Characterization of Lysozyme-Like Effector TseP Reveals the Dependence of Type VI Secretion System (T6SS) Secretion on Effectors in Aeromonas dhakensis Strain SSU

Xiaoye Liang; Tong-Tong Pei; Zeng-Hang Wang; Weiliang Xiong; Li-Li Wu; Ping Xu; Shuangjun Lin; Tao G Dong

doi:10.1128/AEM.00435-21

Characterization of Lysozyme-Like Effector TseP Reveals the Dependence of Type VI Secretion System (T6SS) Secretion on Effectors in Aeromonas dhakensis Strain SSU

Appl Environ Microbiol. 2021 May 26;87(12):e0043521. doi: 10.1128/AEM.00435-21. Epub 2021 May 26.

Authors

Xiaoye Liang^#¹, Tong-Tong Pei^#¹, Zeng-Hang Wang¹, Weiliang Xiong¹, Li-Li Wu¹, Ping Xu¹, Shuangjun Lin¹, Tao G Dong^{1

2}

Affiliations

¹ State Key Laboratory of Microbial Metabolism, Joint International Research Laboratory of Metabolic & Developmental Sciences, School of Life Sciences and Biotechnology, Shanghai Jiao Tong University, Shanghai, China.
² Department of Ecosystem and Public Health, University of Calgary, Calgary, Alberta, Canada.

^# Contributed equally.

Abstract

The type VI secretion system (T6SS) is a widespread weapon employed by Gram-negative bacteria for interspecies interaction in complex communities. Analogous to a contractile phage tail, the double-tubular T6SS injects toxic effectors into prokaryotic and eukaryotic neighboring cells. Although effectors dictate T6SS functions, their identities remain elusive in many pathogens. Here, we report the lysozyme-like effector TseP in Aeromonas dhakensis, a waterborne pathogen that can cause severe gastroenteritis and systemic infection. Using secretion, competition, and enzymatic assays, we demonstrate that TseP is a T6SS-dependent effector with cell wall-lysing activities, and TsiP is its cognate immunity protein. Triple deletion of tseP and two known effector genes, tseI and tseC, abolished T6SS-mediated secretion, while complementation with any single effector gene partially restored bacterial killing and Hcp secretion. In contrast to whole-gene deletions, the triple-effector inactivation in the 3eff_c mutant abolished antibacterial killing but not T6SS secretion. We further demonstrate that the 3eff_c mutation abolished T6SS-mediated toxicity of SSU to Dictyostelium discoideum amoebae, suggesting that the T6SS physical puncture is nontoxic to eukaryotic cells. These data highlight not only the necessity of possessing functionally diverse effectors for survival in multispecies communities but also that effector inactivation would be an efficient strategy to detoxify the T6SS while preserving its delivery efficiency, converting the T6SS to a platform for protein delivery to a variety of recipient cells. IMPORTANCE Delivery of cargo proteins via protein secretion systems has been shown to be a promising tool in various applications. However, secretion systems are often used by pathogens to cause disease. Thus, strategies are needed to detoxify secretion systems while preserving their efficiency. The T6SS can translocate proteins through physical puncture of target cells without specific surface receptors and can target a broad range of recipients. In this study, we identified a cell wall-lysing effector, and by inactivating it and the other two known effectors, we have built a detoxified T6SS-active strain that may be used for protein delivery to prokaryotic and eukaryotic recipient cells.

Keywords: effector; interspecies interaction; pathogen; protein secretion; virulence.

MeSH terms

Aeromonas* / genetics
Aeromonas* / metabolism
Bacterial Proteins* / genetics
Bacterial Proteins* / metabolism
Cell Wall
Dictyostelium
Escherichia coli / genetics
Muramidase* / genetics
Muramidase* / metabolism
Phagocytosis
Type VI Secretion Systems* / genetics
Type VI Secretion Systems* / metabolism

Substances

Bacterial Proteins
Type VI Secretion Systems
Muramidase

Supplementary concepts

Aeromonas dhakensis