Peer review process
Not revised: This Reviewed Preprint includes the authors’ original preprint (without revision), an eLife assessment, and public reviews.
Read more about eLife’s peer review process.Editors
- Reviewing EditorSophie HelaineHarvard Medical School, Boston, United States of America
- Senior EditorDominique Soldati-FavreUniversity of Geneva, Geneva, Switzerland
Reviewer #1 (Public review):
Shigella flexneri is a bacterial pathogen that is an important globally significant cause of diarrhea. Shigella pathogenesis remains poorly understood. In their manuscript, Saavedra-Sanchez et al report their discovery that a secreted E3 ligase effector of Shigella, called IpaH1.4, mediates the degradation of a host E3 ligase called RNF213. RNF213 was previously described to mediate ubiquitylation of intracellular bacteria, an initial step in their targeting of xenophagosomes. Thus, Shigella IpaH1.4 appears to be an important factor in permitting evasion of RNF213-mediated host defense.
Strengths:
The work is focused, convincing, well-performed, and important. The manuscript is well-written.
Reviewer #2 (Public review):
Summary:
The authors find that the bacterial pathogen Shigella flexneri uses the T3SS effector IpaH1.4 to induce degradation of the IFNg-induced protein RNF213. They show that in the absence of IpaH1.4, cytosolic Shigella is bound by RNF213. Furthermore, RNF213 conjugates linear and lysine-linked ubiquitin to Shigella independently of LUBAC. Intriguingly, they find that Shigella lacking ipaH1.4 or mxiE, which regulates the expression of some T3SS effectors, are not killed even when ubiquitylated by RNF213 and that these mutants are still able to replicate within the cytosol, suggesting that Shigella encodes additional effectors to escape from host defenses mediated by RNF213-driven ubiquitylation.
Strengths:
The authors take a variety of approaches, including host and bacterial genetics, gain-of-function and loss-of-function assays, cell biology, and biochemistry. Overall, the experiments are elegantly designed, rigorous, and convincing.
Weaknesses:
The authors find that ipaH1.4 mutant S. flexneri no longer degrades RNF213 and recruits RNF213 to the bacterial surface. The authors should perform genetic complementation of this mutant with WT ipaH1.4 and the catalytically inactive ipaH1.4 to confirm that ipaH1.4 catalytic activity is indeed responsible for the observed phenotype.
Reviewer #3 (Public review):
Summary:
In this study, the authors set out to investigate whether and how Shigella avoids cell-autonomous immunity initiated through M1-linked ubiquitin and the immune sensor and E3 ligase RNF213. The key findings are that the Shigella flexneri T3SS effector, IpaH1.4 induces degradation of RNF213. Without IpaH1.4, the bacteria are marked with RNF213 and ubiquitin following stimulation with IFNg. Interestingly, this is not sufficient to initiate the destruction of the bacteria, leading the authors to conclude that Shigella deploys additional virulence factors to avoid this host immune response. The second key finding of this paper is the suggestion that M1 chains decorate the mxiE/ipaH Shigella mutant independent of LUBAC, which is, by and large, considered the only enzyme capable of generating M1-linked ubiquitin chains.
Strengths:
The data is for the most part well controlled and clearly presented with appropriate methodology. The authors convincingly demonstrate that IpaH1.4 is the effector responsible for the degradation of RNF213 via the proteasome, although the site of modification is not identified.
Weaknesses:
The work builds on prior work from the same laboratory that suggests that M1 ubiquitin chains can be formed independently of LUBAC (in the prior publication this related to Chlamydia inclusions). In this study, two pieces of evidence support this statement -fluorescence microscopy-based images and accompanying quantification in Hoip and Hoil knockout cells for association of M1-ub, using an antibody, to Shigella mutants and the use of an internally tagged Ub-K7R mutant, which is unable to be incorporated into ubiquitin chains via its lysine residues. Given that clones of the M1-specific antibody are not always specific for M1 chains, and because it remains formally possible that the Int-K7R Ub can be added to the end of the chain as a chain terminator or as mono-ub, the authors should strengthen these findings relating to the claim that another E3 ligase can generate M1 chains de novo.
The main weakness relating to the infection work is that no bacterial protein loading control is assayed in the western blots of infected cells, leaving the reader unable to determine if changes in RNF213 protein levels are the result of the absent bacterial protein (e.g. IpaH1.4) or altered infection levels.
The importance of IFNgamma priming for RNF213 association to the mxiE or ipaH1.4 strain could have been investigated further as it is unclear if RNF213 coating is enhanced due to increased protein expression of RNF213 or another factor. This is of interest as IFNgamma priming does not seem to be needed for RNF213 to detect and coat cytosolic Salmonella.
Overall, the findings are important for the host-pathogen field, cell-autonomous/innate immune signaling fields, and microbial pathogenesis fields. If further evidence for LUBAC independent M1 ubiquitylation is achieved this would represent a significant finding.