Molecular Food Microbiology Laboratory, Department of Food Science, Purdue University, West Lafayette, IN 47907-2009, USA.
Infect Immun. 2010 Dec;78(12):5062-73. doi: 10.1128/IAI.00516-10. Epub 2010 Sep 27.
Listeria monocytogenes interaction with the intestinal epithelium is a key step in the infection process. We demonstrated that Listeria adhesion protein (LAP) promotes adhesion to intestinal epithelial cells and facilitates extraintestinal dissemination in vivo. The LAP receptor is a stress response protein, Hsp60, but the precise role for the LAP-Hsp60 interaction during Listeria infection is unknown. Here we investigated the influence of physiological stressors and Listeria infection on host Hsp60 expression and LAP-mediated bacterial adhesion, invasion, and transepithelial translocation in an enterocyte-like Caco-2 cell model. Stressors such as heat (41°C), tumor necrosis factor alpha (TNF-α) (100 U), and L. monocytogenes infection (10(4) to 10(6) CFU/ml) significantly (P < 0.05) increased plasma membrane and intracellular Hsp60 levels in Caco-2 cells and consequently enhanced LAP-mediated L. monocytogenes adhesion but not invasion of Caco-2 cells. In transepithelial translocation experiments, the wild type (WT) exhibited 2.7-fold more translocation through Caco-2 monolayers than a lap mutant, suggesting that LAP is involved in transepithelial translocation, potentially via a paracellular route. Short hairpin RNA (shRNA) suppression of Hsp60 in Caco-2 cells reduced WT adhesion and translocation 4.5- and 3-fold, respectively, while adhesion remained unchanged for the lap mutant. Conversely, overexpression of Hsp60 in Caco-2 cells enhanced WT adhesion and transepithelial translocation, but not those of the lap mutant. Furthermore, initial infection with a low dosage (10(6) CFU/ml) of L. monocytogenes increased plasma membrane and intracellular expression of Hsp60 significantly, which rendered Caco-2 cells more susceptible to subsequent LAP-mediated adhesion and translocation. These data provide insight into the role of LAP as a virulence factor during intestinal epithelial infection and pose new questions regarding the dynamics between the host stress response and pathogen infection.
李斯特菌与肠道上皮的相互作用是感染过程中的关键步骤。我们证明李斯特菌黏附蛋白(LAP)促进与肠道上皮细胞的黏附,并有助于李斯特菌在体内的肠外传播。LAP 的受体是应激反应蛋白 Hsp60,但 LAP-Hsp60 相互作用在李斯特菌感染过程中的精确作用尚不清楚。在这里,我们在肠上皮样 Caco-2 细胞模型中研究了生理应激和李斯特菌感染对宿主 Hsp60 表达和 LAP 介导的细菌黏附、入侵和跨上皮转运的影响。应激源,如热(41°C)、肿瘤坏死因子-α(TNF-α)(100 U)和李斯特菌感染(10(4)至 10(6)CFU/ml),显著增加(P < 0.05)Caco-2 细胞的质膜和细胞内 Hsp60 水平,从而增强 LAP 介导的李斯特菌黏附,但不增强李斯特菌对 Caco-2 细胞的入侵。在跨上皮转运实验中,野生型(WT)通过 Caco-2 单层的转运量比 lap 突变体高出 2.7 倍,这表明 LAP 参与跨上皮转运,可能通过旁细胞途径。Caco-2 细胞中 Hsp60 的短发夹 RNA(shRNA)抑制降低了 WT 的黏附和转运分别减少了 4.5 倍和 3 倍,而 lap 突变体的黏附保持不变。相反,Hsp60 在 Caco-2 细胞中的过表达增强了 WT 的黏附和跨上皮转运,但 lap 突变体则不然。此外,用低剂量(10(6)CFU/ml)李斯特菌初始感染可显著增加质膜和细胞内 Hsp60 的表达,使 Caco-2 细胞更容易受到随后的 LAP 介导的黏附和转运。这些数据深入了解了 LAP 在肠道上皮感染过程中作为毒力因子的作用,并提出了关于宿主应激反应与病原体感染之间动态关系的新问题。
