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利用定量质谱对铜绿假单胞菌PAO1全细胞的浮游和生物膜蛋白质组进行时间序列分析。

A temporal examination of the planktonic and biofilm proteome of whole cell Pseudomonas aeruginosa PAO1 using quantitative mass spectrometry.

作者信息

Park Amber J, Murphy Kathleen, Krieger Jonathan R, Brewer Dyanne, Taylor Paul, Habash Marc, Khursigara Cezar M

机构信息

Department of Molecular and Cellular Biology, University of Guelph, Guelph, Ontario, Canada;

出版信息

Mol Cell Proteomics. 2014 Apr;13(4):1095-105. doi: 10.1074/mcp.M113.033985. Epub 2014 Feb 16.

Abstract

Chronic polymicrobial lung infections are the chief complication in patients with cystic fibrosis. The dominant pathogen in late-stage disease is Pseudomonas aeruginosa, which forms recalcitrant, structured communities known as biofilms. Many aspects of biofilm biology are poorly understood; consequently, effective treatment of these infections is limited, and cystic fibrosis remains fatal. Here we combined in-solution protein digestion of triplicate growth-matched samples with a high-performance mass spectrometry platform to provide the most comprehensive proteomic dataset known to date for whole cell P. aeruginosa PAO1 grown in biofilm cultures. Our analysis included protein-protein interaction networks and PseudoCAP functional information for unique and significantly modulated proteins at three different time points. Secondary analysis of a subgroup of proteins using extracted ion currents validated the spectral counting data of 1884 high-confidence proteins. In this paper we demonstrate a greater representation of proteins related to metabolism, DNA stability, and molecular activity in planktonically grown P. aeruginosa PAO1. In addition, several virulence-related proteins were increased during planktonic growth, including multiple proteins encoded by the pyoverdine locus, uncharacterized proteins with sequence similarity to mammalian cell entry protein, and a member of the hemagglutinin family of adhesins, HecA. Conversely, biofilm samples contained an uncharacterized protein with sequence similarity to an adhesion protein with self-association characteristics (AidA). Increased levels of several phenazine biosynthetic proteins, an uncharacterized protein with sequence similarity to a metallo-beta-lactamase, and lower levels of the drug target gyrA support the putative characteristics of in situ P. aeruginosa infections, including competitive fitness and antibiotic resistance. This quantitative whole cell approach advances the existing P. aeruginosa subproteomes and provides a framework for identifying and studying entire pathways critical to biofilm biology in this model pathogenic organism. The identification of novel protein targets could contribute to the development of much needed antimicrobial therapies to treat the chronic infections found in patients with cystic fibrosis.

摘要

慢性多微生物肺部感染是囊性纤维化患者的主要并发症。晚期疾病中的主要病原体是铜绿假单胞菌,它会形成顽固的、有结构的群落,即生物膜。生物膜生物学的许多方面目前还了解甚少;因此,这些感染的有效治疗方法有限,囊性纤维化仍然是致命的。在这里,我们将三份生长匹配样本的溶液内蛋白质消化与高性能质谱平台相结合,以提供迄今为止已知的关于在生物膜培养物中生长的铜绿假单胞菌PAO1全细胞最全面的蛋白质组数据集。我们的分析包括蛋白质 - 蛋白质相互作用网络以及在三个不同时间点对独特且显著调节的蛋白质的PseudoCAP功能信息。使用提取离子流对一组蛋白质进行二次分析,验证了1884个高可信度蛋白质的光谱计数数据。在本文中,我们证明了在浮游生长的铜绿假单胞菌PAO1中,与代谢、DNA稳定性和分子活性相关的蛋白质有更多的表达。此外,几种与毒力相关的蛋白质在浮游生长期间增加,包括由绿脓菌素基因座编码的多种蛋白质、与哺乳动物细胞进入蛋白序列相似的未表征蛋白质,以及粘附素血凝素家族的成员HecA。相反,生物膜样本含有一种与具有自缔合特性的粘附蛋白序列相似的未表征蛋白质(AidA)。几种吩嗪生物合成蛋白水平升高、一种与金属β -内酰胺酶序列相似的未表征蛋白质,以及药物靶点gyrA水平降低,支持了原位铜绿假单胞菌感染的推定特征,包括竞争适应性和抗生素抗性。这种定量全细胞方法推进了现有的铜绿假单胞菌亚蛋白质组研究,并为识别和研究这种模式致病生物体中对生物膜生物学至关重要的整个途径提供了一个框架。新型蛋白质靶点的鉴定可能有助于开发急需的抗菌疗法,以治疗囊性纤维化患者的慢性感染。

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