A Validation System for Selection of Bacteriophages against Shiga Toxin-Producing Escherichia coli Contamination

Agnieszka Necel,Aleksandra Dydecka,Sylwia Bloch,Grzegorz Węgrzyn,Alicja Węgrzyn,Bożena Nejman-Faleńczyk,Gracja Topka-Bielecka

doi:10.3390/toxins13090644

Abstract

Shiga toxin-producing Escherichia coli (STEC) can cause severe infections in humans, leading to serious diseases and dangerous complications, such as hemolytic-uremic syndrome. Although cattle are a major reservoir of STEC, the most commonly occurring source of human infections are food products (e.g., vegetables) contaminated with cow feces (often due to the use of natural fertilizers in agriculture). Since the use of antibiotics against STEC is controversial, other methods for protection of food against contaminations by these bacteria are required. Here, we propose a validation system for selection of bacteriophages against STEC contamination. As a model system, we have employed a STEC-specific bacteriophage vB_Eco4M-7 and the E. coli O157:H7 strain no. 86-24, bearing Shiga toxin-converting prophage ST2-8624 (Δstx2::cat gfp). When these bacteria were administered on the surface of sliced cucumber (as a model vegetable), significant decrease in number viable E. coli cells was observed after 6 h of incubation. No toxicity of vB_Eco4M-7 against mammalian cells (using the Balb/3T3 cell line as a model) was detected. A rapid decrease of optical density of STEC culture was demonstrated following addition of a vB_Eco4M-7 lysate. However, longer incubation of susceptible bacteria with this bacteriophage resulted in the appearance of phage-resistant cells which predominated in the culture after 24 h incubation. Interestingly, efficiency of selection of bacteria resistant to vB_Eco4M-7 was higher at higher multiplicity of infection (MOI); the highest efficiency was evident at MOI 10, while the lowest occurred at MOI 0.001. A similar phenomenon of selection of the phage-resistant bacteria was also observed in the experiment with the STEC-contaminated cucumber after 24 h incubation with phage lysate. On the other hand, bacteriophage vB_Eco4M-7 could efficiently develop in host bacterial cells, giving plaques at similar efficiency of plating at 37, 25 and 12 °C, indicating that it can destroy STEC cells at the range of temperatures commonly used for vegetable short-term storage. These results indicate that bacteriophage vB_Eco4M-7 may be considered for its use in food protection against STEC contamination; however, caution should be taken due to the phenomenon of the appearance of phage-resistant bacteria.

Highlights

The vast majority of Escherichia coli strains are commensals living in the gut of animals, including humans
Efficiency of the anti-bacterial activity of the phage lysate was observed for each tested multiplicity of infection (MOI) value, ranging from 0.0001 to 10 (Figure 2)
Efficiency of the anti-bacterial activity of the phage lysate was observed for each tested MOI value, ra4nogfi1n4g from 0.0001 to 10 (Figure 2)

Summary

Introduction

The vast majority of Escherichia coli strains are commensals living in the gut of animals, including humans. They belong to natural intestinal microbiota and are harmless to their hosts under healthy conditions. Shiga toxins are major virulence factors of STEC. They are AB5-type protein toxins, consisting of two types of subunits, A and B. Following endocytosis and retro-translocation from Golgi apparatus to endoplasmic reticulum, the A subunit is liberated into the cytoplasm. It acts as a specific enzyme causing removal of one of adenine residues in 28S rRNA which inactivates ribosome function [4]

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