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Extraction of Extracellular Matrix in Static and Dynamic Candida Biofilms Using Cation Exchange Resin and Untargeted Analysis of Matrix Metabolites by Ultra-High-Performance Liquid Chromatography-Tandem Quadrupole Time-of-Flight Mass Spectrometry (UPLC-Q-TOF-MS)

机译:阳离子交换树脂在静态和动态念珠菌生物膜中提取细胞外基质超高效液相色谱-串联四极杆飞行时间质谱(UPLC-Q-TOF-MS)对基质代谢物进行无目标分析

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摘要

Fungal infections caused by Candida albicans poses a great threat to human health. The ability of biofilm formation is believed to be associated with resistance-related Candida infections. Currently, knowledge on extracellular matrix (EM) of C. albicans biofilm is limited. In this study, we introduced ion exchange resin, i.e., cation exchange resin (CER) and anion exchange resin (AER), in EM extraction of C. albicans biofilm as well as several non-albicans Candida (NAC) biofilms under static and dynamic states in combination with vortexing and ultrasonication (VU). The metabolites extracted from the dynamic C. albicans biofilm matrix using the CER-VU and VU were identified with ultra-high-performance liquid chromatography-tandem quadrupole time-of-flight mass spectrometry (UPLC-Q-TOF-MS) via untargeted filtration. Compared with other physical and chemical extraction methods, CER-VU was demonstrated to be an ideal approach with high-yield acquisitions of EM constituents including proteins, triglycerides and carbohydrates and low-level damages on fungal cell viability and integrity. The untargeted MS analysis further showed the high efficacy of CER-VU, as a large quantity of metabolites (217 versus 198) was matched comprising a great number of lipids, carbohydrates, amino acids, nucleic acids and their derivatives together with a high involvement of signaling pathways compared with the VU alone. However, combining the results from both the CER-VU and VU methods could generate more metabolites. In summary, the EM analysis of the dynamic C. albicans biofilm expands our understanding upon a comprehensive depiction of matrix components and provides another effective approach for EM extraction.
机译:白色念珠菌引起的真菌感染对人类健康构成了巨大威胁。生物膜形成的能力被认为与耐药相关的念珠菌感染有关。当前,关于白色念珠菌生物膜的细胞外基质(EM)的知识是有限的。在这项研究中,我们引入了离子交换树脂,即阳离子交换树脂(CER)和阴离子交换树脂(AER),用于在静电和动态条件下EM提取白色念珠菌生物膜以及几种非白色念珠菌(NAC)生物膜。涡旋和超声(VU)相结合的状态。通过超高效液相色谱-串联四极杆飞行时间质谱(UPLC-Q-TOF-MS)通过无目标过滤来鉴定使用CER-VU和VU从动态白色念珠菌生物膜基质中提取的代谢物。与其他物理和化学提取方法相比,CER-VU被证明是一种理想的方法,可以高收率地获得包括蛋白质,甘油三酸酯和碳水化合物在内的EM成分,并且对真菌细胞的生存力和完整性造成低水平的破坏。无目标MS分析进一步显示了CER-VU的高效率,因为匹配了包含大量脂质,碳水化合物,氨基酸,核酸及其衍生物的大量代谢产物(217与198),并且CER-VU的参与度很高。与仅VU相比的信号通路。但是,将CER-VU和VU方法的结果结合起来可以产生更多的代谢物。总之,动态白念珠菌生物膜的EM分析扩展了我们对基质成分的全面描述的理解,并提供了另一种有效的EM提取方法。

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