracted from knobs and mycelia were analyzed using SDS-PAGE and liquid chromatography-tandem mass spectrometry (LC-MS-MS). The peptide sequences were matched against predicted gene models from the recently sequenced M. haptotylum genome. In total, 336 proteins were identified, with 54 expressed at significantly higher levels in the knobs than in the mycelia. The upregulated knob proteins included peptidases, small secreted proteins with unknown functions, and putative cell surface adhesins containing carbohydrate-binding domains, including the WSC domain. Phylogenetic analysis showed that all upregulated WSC domain proteins belonged to a large, expanded cluster of paralogs in M. haptotylum. Several peptidases and homologs of experimentally verified proteins in other pathogenic fungi were also upregulated in the knob proteome. Complementary profiling of gene expression at the transcriptome level showed poor correlation between the upregulation of knob proteins and their corresponding transcripts. We propose that the traps of M. haptotylum contain many of the proteins needed in the early stages of infection and that the trap cells can tightly control the translation and degradation of these proteins to minimize the cost of protein synthesis.

摘要

许多食线虫真菌使用称为陷阱的形态结构通过黏附或机械方式捕获线虫。为了更好地理解黏附陷阱的细胞功能,对真菌 Monacrosporium haptotylum 的陷阱细胞蛋白质组进行了表征。M. haptotylum 的陷阱由一个称为节的单细胞结构组成,该结构在菌丝体的顶端发育。从节和菌丝体中提取的蛋白质使用 SDS-PAGE 和液相色谱-串联质谱 (LC-MS-MS) 进行分析。肽序列与最近测序的 M. haptotylum 基因组的预测基因模型相匹配。总共鉴定了 336 种蛋白质,其中 54 种在节中表达水平明显高于菌丝体。上调的节蛋白包括肽酶、具有未知功能的小分泌蛋白和包含碳水化合物结合结构域的假定细胞表面黏附素,包括 WSC 结构域。系统发育分析表明,所有上调的 WSC 结构域蛋白都属于 M. haptotylum 中一个大的、扩展的平行基因簇。一些肽酶和其他致病真菌中经过实验验证的蛋白质的同源物也在节蛋白质组中上调。转录组水平的基因表达互补分析表明,节蛋白的上调与它们相应的转录物之间相关性较差。我们提出,M. haptotylum 的陷阱包含感染早期所需的许多蛋白质,并且陷阱细胞可以严格控制这些蛋白质的翻译和降解,以最小化蛋白质合成的成本。

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