Abstract
The type VI secretion (T6S) system is a molecular device for the delivery of proteins from one cell into another. T6S function depends on the contractile sheath comprised of TssB/VipA and TssC/VipB proteins. We previously reported on a mutant variant of TssB that disrupts T6S-dependent export of the self-identity protein, IdsD, in the bacterium Proteus mirabilis. Here we determined the mechanism underlying that initial observation. We show that T6S-dependent export of multiple self-recognition proteins is abrogated in this mutant strain. We have mapped the mutation, which is a single amino acid change, to a region predicted to be involved in the formation of the TssB-TssC sheath. We have demonstrated that this mutation does indeed inhibit sheath formation, thereby explaining the global disruption of T6S activity. We propose that this mutation could be utilized as an important tool for studying functions and behaviors associated with T6S systems.
Introduction
Type VI secretion (T6S) systems, widely found among Gram-negative bacteria, are cell-puncturing devices that deliver cargo proteins from one cell into another or into the environment (1-22). T6S function, and ultimately cargo delivery, depends on a contractile sheath made up of TssB/VipA (Pfam family PF05591) and TssC/VipB (Pfam family PF05943) proteins (6, 23, 24). TssB and TssC bind one another to form protomers, which in turn assemble into the contractile sheath (25-27). Subcellular visualization of the T6S machinery has relied on the fusion of TssB to fluorescent proteins such as superfolder Green Fluorescent Protein (sfGFP) and mCherry, thereby allowing the detection of sheath dynamics and interactions between TssB and TssC, as well as measuring the active firing of T6S machines within a population (4-6, 17, 18, 28-32). While many model systems for T6S contain multiple loci encoding different T6S machines, Proteus mirabilis strain BB2000 is one of many less-studied organisms with a single T6S system and single alleles for TssB (BB2000_0821) and TssC (BB2000_0820) (33, 34). We have previously reported that a point mutation in BB2000_0821 results in the blocked export of proteins belonging to the Ids recognition system (35). This mutation lies in an unstructured region of the TssB monomer that was previously unexamined. Here we show that the identified point mutation disrupts global T6S export function. Based on published structures of the TssB-TssC sheath in other organisms, we mapped the point mutation to a region involved in sheath formation (25-27). We specifically demonstrate that this point mutation inhibits sheath polymerization and that this is the likely mechanism for disrupted T6S export. Since this single point mutation disrupts global T6S function without disrupting the structure of the operon, and likely the core membrane components, we posit that the mutation provides a valuable tool for studying T6S-associated phenotypes in multiple organisms.
Materials and Methods
Bacterial strains and media
Strains and plasmids used in this study are described in Table 1. P. mirabilis strains were maintained on LSW- agar (36). CM55 blood agar base agar (Oxoid, Basingstoke, England) was used for swarm-permissive nutrient plates. Overnight cultures of all strains were grown in LB broth under aerobic conditions at 37°C. Antibiotics used were: 35 microgram/milliliter (μg/ml) kanamycin, 50 μg/ml chloramphenicol, 15 μg/ml tetracycline, and 25 μg/ml streptomycin. Kanamycin was added for plasmid maintenance where appropriate.
Construction of strains Δids::tssBwt-sfgfp and Δids::tssBmut-sfgfp
BB2000-derived Δids::tssBwt-sfgfp and Δids::tssBmut-sfgfp were constructed using 5’-GATTAGCAGCAATATCGAGCTC-3’ as the forward and 5’-GCGCGCTCTAGACCTTAAGTTAAACCAAATATAGCTG-3’ as the reverse primer to amplify BB2000_0821, encoding the P. mirabilis TssB homolog, and its upstream region from genomic DNA of the wild-type strain BB2000 (36) or of the BB2000-derived mutant strain Δids::tssBmut (35). The polymerase chain reaction (PCR) product was digested with DpnI (New England Biolabs, Ipswich, MA). Overlap extension PCR (43) was used to combine the PCR product and a gBlock (Integrated DNA Technologies, Inc., Coralville, IA) containing the gene encoding sfGFP (gBlock sequence: 5’CGCGGGCCCGGTATTACCCCATAAATAGTGCTCATGGTCTTGTTTAACATTTTCTG AATAGTTAAACATTTTTACAGGGTTTTCTGTTGGAGAGTATGGCAAACGTAATAAGA AACGCGGTGCTGTTAACCCTAAATAACGGGAATCTTCTGCTTCACGCAGTGAGCGCC ATTTAGTGTGTGCAGGGCCTTCAAAAACAGATTTTAGATCTTTAATTGCCGGCAGTT CAGCGTAGCTATTAATACCAAAGAAATTAGGTGAAACAGATGATAGGAATGGCGCG TGAGCCATTGCACCAACAGTACTAACATACTGCATTAACTTCATATCTGGCGCAGTA TTGTTAAAGGCGTAGTTACCAATAACTGTTGCAACAGGTTCACCACCAAATTGGCCG TATCCTGAAGAGTAGACGTGTTGATAGAAGCCTGATTGAACAATTTCTGGAGAAAAT TCAAAATCTTCTAATAACTCTTCTTTAGTTGCATGAAGAATATTGATCTTAATATTTT CTCTAAAATCAGTGCGATCAACGAGTAATTTTAAAGAACGCCATGAAGCTTCAATTT CTTGAAATTTAGGCGCGTGAAGAATTTCGTCAACTTGAGTACTTAGTTTATTATCAA GTTCAACAAGCATTTTATCGATTAATAATCGATTGATCTGTTGGTCTTCAGATTCACT GGCGAAAATATTACTAATAAAAGCAGCAACACCTTGTTTGGCAATATCGTATGCTTC TGTTTCTGGAGACATACGTGATTGAGCCATAATTTCATCAAGTAAAGAGCCTGTAGA TGCGGGGGCTTGTTGCTCTTGAGCTTCTGCATTTAGTGACATGAAATAATCCTCTATA AACATTATTTGTAGAGCTCATCCATGCCATGTGTAATCCCAGCAGCAGTTACAAACT CAAGAAGGACCATGTGGTCACGCTTTTCGTTGGGATCTTTCGAAAGGACAGATTGTG TCGACAGGTAATGGTTGTCTGGTAAAAGGACAGGGCCATCGCCAATTGGAGTATTTT GTTGATAATGGTCTGCTAGTTGAACGGAACCATCTTCAACGTTGTGGCGAATTTTGA AGTTAGCTTTGATTCCATTCTTTTGTTTGTCTGCCGTGATGTATACATTGTGTGAGTT AAAGTTGTACTCGAGTTTGTGTCCGAGAATGTTTCCATCTTCTTTAAAATCAATACCT TTTAACTCGATACGATTAACAAGGGTATCACCTTCAAACTTGACTTCAGCACGCGTC TTGTAGGTCCCGTCATCTTTGAAAGATATAGTGCGTTCCTGTACATAACCTTCGGGC ATGGCACTCTTGAAAAAGTCATGCCGTTTCATGTGATCCGGATAACGGGAAAAGCAT TGAACACCATAGGTCAGAGTAGTGACAAGTGTTGGCCATGGAACAGGTAGTTTTCC AGTAGTGCAAATAAATTTAAGGGTGAGTTTTCCGTTTGTAGCATCACCTTCACCCTCT CCACGGACAGAAAATTTGTGCCCATTAACATCACCATCTAATTCAACAAGAATTGGG ACAACTCCAGTGAAAAGTTCTTCTCCTTTGCTTCCTCCTCCAGCAGCAGCTTTTTGAT TAGCAGCAATATCGAGCTC-3’). 5’CGCGGGCCCGGTATTACCCCATAAATAGTGC-3’ and 5’-GCGCGCTCTAGACCTTAAGTTAAACCAAATATAGCTG -3’ were used as the forward and reverse primers, respectively. Restriction digestion with ApaI and XbaI (New England Biolabs, Ipswich, MA) was used to introduce the overlap extension PCR product into the suicide vector pKNG101 (41). The resulting vectors pCS48a (tssBmut-sfgfp) and pCS48b (tssBwt-sfgfp) were introduced into the mating strain E. coli SM10λpir (42) and then mated into BB2000-derived Δids (39). The resultant matings were subjected to antibiotic selection using tetracycline and streptomycin on LSW- agar. Candidate strains were subjected to sucrose counter-selection to select for clones that integrated the target DNA sequence into the chromosome in exchange for the wild-type DNA sequence (44). 5’-GCCATCAACATCAAGTACTTTG-3’ and 5’-CATGAGCAGTCCAAATTGATC-3’ were used as the forward and reverse primers, respectively, to amplify the exchanged chromosomal regions by colony PCR. PCR reactions were purified and the entire exchanged region was sequenced to confirm strains. Sequencing was performed by GENEWIZ, Inc. (South Plainfield, NJ).
Trichloroacetic acid precipitations, SDS-PAGE, and LC-MS/MS
Trichloroacetic acid precipitations were performed as previously described (34). Gel fragments corresponding to molecular weights of approximately 10 to 20, 20 to 40, 40 to 60 and 60 to 250 kilodaltons (kDa) were excised and subjected to liquid chromatography-mass spectrometry/mass spectrometry (LC-MS/MS), which was performed by the Taplin Biological Mass Spectrometry Facility (Harvard Medical School, Boston, MA).
Colony expansion and co-swarm inhibition assays
Overnight cultures were normalized to an optical density at 600 nm (OD600) of 0.1 and swarm-permissive nutrient plates were inoculated with one microliter (μl) of normalized culture. Plates were incubated at 37 °C for 16 hours, and radii of actively migrating swarms were measured. Additionally, widths of individual swarm rings within the swarm colonies were recorded.
For co-swarm inhibition assays, strains were processed as described and mixed at a ratio of 1:1 where indicated. Swarm-permissive nutrient plates supplemented with Coomassie Blue (20 μg/ml) and Congo Red (40 μg/ml) were inoculated with one μl of normalized culture/culture mixes. Plates were incubated at 37 °C until boundary formation was visible by eye.
Modeling of TssBwt and TssBL32R
Swiss-Model (45-48) was used for all modeling, and the atomic model, PDB ID: 3j9g (from http://www.rcsb.org (25, 49, 50)) was used as a template. Resulting .pdb files were modified in PyMOL v1.8.4.1 (51).
Microscopy
One millimeter thick swarm-permissive agar pads were inoculated directly from overnight cultures. The agar pads were incubated at 37 °C in a modified humidity chamber. After 4.5 – 5.5 hours, the pads were imaged by phase contrast as well as epifluorescence microscopy using a Leica DM5500B (Leica Microsystems, Buffalo Grove, IL) and a CoolSnap HQ2 cooled CCD camera (Photometrics, Tucson, AZ). MetaMorph version 7.8.0.0 (Molecular Devices, Sunnyvale, CA) was used for image acquisition.
Western blotting
To test for the production of the sfGFP-fused proteins, cells were isolated from swarm-permissive nutrient plates supplemented with chloramphenicol after 16-20 hours, resuspended in 5 ml LB broth, and normalized to an OD600 of 1. Cells were pelleted by centrifugation and the pellet was resuspended in sample buffer and boiled. Samples were separated by gel electrophoresis using 12% Tris-tricine polyacrylamide gels, transferred onto 0.45 micrometer nitrocellulose membranes, and probed with polyclonal rabbit anti-GFP (1:4000, ThermoFisher Scientific, Waltham, MA) or mouse anti-σ70 (1:1000, BioLegend, San Diego,CA, catalog number 663202) followed by goat anti-rabbit or goat anti-mouse conjugated to horseradish peroxidase. The polyclonal rabbit anti-GFP antibody was supplied at a concentration of 2 mg/ml (Thermo Fisher Scientific, Waltham, MA, catalog number A-11122, immunogen: GFP from jellyfish Aequorea Victoria). The goat anti-mouse secondary antibody was used at a 1:5000 dilution (KPL, Inc., Gaithersburg, MD, catalog number 214-1806) as was the goat anti-rabbit secondary (KPL, Inc., Gaithersburg, MD, catalog number 074-1506). A Precision Plus ProteinTM Dual Color Standards molecular size marker (Bio-Rad Laboratories, Inc., Hercules, CA) was included as a size control. Membranes were developed with the Immun-Star HRP Substrate Kit (Bio-Rad Laboratories, Hercules, CA) and visualized using a Chemidoc (Bio-Rad Laboratories, Hercules, CA). TIFF images were exported and figures were made in Adobe Illustrator (Adobe Systems, San Jose, CA).
Results
The tssB mutant strain does not export self-recognition proteins
Several self-recognition proteins in P. mirabilis strain BB2000 are exported by its T6S system; these include the Hcp (Pfam family PF05638) homologs IdsA and IdrA, the VgrG (Pfam family PF05954) homologs IdsB and IdrB, and the self-identity protein IdsD (34). We previously reported that a strain expressing a point mutation (L32R) from gene BB2000_0821, which encodes the P. mirabilis TssB homolog, results in the lack of IdsA, IdsB, and IdsD export (35). To determine whether global T6S export was disrupted or whether the defect was specific to proteins belonging to the Ids system, we examined the Idr-specific secretion profile of the mutant strain. We collected supernatants of liquid-grown cells producing either TssBwt or TssBL32R. These supernatants were subjected to trichloroacetic acid precipitations followed by LC-MS/MS analysis. We identified peptides belonging to IdrA (Hcp), IdrB (VgrG) and the putative Idr effector IdrD in the supernatants of the wild type, but not of the mutant strain (Table 2).
To confirm these secretion profiles, we employed an in vivo assay for Idr self-recognition activity. The Idr proteins contribute to inter-strain competitions during swarm migration (34), which is a highly coordinated, flagella-based social motility in P. mirabilis (52-54). Briefly, the assay consists of mixing two different strains of P. mirabilis at a 1:1 ratio and allowing for swarm migration; at the completion of swarm migration, one strain dominates over the other and thus occupies the outer edges of the swarm colony (34). The dominating strain can be identified by swarm boundary formation assays in which two genetically identical strains merge to form a single larger swarm, while two genetically distinct strains remain separate and form a visible boundary (Fig 1A) (39, 55-57). P. mirabilis strain BB2000 dominates over the genetically distinct strain HI4320, permitting BB2000 to occupy the outer edges of a mixed swarm colony, which thus merges with the swarm colony of BB2000 and forms a boundary with the swarm colony of HI4320 (34). Absence of Idr proteins or of T6S in BB2000 allows for HI4320 to dominate the mixed swarm instead (34). Loss of the Ids proteins in BB2000 has no effect (34). We therefore performed these assays using BB2000-derived strains that lack the Ids proteins (Δids) and produce either TssBwt or the mutant TssBL32R. As a control, we used the BB2000-derived strain, icmF*, which contains a disruption in the gene encoding the T6S core membrane component TssM/IcmF (Pfam family PF12790); this mutant strain is defective for T6S function (33, 34). As expected, Δids producing TssBwt dominated over strain HI4320, and conversely, strain HI4320 dominated over icmF* (Fig 1B). Δids producing the mutant TssBL32R did not dominate over HI4320 (Fig 1B), indicating that Idr-dependent inter-strain competition was disrupted in this strain. As co-swarm inhibition of HI4320 by BB2000-derived strains is dependent on the export of Idr self-recognition proteins, we conclude that a strain producing TssBL32R is defective in the export of Idr proteins. Together, the secretion profile and swarm assays support that this mutation (TssBL32R) causes a global loss in T6S export activity.
The L32R mutation in the TssB homolog prohibits sheath formation
To understand the disrupted T6S export, we modeled the P. mirabilis BB2000 T6S sheath structure on a published structure of the Vibrio cholerae T6S sheath (25) (Fig 2). We then mapped the L32R point mutation onto this P. mirabilis model structure (Fig 2). The point mutation causes a hydrophobic leucine at position 32 to be substituted with a positively charged arginine, which has a larger side chain and different electrochemical properties (Fig 2A). Amino acid 32 maps to an unstructured region between the first two beta sheets of TssB (Figs 2B, 2C) (25, 26). The first beta sheet is involved in interactions between TssB-TssC protomers that hold together the strands of the sheath helix, while the second beta sheet is involved in TssB-TssC interactions within individual protomers (Figs 2B, 2C) (25, 26). Given the position within the T6S sheath, we hypothesized that the L32R mutation interferes with sheath formation.
We introduced the mutation into a Δids strain producing TssB fused to sfGFP to directly observe sheath formation in vivo. To validate the functionality of this tool in P. mirabilis strain BB2000, we examined the ability of the TssB-sfGFP variants to export self-recognition proteins using established assays. We subjected Δids::tssBwt-sfgfp and Δids::tssBmut-sfgfp to Idr-dependent inter-strain competitions with strain HI4320 as described above. Surprisingly, HI4320 dominated over both strains (Fig 3A), which suggested that T6S export is impaired in both strains. A more quantitative assay for T6S function is a swarm expansion assay using the Ids proteins; in this assay, a reduced swarm colony radius indicates that the self-identity determinant IdsD has been exported and that T6S is functional (35). As previously reported (35), the presence of wild-type TssB results in a reduced swarm colony radius, while disrupted T6S function due to the presence of TssBL32R leads to a larger swarm colony radius (Fig 3B). We examined the strain producing TssBwt-sfGFP and found that its swarm colony radius was modestly increased in comparison to that of the strain producing untagged TssBwt (Fig 3B); therefore, fusion of sfGFP to TssBwt caused a modest reduction in T6S function. Interestingly, the reduced functionality of TssBwt-sfGFP in comparison to TssBwt was sufficient to prevent a BB2000-derived strain to outcompete HI4320 in the idr-specific co-swarm assay (Fig 3A), further supporting earlier observations of distinct functions for Ids and Idr proteins (34). As expected, the strain producing TssBL32R-sfGFP exhibited an even larger swarm colony radius, similar to that of a strain producing untagged TssBL32R (Fig 3B). This observation demonstrates a lack of T6S export (35) and thus confirms that strains producing TssBL32R do no export the T6S substrate, IdsD.
We next employed the TssB-sfGFP tool to determine the ability of the mutant TssB variant to support T6S sheath formation, thereby testing the hypothesis that TssBL32R does not support sheath formation. Fluorescence associated with TssBwt-sfGFP appears in multiple discrete (short or elongated) structures throughout cells on swarm-permissive agar (Fig 4A). This fluorescence pattern is consistent with previous reports for TssB-sfGFP (6, 59). In cells producing the mutant fusion protein, diffuse fluorescence signal was present, and no elongated structures or puncta were observed (Fig 4A). Therefore, the discrete structures, thought to be sheaths, did not form. To further examine whether the discrete fluorescence was likely representative of assembled T6S sheaths, we produced TssBwt-sfGFP in the icmF* strain, which lacks the membrane-associated complex of the T6S machinery and which we thus predicted to lack sheaths. Again we observed that fluorescence was diffuse in these cells (Fig 4A), indicating the likely absence of sheath formation.
A possible explanation for the diffuse fluorescence pattern in a strain producing TssBL32R-sfGFP could be that the mutant TssB is less stable than the wild-type variant, which could result in the cleavage of sfGFP from the fusion protein and ultimately a diffuse signal. We examined whole cell extracts that were collected from swarming colonies and then subjected these extracts to western blotting followed by incubation with anti-GFP antibodies. We found no striking differences among the strains producing wild-type or mutant TssB-sfGFP (Fig 4B). For both strains, we observed a dominant band corresponding to the size of the TssB-sfGFP fusion protein and a fainter band corresponding to the size of monomeric sfGFP (Fig 4B). This result suggests that while cleavage of the TssB-sfGFP fusion occurs, it does so for both the wild-type and mutant TssB-sfGFP variants. We conclude that cleavage of the sfGFP does not account for the differences in fluorescence patterns of these strains. Therefore, the L32R mutation in TssB is sufficient to prohibit sheath formation in P. mirabilis.
Discussion
Here we have described the critical contribution of a single residue in TssB for sheath formation and global T6S export activity. We have shown that a L32R mutation in the P. mirabilis TssB variant inhibits sheath assembly (Fig 4A) without altering relative amounts of this protein (Fig 4B). The mutated leucine residue in the P. mirabilis variant corresponds to amino acid 26 in the Pfam model, T6SS_TssB (Pfam family PF05591) (24, 60-62). Leucine 26 is highly conserved in available sequences for Enterobacterales and is also well conserved across the majority of Gammaproteobacteria; the conserved three amino acid sequence amongst Enterobacterales is E/Q-L-P (63-65). Remarkably, the leucine residues maps to an unstructured region between the first two predicted beta sheets of the TssB protein (Fig 2). While the two beta sheets flanking this residue are predicted to be involved in interactions with separate TssC monomers in structural models of the sheath (Fig 2), the contribution of the unstructured region was less apparent (25, 26). Upon closer evaluation, we posit that this leucine residue might contribute to a hydrophobic pocket (Fig 2D). A conversion to arginine then likely leads to both steric and electrostatic conflicts within this pocket (Fig 2E). The hydrophobic pocket and the examined leucine residue within it might be critical for interactions between TssB and TssC in individual protomers or alternatively, for interprotomer interactions of TssB and TssC that hold together the strands of the sheath helix. More examination is needed to elucidate these physical interactions. Nonetheless, the observation that the L32R mutation results in diffuse TssB-sfGFP signal within the cytoplasm (Fig 4A) supports the crucial role of this leucine for sheath assembly.
Visualization of sheath formation and its subcellular localization has proven valuable in multiple bacteria. TssB-sfGFP fusion proteins have been previously reported for Vibrio cholerae (6) and P. mirabilis strain HI4320 (59); the homologous TssB-sfGFP was designed equivalently in P. mirabilis strain BB2000 and introduced to the native locus on the chromosome replacing the wild-type allele. This sfGFP fusion protein showed reduced T6S function as compared to the wild-type variant (Fig 3). As similar defects were not reported previously (6, 59), we posit that possible differences in the protein sequences and tertiary structures between species and strains might be accentuated by the addition of sfGFP. Alternatively, these discrepancies in T6S on the species and strain level might reflect differences in the sensitivity of the respective assays chosen to detect T6S function (Fig 3). Regardless, the reduced T6S function in P. mirabilis strain BB2000 producing TssB-sfGFP appears to allow for greater visualization of elongated sheaths before disassembly (Fig 4). Elongated sheaths were stable over the course of the observation. Similar delayed dynamics might also be true for other microorganisms with nearly identical TssB sequences and a single T6S machinery such as Providencia sp. By contrast, TssB-sfGFP-containing sheaths rapidly transition between elongated structures and single foci during imaging in V. cholerae (4-6). Stable, elongated TssB-sfGFP structures, such as those observed in P. mirabilis BB2000, could be utilized for subcellular co-localization assays using epifluorescence microscopy or for structural examination of the T6S machinery via cryo-electron microscopy.
In conclusion, the L to R mutation has the potential to be an impactful tool, especially in bacteria with a single T6S machinery. We have found that the L32R point mutation in the TssB homolog from P. mirabilis strain BB2000 allows for the disruption of the T6S sheath, which in turn causes global T6S malfunction. These results provide insight into the importance of the TssB N-terminal region for sheath assembly, which has not been fully investigated, and highlights a critical residue that was previously overlooked. These data also complement a previous detailed analysis of the TssB C-terminal region (28). Last, the L to R mutation abrogates T6S function without disrupting the overall tss operon structure and without removing entire proteins from cells. As such, potential secondary effects that could convolute experimental outcomes are minimized and questions regarding the subcellular localization of T6S-associated components and protein-protein interactions can be answered in a nearly native state. Here, we show that this previously underappreciated residue is indeed crucial for sheath assembly and raise new questions of how unstructured regions within TssB contribute to TssB-TssC interactions.
Acknowledgments
We thank Dr. Thomas Bernhardt for the gift of the sfgfp sequence as well as Dr. Kenneth Skinner for helpful advice on the structural modeling. We also thank the members of Dr. Rachelle Gaudet’s research group, as well as the Gibbs research group, for thoughtful discussions.