Translocation of Yersinia enterocolitica across reconstituted intestinal epithelial monolayers is triggered by Yersinia invasin binding to β1 integrins apically expressed on M‐like cells

Yersinia enterocolitica cross the intestinal epithelium via translocation through M cells, which are located in the follicle‐associated epithelium (FAE) of Peyer's patches (PP). To investigate the molecular basis of this process, studies were performed using a recently developed in vitro model, in which the enterocyte‐like cell line Caco‐2 and PP lymphocytes are co‐cultured in order to establish FAE‐like structures including M cells. Here, we demonstrate that Y. enterocolitica does not adhere significantly to the apical membrane of differentiated enterocyte‐like Caco‐2 cells that express binding sites for Ulex europaeus agglutinin (UEA)‐1. In contrast, Y. enterocolitica adhered to, and was internalized by, cells that lacked UEA‐1 binding sites and displayed a disorganized brush border. These cells were considered to be converted to M‐like cells. Further analysis revealed that part of these cells expressed β1 integrins at their apical surface and, as revealed by comparison of wild‐type and mutant strains, interacted with invasin of Y. enterocolitica . Consistently, anti‐β1 integrin antibodies significantly inhibited internalization of inv ‐expressing yersiniae. Experiments with Yersinia mutant strains deficient in YadA or Yop secretion revealed that these virulence factors play a minor role in this process. After internalization, yersiniae were transported within LAMP‐1‐negative vacuoles to, and released at, the basal surface. Internalization and transport of yersiniae was inhibited by cytochalasin D, suggesting that F‐actin assembly is required for this process. These results provide direct evidence that expression of β1 integrins at the apical surface of M cells enables interaction with the invasin of Y. enterocolitica , and thereby initiates internalization and translocation of bacteria.