Molecular Biology & Microbial Food Safety, ‡Mass Spectrometry of Biomacromolecules, and §Biosystems Data Analysis, Swammerdam Institute for Life Sciences, University of Amsterdam , Science Park 904, 1098 XH Amsterdam, The Netherlands.
J Proteome Res. 2018 Feb 2;17(2):903-917. doi: 10.1021/acs.jproteome.7b00732. Epub 2018 Jan 4.
Spores of Bacillus cereus pose a threat to food safety due to their high resistance to the heat or acid treatments commonly used to make food microbiologically safe. Spores may survive these treatments and later resume growth either on foodstuffs or, after ingestion, upon entering the gut they are capable of producing toxins, which cause either vomiting or diarrhea. The outer layers of the spore, the spore coat and exosporium, consist primarily of proteins that may serve as potential biomarkers for detection. The major morphogenetic protein CotE is important for correct assembly and attachment of the outermost layer, the exosporium, and by extension retention of many proteins. However, characterization of the proteins affected by deletion of CotE has been limited to electrophoretic patterns. Here we report the effect of CotE deletion on the insoluble fraction of the spore proteome through liquid chromatography-Fourier transform tandem mass spectrometry (LC-FTMS/MS) analysis. A total of 560 proteins have been identified in both mutant and wild-type spore coat isolates. A further 163 proteins were identified exclusively in wild-type spore isolates indicating that they are dependent on CotE for their association with the spore. Several of these are newly confirmed as associated with the exosporium, namely BC_2569 (BclF), BC_3345, BC_2427, BC_2878, BC_0666, BC_2984, BC_3481, and BC_2570. A total of 153 proteins were only identified in ΔCotE spore isolates. This was observed for proteins that are known or likely to be interacting with or are encased by CotE. Crucial spore proteins were quantified using a QconCAT reference standard, the first time this was used in a biochemically heterogeneous system. This allowed us to determine the absolute abundance of 21 proteins, which spanned across three orders of magnitude and together covered 5.66% ± 0.51 of the total spore weight. Applying the QconCAT methodology to the ΔCotE mutant allowed us to quantify 4.13% ± 0.14 of the spore total weight and revealed a reduction in abundance for most known exosporium associated proteins upon CotE deletion. In contrast, several proteins, either known or likely to be interacting with or encased by CotE (i.e., GerQ), were more abundant. The results obtained provide deeper insight into the layered spore structure such as which proteins are exposed on the outside of the spore. This information is important for developing detection methods for targeting spores in a food safety setting. Furthermore, protein stoichiometry and determination of the abundance of germination mediating enzymes provides useful information for germination and outgrowth model development.
蜡样芽胞杆菌的孢子由于对食品微生物安全常用的热处理或酸处理具有很高的抗性,因此对食品安全构成威胁。孢子可能在这些处理中存活下来,然后在食品上重新生长,或者在摄入后进入肠道时,能够产生毒素,导致呕吐或腹泻。孢子的外层,即孢子壳和外孢囊,主要由蛋白质组成,这些蛋白质可能是潜在的检测生物标志物。主要形态发生蛋白 CotE 对于最外层外孢囊的正确组装和附着很重要,并且通过扩展保留了许多蛋白质。然而,对 CotE 缺失影响的蛋白质的表征仅限于电泳图谱。在这里,我们通过液相色谱 - 傅里叶变换串联质谱法 (LC-FTMS/MS) 分析报告了 CotE 缺失对孢子蛋白组的不可溶性部分的影响。在突变体和野生型孢子壳分离物中总共鉴定出 560 种蛋白质。另外 163 种蛋白质仅在野生型孢子分离物中鉴定出,表明它们依赖 CotE 与孢子结合。其中一些是新确认的与外孢囊相关的,即 BC_2569(BclF)、BC_3345、BC_2427、BC_2878、BC_0666、BC_2984、BC_3481 和 BC_2570。总共 153 种蛋白质仅在 CotE 缺失的孢子分离物中鉴定出。这是在已知或可能与 CotE 相互作用或被 CotE 包裹的蛋白质中观察到的。使用 QconCAT 参考标准对关键的孢子蛋白进行了定量,这是首次在生化异质系统中使用。这使我们能够确定 21 种蛋白质的绝对丰度,这些蛋白质跨越三个数量级,总共占孢子总重量的 5.66%±0.51。将 QconCAT 方法应用于 CotE 突变体允许我们定量分析孢子总重量的 4.13%±0.14,并显示 CotE 缺失后大多数已知的外孢囊相关蛋白的丰度降低。相比之下,一些蛋白质,无论是已知的还是可能与 CotE 相互作用或被 CotE 包裹的蛋白质(即 GerQ),丰度更高。所获得的结果提供了对分层孢子结构的更深入了解,例如哪些蛋白质暴露在孢子的外部。这对于开发针对食品安全中孢子的检测方法非常重要。此外,发芽介导酶的蛋白质化学计量和丰度的确定为发芽和生长模型的开发提供了有用的信息。
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