Ethanolamine utilization supports Clostridium perfringens growth in infected tissues

Hirofumi Yagi; Haruyuki Nakayama-Imaohji; Hirofumi Nariya; Ayano Tada; Hisashi Yamasaki; Hideyo Ugai; Miad Elahi; Tsuneko Ono; Tomomi Kuwahara

doi:10.1016/j.micpath.2018.04.017

Ethanolamine utilization supports Clostridium perfringens growth in infected tissues

Microb Pathog. 2018 Jun:119:200-207. doi: 10.1016/j.micpath.2018.04.017. Epub 2018 Apr 11.

Authors

Hirofumi Yagi¹, Haruyuki Nakayama-Imaohji¹, Hirofumi Nariya², Ayano Tada¹, Hisashi Yamasaki³, Hideyo Ugai¹, Miad Elahi¹, Tsuneko Ono⁴, Tomomi Kuwahara⁵

Affiliations

¹ Department of Microbiology, Faculty of Medicine, Kagawa University, 1750-1 Miki, Kagawa, 761-0793, Japan.
² Laboratory of Food Microbiology and Hygiene, Graduate School of Biosphere Science, Hiroshima University, 1-4-4 Kagamiyama, Higashi-Hiroshima, 739-8528, Japan.
³ Division of Biology, Hyogo College of Medicine, Mukogawa, Nishinomiya, 663-8501, Japan.
⁴ Department of Molecular Microbiology, Institute of Health Biosciences, Tokushima University Graduate School, 3-18-15 Kuramoto-cho, Tokushima, 770-8503, Japan.
⁵ Department of Microbiology, Faculty of Medicine, Kagawa University, 1750-1 Miki, Kagawa, 761-0793, Japan. Electronic address: tomomi@med.kagawa-u.ac.jp.

PMID: 29654901
DOI: 10.1016/j.micpath.2018.04.017

Abstract

Clostridium perfringens possesses the ethanolamine (EA) utilization (eut) system encoded within the eut operon, which utilizes the EA as a carbon, nitrogen and energy source. To determine the role of the eut system in C. perfringens growth, an in-frame deletion of the eutABC genes was made in strain HN13 to generate the eutABC-deleted mutant strain HY1701. Comparison of HN13 and HY1701 growth in media supplemented with 1.0% glucose and/or 1.0% EA showed that glucose enhanced the growth of both strains, whereas EA enhanced HN13 growth, but not that of HY1701, indicating that the eut system is necessary for C. perfringens to utilize EA. The two-component regulatory system EutVW is needed to induce eut gene expression in response to EA whereas the global virulence regulator VirRS differentially controlled eut gene expression depending on glucose and EA availability. To assess the role of the eut system in vivo, an equal number of HN13 and HY1701 cells were injected into the right thigh muscles of mice. Mice infected with HY1701 showed fewer symptoms than those injected with HN13. The mortality rate of mice infected with HY1701 tended to be lower than for mice infected with HN13. In addition, in infected tissues from mice injected with a mixture of HN13 and HY1701, HN13 outnumbered HY1701. PCR screening demonstrated that C. perfringens isolated from gas gangrene and sporadic diarrhea cases carried both eut genes and the perfringolysin O gene (pfoA) as well as the phospholipase C gene (plc). However, pfoA was not detected in isolates from food poisoning patients and healthy volunteers. Culture supernatants prepared from HN13 grown in media containing 7.5% sheep red blood cells induced significantly higher eutB expression levels compared to those from plc- and/or pfoA-deletion mutants. Together, these results indicate that the eut system plays a nutritional role for C. perfringens during histolytic infection.

Keywords: Clostridium perfringens; Ethanolamine; Gas gangrene; Growth; Mouse model.

MeSH terms

Animals
Bacterial Toxins / genetics
Clostridium perfringens / genetics
Clostridium perfringens / growth & development*
Clostridium perfringens / metabolism*
Clostridium perfringens / pathogenicity*
Disease Models, Animal
Ethanolamine / metabolism*
Foodborne Diseases / microbiology
Gas Gangrene / metabolism*
Gene Expression Regulation, Bacterial
Genes, Bacterial / genetics
Hemolysin Proteins / genetics
Humans
Hydroxocobalamin / antagonists & inhibitors
Male
Mice
Mortality
Operon
Sequence Deletion
Sheep
Type C Phospholipases / genetics
Virulence

Substances

Bacterial Toxins
Hemolysin Proteins
Ethanolamine
Clostridium perfringens theta-toxin
Type C Phospholipases
Hydroxocobalamin