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首页> 外文期刊>Frontiers in Microbiology >Preliminary Transcriptome Analysis of Mature Biofilm and Planktonic Cells of Salmonella Enteritidis Exposure to Acid Stress
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Preliminary Transcriptome Analysis of Mature Biofilm and Planktonic Cells of Salmonella Enteritidis Exposure to Acid Stress

机译:酸胁迫下沙门氏菌肠炎沙门氏菌成熟生物膜和浮游细胞的转录组初步分析

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摘要

Salmonella has emerged as a well-recognized food-borne pathogen, with many strains able to form biofilms and thus cause cross-contamination in food processing environments where acid-based disinfectants are widely encountered. In the present study, RNA sequencing was employed to establish complete transcriptome profiles of Salmonella Enteritidis in the forms of planktonic and biofilm-associated cells cultured in Tryptic Soytone Broth (TSB) and acidic TSB (aTSB). The gene expression patterns of S . Enteritidis significantly differed between biofilm-associated and planktonic cells cultivated under the same conditions. The assembled transcriptome of S . Enteritidis in this study contained 5,442 assembled transcripts, including 3,877 differentially expressed genes (DEGs) identified in biofilm and planktonic cells. These DEGs were enriched in terms such as regulation of biological process, metabolic process, macromolecular complex, binding and transferase activity, which may play crucial roles in the biofilm formation of S . Enteritidis cultivated in aTSB. Three significant pathways were observed to be enriched under acidic conditions: bacterial chemotaxis, porphyrin-chlorophyll metabolism and sulfur metabolism. In addition, 15 differentially expressed novel non-coding small RNAs (sRNAs) were identified, and only one was found to be up-regulated in mature biofilms. This preliminary study of the S . Enteritidis transcriptome serves as a basis for future investigations examining the complex network systems that regulate Salmonella biofilm in acidic environments, which provide information on biofilm formation and acid stress interaction that may facilitate the development of novel disinfection procedures in the food processing industry.
机译:沙门氏菌已经成为公认的食源性病原体,许多菌株能够形成生物膜,从而在食品加工环境中引起交叉污染,而食品加工环境中普遍使用基于酸的消毒剂。在本研究中,RNA测序被用来建立完整的肠炎沙门氏菌转录组谱,其形式为在胰蛋白酶大豆肉汤(TSB)和酸性TSB(aTSB)中培养的浮游生物和生物膜相关细胞。拟南芥的基因表达模式。在相同条件下培养的生物膜相关细胞和浮游细胞之间,肠炎明显不同。 S的组装转录组。本研究中的肠炎沙门氏菌包含5,442个组装的转录本,包括在生物膜和浮游细胞中鉴定的3,877个差异表达基因(DEG)。这些DEG在诸如生物过程的调节,代谢过程,大分子复合物,结合和转移酶活性方面富集,这可能在S的生物膜形成中起关键作用。在aTSB中培养的肠炎沙门氏菌。观察到在酸性条件下富集了三个重要途径:细菌趋化性,卟啉-叶绿素代谢和硫代谢。此外,鉴定了15种差异表达的新型非编码小RNA(sRNA),在成熟的生物膜中仅发现一种上调。对S的初步研究。肠杆菌转录组可作为未来研究的基础,以检查在酸性环境中调节沙门氏菌生物膜的复杂网络系统,这些系统可提供有关生物膜形成和酸胁迫相互作用的信息,这可能有助于食品加工业中新型消毒程序的开发。

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