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生物膜分离的单核细胞增生李斯特菌在小鼠感染早期(12-24 小时)表现出系统传播减少。

Biofilm-isolated Listeria monocytogenes exhibits reduced systemic dissemination at the early (12-24 h) stage of infection in a mouse model.

机构信息

Molecular Food Microbiology Laboratory, Department of Food Science, Purdue University, West Lafayette, IN, USA.

Purdue Institute of Inflammation, Immunology and Infectious Disease, Purdue University, West Lafayette, IN, USA.

出版信息

NPJ Biofilms Microbiomes. 2021 Feb 8;7(1):18. doi: 10.1038/s41522-021-00189-5.

Abstract

Environmental cues promote microbial biofilm formation and physiological and genetic heterogeneity. In food production facilities, biofilms produced by pathogens are a major source for food contamination; however, the pathogenesis of biofilm-isolated sessile cells is not well understood. We investigated the pathogenesis of sessile Listeria monocytogenes (Lm) using cell culture and mouse models. Lm sessile cells express reduced levels of the lap, inlA, hly, prfA, and sigB and show reduced adhesion, invasion, translocation, and cytotoxicity in the cell culture model than the planktonic cells. Oral challenge of C57BL/6 mice with food, clinical, or murinized-InlA (InlA) strains reveals that at 12 and 24 h post-infection (hpi), Lm burdens are lower in tissues of mice infected with sessile cells than those infected with planktonic cells. However, these differences are negligible at 48 hpi. Besides, the expressions of inlA and lap mRNA in sessile Lm from intestinal content are about 6.0- and 280-fold higher than the sessle inoculum, respectively, suggesting sessile Lm can still upregulate virulence genes shortly after ingestion (12 h). Similarly, exposure to simulated gastric fluid (SGF, pH 3) and intestinal fluid (SIF, pH 7) for 13 h shows equal reduction in sessile and planktonic cell counts, but induces LAP and InlA expression and pathogenic phenotypes. Our data show that the virulence of biofilm-isolated Lm is temporarily attenuated and can be upregulated in mice during the early stage (12-24 hpi) but fully restored at a later stage (48 hpi) of infection. Our study further demonstrates that in vitro cell culture assay is unreliable; therefore, an animal model is essential for studying the pathogenesis of biofilm-isolated bacteria.

摘要

环境线索促进微生物生物膜的形成和生理及遗传异质性。在食品生产设施中,病原体产生的生物膜是食物污染的主要来源;然而,生物膜分离的固着细胞的发病机制尚不清楚。我们使用细胞培养和小鼠模型研究了固着李斯特菌(Lm)的发病机制。与浮游细胞相比,Lm 固着细胞表达的 lap、inlA、hly、prfA 和 sigB 水平降低,在细胞培养模型中的粘附、侵袭、易位和细胞毒性降低。用食物、临床或 murinized-InlA(InlA)菌株对 C57BL/6 小鼠进行口服攻毒,结果表明,在感染后 12 和 24 小时(hpi),感染固着细胞的小鼠组织中的 Lm 负荷比感染浮游细胞的小鼠低。然而,在 48 hpi 时,这些差异可以忽略不计。此外,肠道内容物中固着 Lm 的 inlA 和 lap mRNA 的表达分别比固着接种物高约 6.0-和 280 倍,这表明固着 Lm 在摄入后(12 h)仍能短暂上调毒力基因。同样,在 pH 为 3 的模拟胃液(SGF)和 pH 为 7 的模拟肠液(SIF)中暴露 13 小时,固着和浮游细胞的数量都等量减少,但诱导 LAP 和 InlA 表达和致病性表型。我们的数据表明,生物膜分离的 Lm 的毒力暂时减弱,并在感染的早期(12-24 hpi)在小鼠中被上调,但在后期(48 hpi)完全恢复。我们的研究进一步表明,体外细胞培养试验不可靠;因此,动物模型对于研究生物膜分离细菌的发病机制至关重要。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/943f/7870835/355897830301/41522_2021_189_Fig1_HTML.jpg

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