This is an uncorrected proof.
The two-component signalling system (TCS) comprising a histidine kinase (HK) and a response regulator (RR) is the predominant bacterial sense-and-response machinery. Because bacterial cells usually encode a number of TCSs to adapt to various ecological niches, the specificity of a TCS is in the centre of regulation. Specificity of TCS is defined by the capability and velocity of phosphoryl transfer between a cognate HK and a RR. Here, we provide genetic, enzymology and structural data demonstrating that the second messenger cyclic-di-GMP physically and specifically binds to RavS, a HK of the phytopathogenic, gram-negative bacterium Xanthomonas campestris pv. campestris. The [c-di-GMP]-RavS interaction substantially promotes specificity between RavS and RavR, a GGDEF–EAL domain-containing RR, by reinforcing the kinetic preference of RavS to phosphorylate RavR. [c-di-GMP]-RavS binding effectively decreases the phosphorylation level of RavS and negatively regulates bacterial swimming. Intriguingly, the EAL domain of RavR counteracts the above regulation by degrading c-di-GMP and then increasing the level of phosphorylated RavS. Therefore, RavR acts as a bifunctional phosphate sink that finely controls the level of phosphorylated RavS. These biochemical processes interactively modulate the phosphoryl flux between RavS-RavR and bacterial lifestyle transition. Our results revealed that c-di-GMP acts as an allosteric effector to dynamically modulate specificity between HK and RR.
c-di-GMP is a multifunctional bacterial second messenger that controls various physiological processes. The nucleotide derivative binds to riboswitches or proteins as effectors during regulation. Here, we found that c-di-GMP physically binds to a histidine kinase, RavS, of a plant pathogenic bacterium. The binding event significantly enhanced the phosphotransferase activity of RavS to phosphorylate a response regulator, RavR. This process tightly modulates the phosphorylation level of RavS, which is important to the lifestyle transition of the bacterium between virulence and swimming motility. Therefore, our results reveal that c-di-GMP controls the bacterial two-component signalling, one of the dominant mechanisms of bacterial cells in adaptation to various environmental stimuli.
Citation: Cheng S-T, Wang F-F, Qian W (2019) Cyclic-di-GMP binds to histidine kinase RavS to control RavS-RavR phosphotransfer and regulates the bacterial lifestyle transition between virulence and swimming. PLoS Pathog 15(8): e1007952. https://doi.org/10.1371/journal.ppat.1007952
Editor: Nian Wang, University of Florida Institute of Food and Agricultural Sciences, UNITED STATES
Received: November 17, 2018; Accepted: June 30, 2019; Published: August 13, 2019
Copyright: © 2019 Cheng et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Data Availability: All relevant data are within the manuscript and its Supporting Information files.
Funding: This work was supported by the Ministry of Science and Technology of China (Grant No. 2016YFD0100602 to WQ, http://www.most.gov.cn/), the Strategic Priority Research Program of the Chinese Academy of Sciences (Grant No. XDB11040700 to WQ, www.cas.ac.cn), the National Natural Science Foundation of China (Grants Nos. 31825021, 31671989, 31600062 and 31370127 to WQ, http://www.nsfc.gov.cn/), and the State Key Laboratory of Plant Genomics (to WQ, http://plantgenomics.genetics.cas.cn/). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
The two-component signalling system (TCS) is one of the predominant molecular machineries used by almost all bacteria to monitor and adaptively respond to environmental cues [1, 2]. The prototypical TCS is composed of a membrane-bound histidine kinase (HK) and a cytosolic response regulator (RR). Upon detecting a stimulus, HK autophosphorylates an invariant histidine residue within its dimerization and histidine phosphotransfer (DHp) domain and then catalyses the transfer of the phosphoryl group onto a conserved aspartic acid within the receiver (REC) domain of the cognate RR . The activated RR then modulates bacterial adaptation by controlling gene transcription or cellular behaviour [4, 5]. There is a high level of specificity between a HK and its cognate RR, which is quantified by the kinetic preference during phosphotransfer [6, 7]. The complexity of TCS regulation was revealed after three decades of extensive investigations. Bacterial cells dynamically and elegantly regulate time, rhythm, space and flux of the phosphotransfer between the HK and RR to adapt to diverse ecological niches . For example, hybrid-type HK-mediated phosphorelay, phosphatases, auxiliary proteins and small RNAs are involved in TCS regulation [9–13].
Cyclic di-GMP (c-di-GMP) is a ubiquitous second messenger involved in regulating bacterial physiology [14–17]. This signalling chemical interacts with riboswitches or protein as effectors to control a diverse set of processes, such as virulence, biofilm formation, motility, cell division and quorum-sensing [18–20]. The c-di-GMP effectors include the PilZ family of proteins, transcription factors, ATPases, transporters and various metabolic enzymes [15, 21, 22]. Intrinsically, the TCS is extensively involved in c-di-GMP signalling because approximately 6% of bacterial RRs encode three types of protein modules that control c-di-GMP turnover . Among them, GGDEF domains have diguanylate cyclase activity to biosynthesize c-di-GMP from two GTP molecules , whereas EAL or HD-GYP domains contains phosphodiesterase activities to degrade c-di-GMP into pGpG or GMP, respectively [23–25]. Some RRs encoding degenerate GGDEF or EAL domains can act as c-di-GMP receptors [14, 26]. Recently, c-di-GMP was found to interact directly with CckA, an essential HK regulating cell division of Caulobacter crescentus, to inhibit kinase activity and activate phosphatase activity of CckA, which triggers DNA replication and initiation of the cell cycle [27–29]. This evidence indicates that c-di-GMP and TCS signalling are tightly associated. However, how c-di-GMP modulates the specificity between HKs and RRs and the biological significance of this signalling crosstalk remain unresolved.
The gram-negative bacterium Xanthomonas campestris pv. campestris is a model organism for studying plant pathology. This bacterium is the causative agent of black rot disease in various cruciferous plants and causes substantial loss of vegetable production yields worldwide . The X. campestris pv. campestris genome encodes a large number of TCS proteins (approximately 52 HKs and 54 RRs) , and a number of these proteins, including RpfC-RpfG, RavS-RavR and PcrK-PcrR, are regulators of bacterial virulence that are associated with c-di-GMP turnover [32–36]. Among these regulators, RavS-RavR was reported to constitute a putative TCS. RavS is a membrane-bound HK with two tandem PAS domains as potential intracellular sensors, and RavR is a RR that contains N-terminal degenerate GGDEF and EAL domains . In the vicinity of the ravR-ravS locus, a HK gene named ravA was identified and encodes a protein that may phosphorylate RavR . Inactivation of ravA and ravR causes a significant decrease in virulence [37, 38]. Therefore, RavS-RavA-RavR is likely to form a “three-component signalling system” that most likely has complex associations and outputs. However, the regulatory relationship and protein phosphorylation processes among RavS-RavA-RavR, and the potential role of c-di-GMP in the dynamics of the signalling system, remain unknown.
In this study, we reveal that c-di-GMP regulates the HK-RR phosphotransfer flux. c-di-GMP physically binds to the catalytic and ATP-binding domain (CA) of RavS to significantly enhance the phosphotransferase activity of RavS towards RavR. This process efficiently decreases the phosphorylation level of RavS. In controlling bacterial swimming and flagellar development, the REC domain of RavR acts as a highly efficient phosphate sink to decrease the phosphorylated RavS level, which is subject to the control of c-di-GMP. Epistasis analysis also revealed that unlike typical TCSs, the RR RavR is upstream of the HK RavS in regulation. In addition, the EAL domain of RavR degrades c-di-GMP to reduce the RavS-RavR phosphotransfer, thereby maintaining a high level of phosphorylated RavS. Therefore, RavR subtly modulates the phosphorylation level of RavS, which is critical in controlling bacterial swimming and flagellar biogenesis. In this process, c-di-GMP controls the phosphotransfer flux from the HK to the RR and plays a critical role during the lifestyle transition between swimming and bacterial virulence.
ravA-ravR and ravS control bacterial virulence, flagellar development and swimming motility
The genomic organization of ravS, ravR and ravA and the putative structures of their products are shown in Fig 1A. Western blotting revealed that RavS is located in the membrane and cytoplasm, and that RavR is a cytoplasmic protein (Fig 1B). Although RavA does not contain a recognisable transmembrane helix, repeated experiments showed that RavA is also located in both the membrane and cytoplasm (Fig 1B), which suggests that the HK has a membrane-anchored peptide or that the protein contains an unrecognised transmembrane region. Semi-quantitative western blotting demonstrated that the estimated ratio of RavA:RavR:RavS is approximately 10:29:17, amounting to approximately 1890, 5510 and 3230 molecules, respectively, in a bacterial cell grown under the tested conditions (Fig 1C and S1 Fig). The estimated concentrations of RavA, RavR and RavS in a cell were 2.05 ± 0.53, 5.99 ± 0.46, and 3.51 ± 0.27 μM, respectively (average bacterial cell volume was defined as 1.53 ± 0.23 μM3). This HK:RR ratio is remarkably higher than the general trend observed that RR molecules are often several dozen times more than the HK .
(a) Genomic organisation of ravARS genes and putative secondary structures of their protein products. Protein secondary structures were predicted by the SMART program. TrM: transmembrane domain; PAS: Per-ARNT-Sim domain; DHp: dimerisation and histidine phosphotransfer domain; CA: catalytic and ATP binding domain; REC: receiver domain. GGDEF and EAL domains are also shown. (b) Subcellular localisation of RavA, RavR and RavS. Western blotting was used to detect the proteins in different subcellular fractions. The known membrane-bound RpfC and cytoplasmic HPPK were detected as controls. (c) The ratio of RavA, RavR and RavS proteins in bacterial cells. Semi-quantitative western blotting was used to estimate the levels of these proteins (n = 3). (b) and (c), each experiment was repeated three times. (d–e) Mutation of ravA and ravR rather than ravS attenuated bacterial virulence significantly. (d) Bacterial virulence against host plant Brassica oleracea cv Zhonggan 11. Strains were inoculated onto plant leaves by scissor cutting. The lesion length was recorded 10 d after inoculation. The negative control was an inoculation of 10 mM MgCl2. EV: empty vector. (e) Quantification of the lesion length in (d). Average lengths and standard deviations are shown. Asterisk: significant difference, as tested by Student’s t-test (P ≤ 0.05, n = 30 inoculation sites). (f) Extracellular polysaccharide (EPS) production of bacterial strains. EPS production was measured as the dry weight of EPS vs. the dry weight of bacterial cells. Asterisk: significant difference, as tested by Student’s t-test (P ≤ 0.05, n = 3). (g–h) Swimming motility of bacterial strains. (g) Bacterial strains were inoculated in NYG plates containing 0.15% agar and grown at 28°C for 28 h. (h) Average diameters of the migration zones of (g). Asterisk: significant difference, as tested by Student’s t-test (P ≤ 0.05, n = 10).
To further investigate the roles of ravA, ravR and ravS in controlling physiological processes, we performed phenotypic profiling of the in-frame deletion mutants of ΔravA, ΔravR and ΔravS. These mutants have phenotypes similar to those of the wild-type (WT) strain in growth in rich NYG medium, secretion of extracellular enzymes and resistance to oxidative stress (S2 Fig). However, these mutants exhibited remarkable but differing phenotypic changes in bacterial virulence and motility. Deletion of ravA and ravR substantially decreased bacterial virulence against the host plant Brassica oleracea cv. Zhonggan 11 (Fig 1D and 1E). Genetic complementation of the two genes, whose expression levels were controlled by their native promoters, fully or partially restored virulence to levels of the WT strain (Fig 1D and 1E). Although deletion of ravS has no impact on bacterial virulence, a genetic complementary strain (ΔravS-ravS) showed significant attenuation in virulence (Fig 1D and 1E), which might be caused by overexpression of ravS in a medium-copy, broad-host vector (pHM2). Accordingly, the production of extracellular polysaccharides (EPS), a major virulence determinate of X. campestris pv. campestris, decreased significantly to 43% and 42% of the levels of the WT strain in the ΔravA and ΔravR mutants, respectively, whereas the EPS levels were similar to the WT strain in their genetic complementary strains (Fig 1F). EPS production remained nearly unchanged in the ravS null mutant but decreased significantly in the ravS complementary strain (31% compared with that of the WT strain, (Fig 1F)). These results indicate that ravA and ravR are positive regulators of bacterial virulence but overexpression of ravS decreased bacterial virulence.
As shown in Fig 1G and 1H, compared with the WT, deletions of ravA and ravR increased swimming motility by approximately two-fold, but deletion of ravS almost completely eradicated the swimming capability of the mutant. Genetic complementation successfully restored the observed deficiencies to levels similar to that of WT strain (Fig 1G and 1H). Since bacterial swimming motility is controlled mainly by flagella, bacterial flagella were observed by transmission electron microscopy (TEM). As measured by the flagellar cell ratio (Fig 2A and 2B), ravA (flagellar cell ratio = 71.6%) and ravR (77.1%) mutant strains had a higher frequency of flagella in cells and significantly longer flagella than observed in the WT strain (32.5%). The average flagellar lengths of ΔravA and ΔravR mutant strains and the WT strain were 4.60, 4.84 and 2.82 μm (Fig 2C), respectively. However, inactivation of ravS resulted in complete loss of flagella (Fig 2A–2C). Genetic complementation of ravA, ravR or ravS in the corresponding mutant significantly suppressed these deficiencies in flagellar morphology.
(a) Morphology of bacterial flagella. Bacterial flagella were observed by transmission electron microscopy after negative staining. A representative image of each strain is shown (n > 30). Upper panel: bacterial population profile; lower panel: morphology of a single bacterium. (b) Ratio of bacteria with flagella. For each strain, cells with flagella were counted for three biological replicates with each containing at least 100 cells. (c) The average flagellar length of bacterial strains. The length was measured using the AutoCAD software. Three biological replicates were taken with each comprising at least 30 measurements. (d) The fliC mRNA level in bacterial strains. The level of fliC mRNA was measured by qRT-PCR. Amplification of cDNA from tmRNA was used as an internal control. The experiment was repeated three times and the result of a representative experiment is shown. In (b–d), standard deviations are provided; asterisk: significant difference, as tested by Student’s t-test (P ≤ 0.05).
ravA-ravR-ravS is located in the vicinity of gene clusters that encode flagella-associated proteins and may regulate the expression of these genes (S3 Fig). We selected eight genes to examine their transcription levels in various strains and found that fliC (encoding flagellin) is a representative gene that is controlled by ravA-ravR-ravS (S3A Fig). Deletion of ravA and ravR significantly increased the mRNA levels of fliC to 363% and 402% of the levels of the WT strain, respectively (Fig 2D). In contrast, mutation of ravS caused a significant decrease in the fliC transcription level to 5.6% of the level of the WT strain, while genetic complementation of ravS increased fliC mRNA to 253% of the level of the WT strain (Fig 2D). Based on these results, in controlling the development of bacterial flagella and fliC transcription, both ravA and ravR act as negative regulators but ravS is a positive regulator.
In addition, because type III secretion (T3SS) genes (hrp) are critical in virulence of X. campestris, we selected three hrp cluster genes (hrpD, hrpF and hrpG) to measure their expression levels. As shown in S3C Fig, the mRNA levels of hrpF did not have remarkable change in the ravR and ravA mutants. However, the amounts of hrpG and hrpD transcripts were significantly decreased comparing to the WT strain. Therefore, we further analysed the expression level of hrpG because HrpG is an OmpR-family response regulator to control the transcription of an AraC-family transcription factor HrpX, and the latter binds to the plant inducible promoters (PIP) of some hrp gene clusters to modulate the expressions of these T3SS genes [30, 40]. In the ravR and ravA mutants, the hrpG transcripts significantly decreased to the 5.2% and 2.2% levels of the WT strain, while genetic complementation of the two genes restored the hrpG expression to 111.1% and 75.6% levels of the WT strain (S3D Fig). This result reveals that ravR and ravA positively modulate the transcription of hrpG.
ravS is genetically downstream of ravA–ravR in regulating bacterial swimming
Epistatic analysis was performed to dissect the regulatory relationships among ravR and ravA or ravS. Although deletion of ravA or ravR significantly decreased the bacterial virulence and production of EPS (Fig 1), the double mutants (ΔravA-ΔravS or ΔravR-ΔravS) exhibited virulence levels similar to those of the WT strain (Fig 3A and 3B and S4A Fig). Similarly, inactivation of ravS effectively suppressed the increased swimming motility, flagellar cell ratio and flagellar length that were caused by ravA or ravR deletion (Fig 3C–3E, and S4B and S4C Fig). The fliC expression level of the ravA or ravR mutant was increased significantly (Fig 2D). However, in the double mutants, fliC mRNA levels decreased significantly to the level of ΔravS (Fig 3F). Furthermore, two double mutants on ΔravA and ΔravR backgrounds were constructed with the conserved phosphorylation residue (His500) of RavS substituted by Ala (ΔravA-ravSH500A and ΔravR-ravSH500A). The phenotypic changes in the single mutant ravSH500A were similar to those observed for the ΔravS mutant, and in the double mutants, analyses revealed that the ravSH500A point mutation effectively suppressed all the tested phenotypic deficiencies that were caused by the ravA or ravR deletion (Fig 3A–3F and S4A–S4C Fig). Collectively, these genetic results suggest that ravS is downstream of ravR and ravA in regulation. The point mutant ravSH500A, in which RavS is constitutively dephosphorylated, exhibits reduced swimming capacity, which suggests that a high level of phosphorylated RavS (RavS~P) positively controls bacterial swimming but negatively modulates virulence. Furthermore, the suppressive function of ravS depends completely on the function of the conserved His500 residue, which suggests that RavA and RavR may negatively regulate the RavS~P level in the epistasis relationship.
(a–f) Deletion of ravS or the ravSH500A point mutation effectively suppressed the phenotypic deficiencies of X. campestris pv. campestris caused by ravA or ravR mutations. (a) Bacterial virulence measured by the lesion length on leaves. Bacterial strains were inoculated onto plant leaves of Brassica oleracea cv Zhonggan 11. The lesion length was recorded 10 d after inoculation (n = 30). (b) Production of extracellular polysaccharides (EPS). EPS production was quantified as the ratio of dry weight of EPS vs. the dry weight of bacterial cells (n = 3). (c) Bacterial swimming motility measured by the diameters of swimming zones. Bacterial strains were inoculated in NYG plates containing 0.15% agar and grown at 28°C for 28 h. The average diameters of the migration zones were measured (n = 10). (d) Ratio of bacterial cells with flagella. For each strain, cells with flagella were counted (n = 100). (e) The average flagellar length of bacterial strains (n = 30). (f) fliC mRNA levels in bacterial strains. The level of fliC mRNA was measured by qRT-PCR. Amplification of cDNA from tmRNA was used as an internal control. The experiment was repeated three times and the result of a representative experiment is shown. In (a–f), standard deviations are provided; asterisk: significant difference, as tested by Student’s t-test (P ≤ 0.05).
The EAL domain of RavR positively regulates RavS-mediated bacterial swimming in an Asp496-dependent manner
Intriguingly, the RR RavR is upstream of RavS (HK) in regulation. The protein has an EAL domain and a GGDEF domain that associated with c-di-GMP turnover. Using 32P-labelled c-di-GMP produced by a tDGC cyclase (S5A Fig) , we confirmed that the EAL domain of RavR can form a homodimer in vitro and has phosphodiesterase activity to degrade c-di-GMP into pGpG, which depends on the E-A-L motif of the domain (Fig 4A, S5B Fig and S5C Fig). The GGDEF signature motif of RavR is degenerate as “GSDEM” and did not have diguanylate cyclase activity to synthesize c-di-GMP from GTP (S5B Fig), suggest that RavR does not encode cyclase activity. Phosphorylation of RavR by RavA did not affect its phosphodiesterase activity (S5D Fig and S5E Fig), consistent with the result that inactivation of two HK genes (ravS or ravA) did not remarkably affect the intracellular concentration of c-di-GMP (S5F Fig). Additionally, deletion of the coding sequences of the EAL domain or ravR gene increased the intracellular c-di-GMP to 185.9% and 150.0% of the level of the WT strain, respectively (Fig 4B). These results suggest RavR mainly acts as a phosphodiesterase.
(a) RavR and its EAL domain have phosphodiesterase activities to degrade c-di-GMP. 32P-labelled c-di-GMP was synthesised by tDGC cyclase in vitro. None or 5 μM purified proteins were added to the PDE reaction mixture with 1 μM 32P-labelled c-di-GMP, and reactions were incubated at 28°C for 30 min. Samples were analysed on thin-layer chromatography plates. (b) Deletion of coding sequences of the EAL domain and ravR increased intracellular c-di-GMP concentrations. Cellular c-di-GMP was extracted from 5 mL mid-log phase bacterial cells (OD600 = 0.8) and quantified by HPLC-MS/MS. (a, b) Each experiment was conducted three times. (c, d) Bacterial virulence assay. (c) Bacterial strains were inoculated onto plant leaves of Brassica oleracea cv Zhonggan 11. (d) The lesion length was recorded 10 d after inoculation (n = 30). (e) Production of extracellular polysaccharides (EPS). Bacterial strains were grown in TGM medium at 28°C for 72 h before EPS quantification, which was calculated as the dry weight of EPS vs. the dry weight of bacterial cells (n = 3). (f, g) Bacterial swimming motility. (f) Bacterial strains were inoculated in NYG plates containing 0.15% agar and grown at 28°C for 28 h. (g) Average diameters of the migration zones were measured (n = 10). (h–j) Morphology of bacterial flagella. (h) Bacterial flagella were observed by TEM. A representative image of each strain is shown. Upper panel: bacterial population profile; lower panel: a single bacterium. (i) Ratio of bacterial cells with flagella. For each strain, cells with flagella were counted (n = 100). (j) The average flagellar length of bacterial strains (n = 30). (k) fliC mRNA level in bacterial strains. The level of fliC mRNA was measured by qRT-PCR. Amplification of cDNA from tmRNA was used as an internal control. The experiment was repeated three times and the result of a representative experiment is shown. Standard deviations are provided; asterisk: significant difference, as tested by Student’s t-test (P ≤ 0.05).
We further genetically analysed the interaction between the phosphor-receiving domain (REC) and the EAL domain of RavR and their regulatory relationship in controlling ravS. Similar to the null mutant of ravR (ΔravR), point mutation of the conserved Asp496 residue within the REC domain of RavR decreased bacterial virulence and EPS production (Fig 4C–4E) but increased bacterial swimming (Fig 4F and 4G), flagellar cell ratio (Fig 4H and 4I), flagellar length (Fig 4J) and the transcriptional level of fliC (Fig 4K), which suggests that phosphorylation residue Asp496 of RavR is indispensable for regulation.
Surprisingly, inactivation of RavR phosphodiesterase activity by an in-frame deletion of the coding sequence of its EAL domain (ravRΔEAL) caused phenotypic changes that were completely different from those of the ravR null mutant (ΔravR) or ravRD496A point mutant. The virulence level and EPS production of ravRΔEAL were unaffected (Fig 4C–4E) rather than reduced. The swimming motility of the ravRΔEAL mutant was reduced significantly (Fig 4F and 4G) rather than showing a dramatic increase that was observed for ΔravR or the ravRD496A mutant. TEM analysis revealed the absence of flagellum in the bacterial cells of the ravRΔEAL mutant; thus, its flagellar cell ratio was zero (Fig 4H–4J). Additionally, the fliC mRNA level of the ravRΔEAL mutant was reduced significantly (Fig 4K). We then constructed a double mutant of ravRΔEAL(D496A) to investigate the epistatic relationship between the EAL domain and Asp496. ravRΔEAL(D496A) phenocopied the ravRD496A mutant displaying a decrease in virulence and EPS production but increases in swimming capability, flagellar length, flagellar cell ratio and fliC transcription level (Fig 4A–4K). This genetic evidence suggests that RavR has two opposite functions in regulating bacterial swimming. Full-length RavR negatively controls swimming and flagellar development in an Asp496-dependent manner, whereas its EAL domain positively controls swimming and flagellar development. Additionally, epistatic analysis revealed that the phosphorylation of Asp496 potentially downstream of the PDE activity of EAL domain in regulating bacterial swimming. The biochemical relationship will be dissected in the following experiments.
Based on the above results, the genetic code of the conserved His500 residue of the downstream HK gene ravS was mutated on the backgrounds of ravRD496A and ravRΔEAL(D496A) to construct triple mutants. As predicted, the pattern of phenotypic changes in these three triple mutants was suppressed by the mutation and similar to that of ΔravS or ravSH500A (Fig 4A–4K).
Both RavA and RavS phosphorylate RavR
The phosphorylation process and regulation of RavA-RavR-RavS have not been investigated previously. In vitro phosphorylation assays using autoradiography and Phos-tag gel analysis revealed that full-length RavA autophosphorylates its conserved RavAHis164 residue because the RavAH564A substitution completely inactivated RavA autophosphorylation (S6A Fig, S6B Fig and S6D Fig). The addition of RavR or RavRΔEAL into the reaction mixture remarkably decreased the RavA phosphorylation level (RavA~P), although no recognisable signal of phosphorylated RavR (RavR~P or RavRΔEAL~P) was detected in autoradiography (S6A Fig, S6B Fig and S6D Fig). Recombinant RavR with a conserved Asp496 substitution did not cause a decrease in the RavA~P level (S6A Fig, S6B Fig and S6D Fig), which suggests that RavA transfers the phosphoryl group onto Asp496 of RavR and that RavR~P is highly unstable. Unlike isotope-labelling method, Phos-tag gel analysis successfully detected a RavR~P band in the RavA-RavR phosphotransfer reaction under an extremely high ATP concentration (2 mM, S6D Fig, lane 5), providing an evidence to demonstrate that RavA phosphorylates RavR.
For RavS, repeated efforts failed to detect any signal representing the autophosphorylated RavS-containing cytosolic region (RavSΔTrM, S6C Fig). However, a truncated RavS that lacks the N-terminal transmembrane helix and the two PAS domains (RavSΔN) exhibited strong autokinase activity in the presence of ATP (Fig 5A, lane 1 and S6C Fig). The addition of RavRΔEAL to the reaction mixture slightly decreased the level of RavS~P after 30 min of co-incubation (Fig 5A, lane 2, S6E Fig, lane 3). No signals representing RavR~P were observed by the isotope-labelling and Phos-tag gel analysis (Fig 5A, lane 3, S6E Fig and S6F Fig) and substitution of the conserved Asp496 of RavR (RavRΔEAL(D496A)) eliminated its activity to decrease the RavS~P level. Together, these biochemical analyses demonstrated that RavA and RavS are bona fide HKs. RavA can phosphorylate RavR at residue Asp496, and RavR~P is highly unstable.
(a) c-di-GMP enhances RavS-RavR phosphotransfer in vitro. A total of 5 μM RavSΔN was autophosphorylated for 15 min by the addition of 10 μCi [γ-32P]ATP. A total of 15 μM RavRΔEAL or RavRΔEAL(D496A) was added and incubated for 30 min at 25°C. A total of 100 μM c-di-GMP was added if necessary. The reactions were terminated with 5× SDS loading buffer before autoradiography. The experiment was repeated three times. (b) Time course analyses of the impact of c-di-GMP on the velocity of RavS-RavR phosphotransfer. The autophosphorylation and phosphotransfer reactions were set as mentioned in (a). Various concentrations of c-di-GMP were added to the reactions and isotopic signals (band intensities) of RavS~P were measured after autoradiography. (c–d) c-di-GMP triggered an increase in RavS-RavR phosphotransfer in a dose-dependent manner. (c) Various concentrations of c-di-GMP (0, 5, 10, 15, 30, 50, 75 and 100 μM) were added to the RavS-RavR phosphotransfer reactions. (d) The phosphorylated level of RavSΔN~P was quantified by ImageJ and the EC50 value was estimated by Origin 8.5 software. In (b) and (d), the intensity of each data point is the average from three experimental repeats. (e) c-di-GMP triggered increase in RavS-RavR phosphotransfer is highly specific. Other nucleotides, including GTP, GMP, cGMP and c-di-AMP, did not affect the velocity of the RavS-RavR phosphotransfer. (f) RavS specifically interacts with fl-c-di-GMP. The interaction between RavSΔTrM and various nucleotides, including fl-c-di-GMP, fl-cGMP and fl-c-di-AMP, were measured by microscale thermophoresis (MST). A total of 20 nM fluorescein-labelled nucleotides and increasing concentrations of proteins were incubated and measured by MST. The dissociation constant (Kd) was quantified to estimate the binding affinity. Each experiment was repeated three times.
c-di-GMP specifically and significantly enhances RavS-RavR phosphotransfer
Since ravS is downstream of ravR during the regulation of bacterial swimming and RavR is a functional phosphodiesterase that degrades c-di-GMP, we reasoned that c-di-GMP modulates the activity of RavS in controlling bacterial swimming. We analysed the impact of c-di-GMP on the enzymatic activities of RavS to test this hypothesis.
In the absence or presence of c-di-GMP (Fig 5A, lane 1 and lane 4), the autokinase activity of RavSΔN was unchanged, which suggests that c-di-GMP does not affect RavSΔN autophosphorylation. However, when RavRΔEAL was added to the RavS-RavR phosphotransfer reaction, the presence of c-di-GMP in the mixture remarkably increased RavS-RavR phosphotransfer because the RavSΔN~P level immediately decreased when compared with the level in the absence of c-di-GMP (Fig 5A, lane 5 vs. lane 2, and Fig 5B). The time (T50) that signal intensity of the RavS~P decreased to the half of the initiation stage (before adding RavRΔEAL) was estimated: without c-di-GMP, the T50 value of RavS~P is 38.2 min. When 15 μM c-di-GMP is presence, the T50 value of RavS~P remarkably decreased to 16.9 min. Since some HKs or RRs have phosphatase activity to dephosphorylate HKs, it is possible that c-di-GMP positively regulates RavS or RavR phosphatase activity to decrease the RavS~P level. However, addition of c-di-GMP alone did not affect RavSΔN~P levels (Fig 5A, lane 4 vs. lane 1, and Fig 5B) and the addition of an inactive RavRΔEAL(D496A) did not have any impact on RavS phosphorylation levels, regardless of the presence or absence of c-di-GMP (Fig 5A, lanes 3 and 6). These results indicate that c-di-GMP enhanced significantly RavS phosphotransferase activity towards RavR. This c-di-GMP-triggered kinetic preference effectively decreases the RavS~P level.
Along with the elevation of c-di-GMP concentrations, the RavS-RavR phosphotransfer, which was measured by the intensity of the RavS~P signal, gradually increased. This suggests that the impact of c-di-GMP on RavS autokinase activity is dose-dependent (Fig 5C). The estimated value of the median effect concentration (EC50) of c-di-GMP was approximately 15.58 μM (Fig 5D). Furthermore, the regulation of c-di-GMP on the RavS-RavR phosphotransfer to decrease the RavS~P level is highly specific because that other nucleotides and derivatives, including GTP, GMP, cGMP and c-di-AMP, did not have any impact on RavS phosphotransferase activity (Fig 5E).
Arg656 within the CA region of RavS is essential for c-di-GMP binding
Next, microscale thermophoresis (MST) was used to determine whether c-di-GMP binds directly to RavS. 2′-Fluo-AHC-c-di-GMP (fl-c-di-GMP) was used in the assay since the analogue contains a carboxyfluorescein that has excitation and emission wavelengths of 497 nm and 520 nm, respectively, which can be detected directly by a MST instrument . As shown in Fig 5F, fl-c-di-GMP directly bound a truncated, soluble RavS protein lacking the transmembrane region (RavSΔ). The dissociation constant was 6.06 ± 0.92 μM, which is in the range of physiological concentrations of c-di-GMP in bacterial cells . As controls, 2′-Fluo-AHC-cGMP (fl-cGMP) or 2′-Fluo-AHC-c-di-AMP (fl-c-di-AMP) bound RavSΔTrM with weaker affinity (fl-cGMP, 64.4 ± 9.43 μM) or completely failed to bind the protein (fl-c-di-AMP, Fig 5F). Furthermore, to determine the c-di-GMP binding region on RavS, we expressed and purified various RavS fragments (S7A Fig). MST assays revealed that fl-c-di-GMP bound RavS with the DHp-CA or CA region, whereas this second messenger did not bind the PAS-A, PAS-B and DHp regions of RavS (Fig 6A and 6B). Of note, a lower binding affinity of c-di-GMP with the CA domain than the DHp-CA domain was observed, which suggests that the DHp domain indirectly affects the interaction (Fig 6B). MST analysis also revealed that fl-c-di-GMP did not bind to RavRΔEAL, RavA and an unrelated HK VgrS since the Kd values were greater than 80 μM (S7B Fig), which did not have physiological significance. Therefore, these results revealed that c-di-GMP specifically binds to RavS and the CA domain of RavS is the possible interacting region of c-di-GMP.
(a, b) c-di-GMP binds to the DHp-CA domain of RavS. PAS-A, PAS-B and DHp-CA in (a), and DHp and CA domains of RavS in (b), were purified and the interaction with c-di-GMP was measured by MST. Each assay was repeated three times. Standard deviations are shown. (c) Molecular docking model of the interaction between c-di-GMP and DHp-CA of RavS. c-di-GMP is shown as a ball-and-stick model and DHp-CA is shown in ribbon representation. (d) Schematic view of the predicted docking site between c-di-GMP and DHp-CA. Potential hydrogen bonds are indicated as blue dashed lines. Autodock software was used to predict the interaction. (e) Effect of amino acid substitutions on RavS–c-di-GMP binding. Ten recombinant proteins of the DHp-CA region, each containing a substitution of a putative essential residue involved in c-di-GMP binding, were used in the MST assay to quantify the Kd value of RavS–c-di-GMP binding. fl-c-di-GMP was used in the MST assay. Each experiment was repeated three times. (f) Substitution of Arg656 of RavS resulted in the loss of RavS-RavR phosphotransfer upon stimulation by c-di-GMP. A total of 5 μM RavSΔN or RavSΔN(R656A) was phosphorylated by 10 μCi [γ-32P]ATP for 15 min in the absence or presence of 15 or 100 μM c-di-GMP, and then 15 μM RavRΔEAL was added and incubated for 30 min at 25°C. The reactions were terminated with 5× SDS loading buffer and the products were separated by 12% SDS-PAGE, exposed to a phosphor screen and analysed by Typhoon FLA7000. The experiment was repeated three times.
Similar to most HKs, the three-dimensional (3D) structure of RavS has not been elucidated. As an alternative, molecular docking was used to predict the structural interaction of the RavS–c-di-GMP complex. We predicted the DHp-CA (residues E464–R697) structure of RavS by homology modelling with the crystal structures of other HKs, such as CpxA-HDC (PDB ID: 4BIU), DivL (4EW8) and VraS (4GT8), as templates. As shown in Fig 6C, the putative structure of DHp-CA is composed of seven α-helices, four β-strands and random crimps. The active centre includes the helices of α3, α4, α5 and α6 and strands β3 and β4, and is highly similar to other DHp-CA domains of HKs. The 3D structure of c-di-GMP was extracted from the crystal structure of the c-di-GMP-VCA0042 complex (PDB ID: 2RDE) . Autodock 4.0 software was used for molecular docking. The results showed that helices α4 and α7 and strands β3 and β4 of the RavS DHp-CA domain formed a c-di-GMP binding pocket and 10 residues in the vicinity of the pocket potentially interact with c-di-GMP (Fig 6C and 6D). Among these residues, Ser636, Asp638, Asp640, Ile653, Glu657 and Leu666 putatively interact with c-di-GMP via hydrophobic interactions and van der Waals forces, whereas Asp637, Gly639, Leu652 and Arg656 form hydrogen bonds with c-di-GMP (Fig 6D). In contrast to the other residues, the amino hydrogens of Arg656 and the phosphate group oxygens of c-di-GMP formed two hydrogen bonds with bond lengths of 2.3 Å and 2.5 Å, respectively (Fig 6D). These results suggest that c-di-GMP potentially interacts with the CA region of RavS and that Arg656 is a key residue in the interaction.
To experimentally verify the above prediction, we expressed and purified 10 recombinant DHp-CA proteins in which each of the predicted c-di-GMP-interacting amino acids were separately substituted to Ala. MST assays revealed that the recombinant proteins DHpCAD637A, DHp-CAG639A, DHp-CAD640A, DHp-CAI653A, DHp-CAE657A and DHp-CAL666A exhibited no significant change in c-di-GMP binding affinity. In contrast, DHp-CAS636A, DHp-CAD638A and DHp-CAL652A exhibited 1–2-fold increases in Kd values when compared with that of the positive control (DHp-CA protein), which suggests that these substitutions disrupt the protein-nucleotide interaction. Notably, the Kd value of the c-di-GMP–DHp-CAR656A interaction was 62.4 ± 3.19 μM, which showed a 10-fold decrease in binding affinity (Fig 6E). Consistent with this result, an in vitro phosphotransfer assay revealed that c-di-GMP failed to stimulate the phosphotransferase activity of RavSΔN(R656A)~P towards RavRΔEAL and the RavSΔN(R656A)~P level did not change noticeably or decreased slightly in the presence of c-di-GMP (15 or 100 μM, Fig 6F). Thermal shift assay revealed that the DHp-CAR656A is as stable as DHp-CA protein (S8A Fig), and RavSΔN and RavSΔN(R656A) have similar autokinase activity (S8B Fig), suggesting that the Arg656 substitution did not remarkably affect the structure of the recombinant protein. Collectively, these results demonstrate that Arg656 of RavS is a key residue in c-di-GMP binding. Substitution of Arg656 leads to dissociation between c-di-GMP and RavS such that the RavS-RavR phosphotransfer is not accelerated. Under these circumstances, the majority of RavS remains phosphorylated.
RavSR656A substitution causes phenotypic changes that mimic constitutively activated RavS
Based on the above results, we constructed a ravSR656A point mutant to determine whether the dissociation of c-di-GMP from RavS affects bacterial phenotypes. Western blotting revealed that RavS is stable in this mutant (S8C Fig). As shown in Fig 7A and 7B, the virulence of the ravSR656A mutant was attenuated substantially and the production of EPS by this mutant had also decreased significantly (Fig 7C). The swimming zone diameter of the ravSR656A mutant was 2.38 ± 0.10 cm, which was much larger than that of the WT strain (1.16 ± 0.08 cm) (Fig 7D and 7E). Therefore, we measured the parameters of bacterial flagella and found that the ravSR656A mutant had longer flagella (4.79 ± 1.31 μm, Fig 7F and 7H). The ravSR656A mutant flagellar cell ratio was two-times the level of the WT strain (Fig 7G) and the fliC mRNA level had increased by 292% when compared with that of the WT strain (Fig 7I). Therefore, the pattern of phenotypic changes of the ravSR656A point mutant is similar to that of the ravS overexpression strain (ΔravS-ravS; S9A–S6F Figs) but is quite different from that of the ravS deletion or ravSH500A mutant whose virulence and EPS production were unaffected, whereas the tested parameters of swimming motility were reduced significantly (Fig 3).
(a, b) Bacterial virulence. Bacterial strains were inoculated onto plant leaves of Brassica oleracea cv. Zhonggan 11. The lesion length was recorded 10 d after inoculation (n = 30). (c) Production of extracellular polysaccharides (EPS). EPS quantification was calculated as the dry weight of EPS vs. the dry weight of bacterial cells (n = 3). (d, e) Bacterial swimming motility. (d) Bacterial strains were inoculated in NYG plates containing 0.15% agar and grown at 28°C for 28 h. (e) Average diameters of the migration zones were measured (n = 10). (f) Morphology of bacterial flagella. Bacterial flagella were observed by TEM after negative staining. A representative image of each strain is shown. Upper panel: bacterial population profile; lower panel: single bacterium. (g) Ratio of bacterial cells with flagella. For each strain, cells with flagella were counted (n = 100). (h) The average flagellar length of bacterial strains (n = 30). (i) fliC mRNA levels in bacterial strains. The amount of fliC mRNA was measured by qRT-PCR. Amplification of cDNA from tmRNA was used as an internal control. The experiment was repeated three times and the result of a representative is shown. In the figure, standard deviations are shown; asterisk: significant difference, as tested by Student’s t-test (P ≤ 0.05). Three biological replicates were performed.
Thus, these results suggest that the ravSR656A substitution, which eliminated the binding capability of c-di-GMP, mimics the constitutive phosphorylated state of RavS. Subsequently, the conserved His500 residue was mutated on the genetic background of ravSR656A. Compared with the ravSR656A mutant, the double mutant ravSR656A-H500A exhibited restored virulence and EPS production levels (Fig 7A–7C). The swimming motility (Fig 7D and 7E), flagellar cell ratio (Fig 7F and 7G), flagellar length (Fig 7H) and fliC mRNA levels (Fig 7I) of the double mutant were all significantly reduced or undetectable. Therefore, point mutation of His500 completely suppressed the mutational effects caused by the Arg656 point mutation. Together with the biochemical results demonstrating that c-di-GMP did not bind ravSR656A and that the phosphorylation level of RavSR656A is insensitive to c-di-GMP inhibition, these findings suggest that c-di-GMP associates with the Arg656 residue to negatively regulate the RavS phosphotransferase activity towards RavR.
RavR regulates RavS~P levels through a c-di-GMP-enhanced phosphate sink
The aforementioned genetic and biochemical results prompted the following hypothesis: a high level of RavS~P positively regulates bacterial swimming but is detrimental to virulence; however, dephosphorylation of RavS reduces the expression of fliC and is negative in modulating bacterial swimming. Since c-di-GMP binds to RavS to inhibit the phosphotransferase activity of RavS towards RavR, RavR is likely to be a special phosphate sink that controls the RavS~P level through opposite mechanisms: 1) the REC domain of RavR receives the phosphoryl group from RavS~P, which decreases the RavS~P level and then negatively regulates bacterial swimming. Additionally, c-di-GMP inhibits bacterial swimming by further enhancing the RavS-RavR phosphotransfer; and 2) the EAL domain of RavR degrades c-di-GMP and then inhibits the c-di-GMP-triggered RavS-RavR phosphotransfer. This process prefers to maintain the RavS~P level and positively regulates bacterial swimming. This hypothesis is true when constitutive dissociation by genetic manipulation of the binding event between c-di-GMP and RavS results in a high RavS~P level. As a consequence, this process will positively modulate bacterial swimming independent of the c-di-GMP concentration in cells.
To test this hypothesis, we point mutated Arg656 of ravS to Ala to construct a double mutant on the ravRΔEAL genetic background (ravRΔEALravSR656A). The RavR phosphodiesterase activity of this mutant was genetically inactivated and recombinant RavS did not bind c-di-GMP because Arg656 is essential for the protein-[c-di-GMP] interaction. As shown in Fig 7, the point mutation of ravSR656A effectively suppressed the phenotypic effects (i.e., virulence and EPS production) caused by the EAL domain deletion (Fig 7A–7C) and bacterial swimming was restored completely (1.48 ± 0.08 cm; Fig 7D and 7E). The number of flagella and flagellar cell ratio were increased significantly when compared with the level of the WT strain (Fig 7F–7H). The fliC mRNA level of the ravRΔEALravSR656A mutant was also significantly increased from 9.4% (ravRΔEAL) to 199% of the level of the WT strain (Fig 7I). Similarly, overexpression of ravS on the ravRΔEAL ΔravS background (ravRΔEALΔravS-OE-ravS; S9A Fig), which mimics constitutive phosphorylation of RavS, also effectively suppressed the mutational effects of the EAL domain deletion on bacterial swimming (S6 Fig).
Furthermore, the suppression of the ravSR656A mutation and ravRΔEAL deletion completely depends on the conserved His500 site of RavS. The triple mutant of ravRΔEALravSR656A(H500A) exhibited performance similar to that of ravRΔEAL in all of the tested parameters associated with swimming or flagella development (Fig 7A–7I). Collectively, these genetic analyses support the hypothesis regarding the regulation of RavR in controlling the RavS~P level. Asp469 within the REC domain of RavR receives the phosphoryl group from RavS to reduce the RavS~P level, whereas the EAL domain of RavR degrades c-di-GMP, which binds to RavS and promotes the specificity between RavS-RavR by broadening the phosphotransfer flux. Dissociation of RavS–c-di-GMP leads to enhanced bacterial swimming, which depends on the high phosphorylation level of RavS.
Kinetic preferences between HKs and RRs define the specificity of TCS regulation [7, 44], which is quantified by the velocity of a HK to phosphorylate a RR . In the present study, genetic, biophysical and biochemical data revealed that c-di-GMP substantially enhanced the specificity between RavS and RavR of X. campestris pv. campestris. RavS physically interacts with c-di-GMP via its CA region. This interaction remarkably accelerated phosphoryl transfer from RavS~P towards RavR, resulting in efficient dephosphorylation of RavS~P. Intriguingly, the EAL domain-containing RavR acts as a phosphate sink of RavS~P. Stimulated by c-di-GMP, the REC domain of RavR receives a phosphoryl group from RavS to decrease the RavS~P level, which negatively modulates bacterial swimming. However, the EAL domain of RavR degrades c-di-GMP. Degradation of c-di-GMP revokes the accelerating effect of c-di-GMP on RavS-RavR phosphotransfer, leading to a high level of RavS~P, which positively regulates bacterial swimming (Fig 8). Therefore, these results suggest that RavS is a pivotal node for integrating the regulatory pathways of c-di-GMP and TCS, and RavR is a bifunctional regulator that finely controls the phosphorylation state of RavS (Fig 8). The crosstalk between c-di-GMP and RavS–RavR phosphoryl transfer regulates a bacterial lifestyle transition from virulence to freely swimming.
Left panel: During infection, RavA–RavR phosphotransfer is necessary to control bacterial virulence, whereas RavS is maintained at a low phosphorylation level. c-di-GMP binds to RavS to enhance the phosphotransfer to the REC domain of RavR, which acts as a phosphate sink. Right panel: During bacterial swimming, the level of phosphorylated RavS is high. The EAL domain of RavR is activated and degrades the c-di-GMP binding to RavS. This process decreases RavS-RavR phosphotransfer and promotes an increase in the RavS~P level to regulate flagella development. TrM: transmembrane helix. DHp: dimerization and histidine phosphotransfer domain. CA: catalytic and ATP binding domain. REC: receiver domain. P in the red circle represents the phosphoryl group. Grey dashed arrows or terms indicate that the biochemical processes were inactivated.
c-di-GMP plays a pleiotropic role in controlling the physiological processes of bacterial cells. This cyclic dinucleotide is a versatile, flexible molecule and the regulatory function of c-di-GMP is usually exerted by binding to a diverse array of effectors to elicit allosteric changes [14, 18, 45]. However, the intracellular concentration of c-di-GMP is complex and changed dynamically . The local, subcellular c-di-GMP concentrations are critical and have profound effects on physiological processes . Currently, the reported Kd values between c-di-GMP and proteins range from 0.1 μM (PizD) to 14.5 μM (STING) . Our MST assay revealed that c-di-GMP physically binds to RavS in vitro with a Kd of 6.06 μM (Fig 5F), which is similar to the previously identified effector CLP of Xanthomonas campestris pv. campestris , suggesting that RavS is a bona fide c-di-GMP effector. The binding of c-di-GMP to RavS substantially increased its phosphotransferase activity towards RavR but did not affect RavS autokinase and phosphatase activities (Fig 5A and 5B). In TCS regulation, phosphotransfer from HK to RR is generally controlled by their specificity, which is defined by key ‘specificity residues’ in these proteins [6, 44]. However, our results showed that c-di-GMP did not bind the RR RavR (S7B Fig), thus excluding the possibility that c-di-GMP increases RavR phosphatase activity towards RavS~P. Since the DHp and CA domains of HK are associated, we reasoned that the binding of c-di-GMP to the CA domain confers a conformational switch in the DHp domain, which leads to more efficient phosphoryl transfer from the DHp domain to the REC domain of RavR. Details on c-di-GMP-mediated enhancement of phosphoryl transfer require further structural analysis.
According to previous studies, c-di-GMP binds to diverse regions of proteins, such as the degenerate GGDEF and EAL domains, PilZ domain and the interdomain linker . In the absence of the RavS structure, we employed a molecular docking method together with mutational analysis to define residues essential to interaction with c-di-GMP (Fig 6). The analysis suggests that Arg656 within the helix α7 region of the CA domain potentially forms two hydrogen bonds with c-di-GMP (Fig 6C and 6D). Substitution of this residue eliminated RavS–c-di-GMP binding in vitro (Fig 6E). Additionally, point mutant ravSR656A exhibited enhanced bacterial swimming, elongation of flagella, a higher ratio of flagellar cells and increased fliC transcription levels (Fig 7). Similar to the overexpression of ravS (S9 Fig), the ravSR656A mutation suppressed completely the mutational effects of the ravRΔEAL deletion that decreased swimming motility (Fig 7). Therefore, Arg656 within the CA region is an essential residue for binding c-di-GMP. This finding is in accordance with the preference of Arg or Asp/Glu residues to form hydrogen bonds with the phosphate group of c-di-GMP . Compared with CckA of C. crescentus, which also binds to c-di-GMP, both HKs contain two PAS domains and a DHp-CA core; however, RavS lacks the C-terminal REC domain and is not a hybrid-type HK. When interacting with c-di-GMP, the autokinase activity of CckA was inhibited but its phosphatase activity was increased [27–29]. However, c-di-GMP binding did not affect the RavS autophosphorylation. It increases the phosphoryl flux from RavS towards RavR. The structural basis of this difference is unclear.
Intriguingly, RavR plays a special role in regulation. Previous studies on c-di-GMP turnover found a general trend in which an elevated cellular concentration of c-di-GMP leads to a reduction in motility behaviours [14, 18, 48]. Therefore, inactivation of EAL domain-containing proteins usually increases c-di-GMP concentrations and inhibits bacterial swimming. In this study, deletion of the ravR gene increased the cellular concentration of c-di-GMP (Fig 4B) but this increase promoted bacterial swimming substantially rather than reducing this activity (Fig 1G). Further investigation revealed that deletion of the EAL domain of RavR caused completely opposite phenotypic changes as the swimming zone was significantly reduced (Fig 4F). This phenotype led us to examine the function of the EAL and REC domains of RavR. We found that RavR acts as a phosphate sink of RavS. Since the point mutation of ravRD496A restored the reduced swimming motility caused by EAL deletion (Fig 4F–4K), the Asp496-dependent phosphoryl-receiving activity of RavR functions to regulate RavS~P levels by c-di-GMP-triggered RavS-RavR phosphotransfer, rather by directly modulating the PDE activity of the EAL domain, as revealed by S5D–S5F Fig. Based on these findings, the EAL domain degrades cellular c-di-GMP to release the negative regulation of c-di-GMP at the RavS~P level by promoting RavS-RavR phosphotransfer. Therefore, RavR is a bidirectional regulator that controls the RavS~P level through degrading c-di-GMP and accepting phosphoryl group from RavS.
As genetic and biochemical analyses revealed, both HKs RavA and RavS phosphorylate RavR, and all three proteins control the virulence and swimming of X. campestris pv. campestris (Figs 1 and 5). Among these proteins, RavA and RavR compose a typical TCS that regulates bacterial virulence. As a previous study revealed, ravR is downstream of ravA in regulation [37, 38]. In X. oryzae pv. oryzae, a close relative of X. campestris pv. campestris, ravA-ravR orthologues (pdeK-pdeR) have the same relationship in modulating bacterial blight disease against rice (Orzya sativa) . As mentioned above, ravR is upstream of ravS in regulating bacterial swimming because RavR acts as a phosphate sink to dephosphorylate RavS (Fig 3). Our results further suggest that the regulation of bacterial virulence by RavA–RavR also depends on RavS because the ravS mutation suppressed the deficiencies of ravA and ravR mutants in virulence as well as in swimming (Figs 3 and 7). Since RavS and RavA are HKs that detect environmental and intracellular stimuli, it is important to know what signals were monitored by the two HKs. Because RavA lacks a recognizable signal input domain, it is challenging to predict the stimulus detected by RavA. However, RavS contains two intracellular PAS domains. PAS domain was found to sense low oxygen, redox, light or binds to small chemicals [50, 51]. A previous study also demonstrated that hypoxia sensing by RavS is involved in regulating virulence of X. campestris . In our study, we found that the truncated RavS without the N-terminal transmembrane and PAS domains had a higher level of autokinase activity, indicating that the PAS domains autoinhibit the phosphorylation of RavS. If this hypothesis is true, the signals detected by PAS domains, such as low oxygen and still to-be-identified stimuli, will regulate RavS phosphorylation and play important roles in controlling virulence and motility of X. campestris.
In vitro phosphotransfer assays revealed that upon phosphorylation by RavA or RavS, there is no signal representing the observed RavR~P, which suggests that RavR~P is highly unstable (Fig 5A and S6 Fig). This biochemical feature of RavR may have an essential role in regulation because regardless of whether the phosphoryl groups are obtained from RavS or RavA or even if the transfer speed is enhanced by c-di-GMP, RavR can be promptly uncharged and avoid rapid saturation in phosphorylation. The unstable nature of RavR~P make the protein to be uncharged by dephosphorylation very quickly [52, 53]. Furthermore, considering that dissociation of the interaction between RavS and c-di-GMP either by substitution of Arg656 or by overexpression of ravS led to virulence attenuation, we speculate that RavR~P dephosphorylation has an important role in regulating the lifestyle transition between virulence and swimming motility. Future investigations are needed to dissect the molecular mechanism controlling the half-life of RavR~P in the context of RavA-RavR-RavS regulation.
Materials and methods
Bacterial strains, plasmids and culture conditions
All bacterial strains and recombinant vectors used in this work are listed in S1 Table. The WT strain of X. campestris pv. campestris ATCC 33913 and recombinant strains were grown at 28°C in rich NYG medium (5 g L−1 tryptone, 3 g L−1 yeast extract and 20 g L−1 glycerol, pH 7.0). We used 210 medium (5 g L−1 sucrose, 8 g L–1 casein enzymatic hydrolysate, 4 g L−1 yeast extract, 3 g L−1 K2HPO4 and 0.3 g L−1 MgSO4·7H2O, pH 7.0) to prepare for electro-component cell production and the TGM medium (10 g L−1 tryptone, 5 g L−1 yeast extract, 20 g L−1 glycerol, 10 g L−1 glucose, 0.7 g L–1 K2HPO4, and 0.25 g L−1 MgSO4.7H2O) for the EPS production assay. Escherichia coli (E. coli) DH5α cells were used as a host for the construction of all recombinant vectors. The E. coli BL21(DE3) strain was used as a host for expressing recombinant proteins with the pET30a, pET22b or pET28b vectors (Novagen, USA), and the E. coli TB1 strain was used as a host for expressing recombinant proteins with the pMAL-p2X vector (Novagen). Appropriate antibiotics were added to the media when needed at the following concentrations: kanamycin (50 μg ml–1), spectinomycin (150 μg ml–1) and ampicillin (100 μg ml–1). Electro-competent cells were prepared by washing bacterial cells thoroughly three times with ice-cold glycerol (10%). The transformation conditions of bacterial cells were set at 1.8 kV cm–1, 25 μF and 200 Ω and conducted in a Bio-Rad Pulser XCell (Bio-Rad, USA).
Construction of mutant and genetic complementation
General molecular biology experiments, including PCR, DNA ligation, enzyme restriction and western blotting, followed the protocols from Molecular Cloning unless otherwise mentioned. All in-frame deletion (markerless) mutants were constructed using the suicide vector pK18mobsacB by a homologous, double crossover method. Briefly, the 5′ and 3′ genomic sequences of a targeted region were amplified using the primers listed in S2 Table, and correct PCR products were ligated into pK18mobsacB. Point mutants were constructed from the corresponding deletion mutants using pK18mobsacB with the point mutated genes. The recombinant pK18mobsacB vector was electroporated into X. campestris pv. campestris competent cells to generate single-crossover mutants by selection on NYG plates containing kanamycin. Next, single-crossover mutants were cultured in NYG medium for 1–2 h and then grown on NYG plates containing 10% sucrose to select second-round homologous crossovers. Candidate bacterial mutants were verified by PCR and sequencing. To genetically complement mutants, a full-length gene with a native promoter was amplified using primers listed in S2 Table and ligated into the broad-host vector pHM2. Then, the pHM2 recombinant vector was used to complement the mutated genes. The recombinant medium-copy, broad-host-range vector pBBR1MCS2 that carries full-length sequences of the genes of interest (under the control of the Plac promoter) was used to construct overexpression strains.
Semi-quantitative western blotting
Briefly, bacterial culture grown to OD600 nm = 0.5 and 0.1 ml or 1.0 ml cell cultures were transferred to into two new tubes, A and B, respectively. The tube B were centrifuged for 10 min at 4°C at 5,000 g. Cell pellets in tube B were resuspended in 80 μl ddH2O and 20 μl 5×sample loading buffer and the mixtures were boiled for 15 min before being subjected to12% (w/v) SDS-PAGE gels for electrophoresis analysis. Proteins were then electrotransferred onto a Fluoro Trans polyvinylidene fluoride membrane (PALL, USA) following the manufacturer's protocol and were detected with immunoblotting by the antiserum against RavS, RavA or RavR and HRP-conjugate goat anti-rabbit IgG secondary antibody (Abmart, China) at a dilution of 1:5,000. The protein bands were visualized by Enhanced ECL Chemiluminescent Substrate Kit (Yeasen, China). The densities of protein bands were determined by Image J. The amounts of individual protein bands were calculated from the standard curves derived from a set of purified and quantified RavS, RavA or RavR protein standards run on the same blot. Protein levels were normalised to bacterial cells, which were counted in a serially diluted bacterial culture from tube A that was grown on NYG plates for 48 hours. To estimate the concentration of a protein in a cell, morphology of 30 bacterial cells were selected and their volumes were calculated as cylinders. Each experiment was performed with three biological replicates.
Plant inoculation and virulence assays were conducted using six-week-old cabbage cultivar Brassica oleracea cv. Zhonggan 11 as host plants. The WT strain of X. campestris pv. campestris ATCC 33913 and sterile 10 mM MgCl2 were used as positive and negative controls, respectively. All bacterial strains were cultured overnight in NYG medium containing appropriate antibiotics. Cells were collected and washed with 10 mM MgCl2 and the concentrations were adjusted to OD600 = 0.1 before inoculation using sterile scissors. After inoculation, the plants were kept in a greenhouse at 25–30°C and relative humidity >80%. The lesion length was measured 10–12 d after inoculation. For each strain, at least 30 cutting sites were made to evaluate the virulence level.
EPS production assays
An assay of EPS production was conducted according to a previous study with small modifications [37, 54]. Bacterial strains were cultured at 28°C in NYG medium until the OD600 = 0.8. Then, 200 μL subculture was inoculated into 20 mL TGM medium and cultured at 28°C for 72 h before measurement. To determine the production of EPS, the supernatants of 12 mL bacterial cultures were separated by centrifugation at 25,000 g for 30 min. A total of 24 mL ethanol and 1.2 mL saturated KCl were added into the supernatants and the mixtures were kept at 4°C for 4 h. The precipitated EPS was pelleted by centrifugation at 25,000 g for 30 min and washed twice with 12 mL 95% ethanol. The bacterial cells and EPS were dried at 60°C overnight before determination of their dry weights. EPS production was quantified by the ratio of the weight of EPS vs. the dry weight of bacterial cells.
Swimming motility assays
NYG semi-soft agar (0.15% agar) motility plates were used to determine the swimming capability of bacterial strains. Semi-soft plates were prepared and allowed to cool and dry at room temperature for 3 h prior to inoculation. Strains were cultured at 28°C overnight and adjusted to OD600 = 0.8. Then, 2.5 μL of the mixture was transferred to the motility plates and incubated at 28°C for 28 h. The plates were photographed and the diameter of the migration zone of bacteria was measured. Assays were performed with at least three biological replicates, each containing 10 repeats. Statistical analysis was performed using the two-tailed Student’s t-test.
Negative staining and transmission electron microscopy (TEM)
Bacterial strains were cultured at 28°C for 36 h. Negative staining and TEM observations were performed. Briefly, bacterial cells were acquired from NYG plates and gently suspended in 40 μL ddH2O for 15 min. The bacterial turbid liquid was then spotted onto 400 mesh carbon-coated copper grids, which were glow discharged for 15 s immediately prior to use. Samples on the grids were negatively stained twice with 0.15% uranyl acetate before blotting with filter paper. Pictures were taken with a JEM-1400 electron microscope (JEOL, Japan) at an operating voltage of 80 kV.
Flagellated cell ratio statistics and flagellar length measurements
The number of flagellated cells (Nf) and non-flagellar cells (Nnf) in the TEM images were counted and the flagellated cell ratio = Nf/(Nf + Nnf) determined. Assays were performed with three biological replicates and the number of counted cells in each assay was larger than 100. Statistical analysis was performed using the two-tailed Student’s t-test.
To measure flagellar length, the tagged image file (TIF) format pictures of cells were transformed to the AutoCAD Drawing Database (DWG) format and then opened by auto Desk auto CAD 2014 software. Flagella were traced by the PLINE model and the relative lengths were calculated by the PROPERTIES model. The scale segment of each picture was measured in the same way to calculate the flagellar length. Assays were repeated with three biological replicates and the number of measured flagella in each assay was larger than 30.
qRT-PCR was used to measure the level of mRNA. Total RNA was extracted by TRIzol (Invitrogen, USA). The DNA contamination in total RNA samples was eliminated by RNAase-free DNase I (Ambion, USA). The first strand of cDNA was generated using random primers (Promega, USA) and Superscript III reverse transcriptase (Invitrogen). qRT-PCR was conducted using Maxima SYBR Green (Fermentas, USA) in a DNA Engine Option 2 System (Bio-Rad), according to the manufacturer’s instructions. Amplification of tmRNA was used as an internal control. Generally, a qRT-PCR experiment was repeated independently three times with three technical repeats of each sample. A representative of all the biological repeats was selected and reported.
Protein expression, purification and polyclonal antibodies
C-terminal, His6-tagged recombinant proteins were produced by corresponding recombinant pET30a, pET22b or pET28b (Novagen) vectors that were transformed into the E. coli BL21(DE3) strain. His6-tagged proteins were extracted and purified using affinity chromatography with Ni-NTA agarose beads (Novagen), according to the manufacturer′s instructions. N-terminal MBP-tagged recombinant proteins were produced by the corresponding recombinant pMAL-P2X (Novagen) vector that was transformed into the E. coli TB1 strain. If necessary, the TEV protease cleavage sequence was appended at the N-terminus of the target protein. The MBP fusion protein was purified and the elute buffer was exchanged to the reaction buffer (50 mM Tris-HCl, pH 8.0, 50 mM NaCl, 0.5 mM EDTA and 1 mM DTT), then incubated with TEV protease at a ratio of 1:100 for 8 h at 4°C. Cleaved MBP or uncleaved fusion protein was removed by MBP resin and the TEV protease was removed by Ni-NTA agarose beads. Purified target protein was obtained by size exclusion chromatography with a Superdex 75 10/300 GL column (GE Healthcare, Piscataway, NJ, USA). Purified proteins were concentrated using Centricon YM-10 columns (Millipore) and the elute buffer was changed to the storage buffer (50 mM Tris-HCl, pH 8.0, 0.5 mM EDTA, 50 mM NaCl and 5% glycerol) for further use or storage at −80°C. Protein preparations were examined for purity by SDS-PAGE and quantified by a Bradford assay (Bio-Rad). Polyclonal antiserums of RavR, RavS and RavA were prepared by immunising rabbits with approximately 3 mg purified, soluble proteins. The polyclonal antibodies of RpfC and HPPK were reported by our previous studies [32, 55].
Gel filtration chromatography
The purified EAL protein was concentrated by VivaSpin Turbo, 5K MWCO (Sartorius, German). A total of 15 μM protein and 300 μM c-di-GMP are incubated in phosphodiesterase reaction buffer (50 mM Tris-HCl pH 7.5, 250 mM NaCl, 25 mM KCl, 10 mM MgCl2 and 2 mM DTT) at 4°C for 30 min and subsequently subjected to gel filtration with Fast Protein Liquid Chromatography AKTA Purifier 10 with Frac-900 (GE Healthcare, USA). The ATKA system was pre-equilibrated with phosphodiesterase reaction buffer at a flow rate of 0.5 ml/min and then applied to a Superdex 75 10/300 GL column to separate dimer and monomer. The elution profiles were collected at A280 and confirmed by SDS-PAGE and Coomassie brilliant blue staining.
In vitro autophosphorylation and the phosphoryl transfer assay
An in vitro autophosphorylation assay was conducted as described in our previous study [32, 55]. Purified protein was incubated with 10 μM ATP containing 10 μCi [γ-32P]ATP (PerkinElmer, USA) in the reaction buffer (50 mM Tris-HCl, pH 7.8, 25 mM NaCl, 25 mM KCl, 5 mM MgCl2, 2 mM DTT) for the indicated time at 28°C. If necessary, c-di-GMP was added to the mixture at the same time as ATP. For the phosphoryl transfer assay, purified RR protein or its derivative was added into the reaction mixture containing the phosphorylated HK. The autophosphorylation or phosphoryl transfer reaction was terminated by adding 5× SDS-PAGE loading buffer. Phosphorylated proteins were separated by 12% SDS-PAGE. After electrophoresis, gels were exposed to a phosphor screen (GE Healthcare) and the autoradiographic signals were detected by a Typhoon FLA7000 (GE Healthcare).
Phos-tag acrylamide gel analysis
Phos-tag acrylamide gels were prepared according to the instructions described by the manufacturer with minor modifications. Phos-tag acrylamide running gels contained 8% or 12% (w/v) 29:1 acrylamide:N, N”-methylene-bis-acrylamide, 375 mM Tris pH 8.8, 0.1% (w/v) SDS. All the gels were copolymerized with 50 μM Phos-tag acrylamide and 100 μM MnCl2. All stacking gels contained 5% (w/v) 29:1 acrylamide:N, N”-methylene-bis-acrylamide, 125 mM Tris pH 6.8, 0.1% (w/v) SDS. All Phostag acrylamide containing gels were run at 4°C for 3.5 hours under constant voltage (150 V). Coomassie brilliant blue staining was used to detect the phosphorylated proteins.
Microscale thermophoresis assay
The interaction between c-di-GMP nucleotides and various proteins was measured by using MST with a fluorescein-labelled c-di-GMP (2′-Fluo-AHC-c-di-GMP, abbreviated as fl-c-di-GMP; 2′-Fluo-AHC-c-di-AMP, fl-c-di-AMP; 2′-Fluo-AHC-cGMP, fl-cGMP; Biolog, Germany). These chemicals contain carboxyfluorescein that has excitation and emission wavelengths of 497 nm and 520 nm, respectively, which can be detected directly by a MST instrument. The experiments were performed on a Monolith NT.115 device using standard treated capillaries (NanoTemper Technologies, Germany). The concentration of the particular protein varied from 0.036 to 150 μM with a 2-fold gradient and the concentration of fl-c-di-GMP was constant at 20 nM. Fluorescence intensity due to thermophoresis was recorded using the blue channel optics of the instrument (λex = 470 ± 15 nm, λem = 520 ± 10 nm) during a 30 s period of infrared laser heating at 80% of the maximum laser power, followed by a 5 s cooling period. Measurements were performed in buffer containing 20 mM HEPES, pH 7.5, 150 mM NaCl, 2 mM MgCl2, 2 mM DTT and 0.05% Tween 20. The KD Fit of NanoTemper Analysis software (ver. 1.5.41) was used for fitting the curve and calculation of the dissociation constant (Kd). Assays were repeated with at least three biological replicates in triplicate.
Thermal shift assay
Thermal shift assays were performed as previously described with minor modification. Briefly, purified protein was added to the reaction to a final concentration of 5 μM in the MST buffer [20 mM HEPES, pH 7.5, 150 mM NaCl, 2 mM MgCl2, 2 mM DTT, 0.05% Tween 20 and 1:500 dilution of SYPRO Orange Dye (Invitrogen, USA)]. A melt curve protocol was run on a Bio-Rad qPCR instrument (Bio-Rad, USA). The fluorescence was measured using the ROX reporter with a temperature gradient of 20–95°C in 1.0°C increments at 30 second intervals. Melt curve data were trimmed to three data points after maximum and the data were plotted with Boltzmann model to obtain the temperature midpoint of unfolding (Tmid) of the protein using Prism 5.0 software (GraphPad). Three biological replicates were assayed in triplicate and statistical significance was determined with two-tailed Student’s t-test.
Synthesis and purification of [32P]c-di-GMP
[32P]-labelled c-di-GMP was chemically synthesised using a labelled [32P]GTP (3000 Ci/mmol, PerkinElmer, USA) and the purified His6-tagged enzyme tDGC; a protein construct with a key residue mutation (R158A) of diguanylate cyclase from Thermotoga maritime . Five micromolar tDGC and 20 μCi [32P]GTP (mixed with 50 μM cold GTP) were added to a mixture of 20 μL reaction buffer (300 mM NaCl, 50 mM Tris-HCl, pH 7.5, 20 mM MgCl2, and 2 mM DTT). After 3 h at 45°C, the reaction was terminated by heating at 98°C for 10 min. The precipitated protein was removed by centrifugation at 20,000 g for 5 min. Radioactive [32P]c-di-GMP was tested by separation on a polyethyleneimine-cellulose plate (1:1.5 (v/v) saturated (NH4)2SO4 and 1.5 M KH2PO4, pH 3.6). The mixture contained more than 95% [32P]c-di-GMP without further purification.
In vivo c-di-GMP quantification
c-di-GMP extraction was performed as described previously with modifications . Briefly, 8 mL bacterial culture grown to OD600 = 0.8 was centrifuged at 5000 g and 4°C for 10 min. Cell pellets were resuspended in 2× 800 μL NYG medium and 0.2 and 1.0 mL of the cell resuspension was transferred to two tubes, A and B, respectively. The tubes were centrifuged at 5,000 g and 4°C for 10 min. The cell pellet in tube B was resuspended in 300 μL extraction solution (40% acetonitrile, 40% methanol and 20% water), incubated on ice for 15 min and lysed by a non-contact ultrasonication system (Bioruptor UCD-200, Diagenode, Belgium) for 10 min with an alternating 30 s power on and 30 s power off procedure. Samples were then centrifuged at 20,000 g and 4°C for 10 min and the supernatant was transferred into a 2.0 mL tube. Extraction was repeated twice with 200 μL extraction solution but heating at 95°C was omitted. The combined supernatant fluids of three extractions were completely evaporated. c-di-GMP powders were resuspended in 100 μL HPLC-grade ddH2O and analysed by liquid chromatography-tandem mass spectrometry (LC-MS/MS) on an AB SCIEX QTRAP 4500 system (AB SCIEX, USA). A Synergi Hydro-RP 80A LC column (4 μM, 150 × 2 mm, Phenomenex, Torrance, CA, USA) was used for reversed-phase liquid chromatography. Solvent A was 0.1% acetic acid in 10 mM ammonium acetate and solvent B was 0.1% formic acid in methanol. The gradient used was as follows: time (t) = 0–4 min, 98% solvent A, 2% solvent B; t = 10–15 min, 5% solvent A, 95% solvent B. The injection volume was 5 μL and the flow rate for chromatography was 200 μL/min. The amount of c-di-GMP in samples was calculated with a standard curve generated from pure c-di-GMP (Sigma-Aldrich, St. Louis, MO, USA) suspended in ddH2O (Biolog, Germany). c-di-GMP levels were normalised to bacterial cells, which were counted in a serially diluted bacterial culture in tube A that was grown on NYG plates for 48 h. Each c-di-GMP quantification experiment was performed with three biological replicates. The levels of c-di-GMP were compared with those of WT with the two-tailed Student’s t-test.
Diguanyl cyclase (DGC) and phosphodiesterase (PDE) activity assay
For the DGC activity assay, purified proteins were added to the reaction buffer (300 mM NaCl, 50 mM Tris-HCl, pH 7.5, 20 mM MgCl2, 2 mM DTT) and 20 μCi [32P]GTP (mixed with 50 μM cold GTP) was added. After 1 h at 28°C, the reaction was terminated by the addition of an equal volume of 0.5 M EDTA, pH 8.0. For the PDE activity assay, the purified RavR protein was added to the reaction buffer consisting of 50 mM Tris-HCl, pH 7.5, 250 mM NaCl, 25 mM KCl, 10 mM MgCl2 and 2 mM DTT. Reactions were initiated by the addition of ~1 μM of [32P]c-di-GMP substrate. Reactions were incubated at 28°C for 30 min before termination by adding an equal volume of 0.5 M EDTA, pH 8.0. For the DGC and PDE assays, reaction products were mixed with an equal volume of running buffer consisting of 1:1.5 (v/v) saturated (NH4)2SO4 and 1.5 M KH2PO4, pH 3.6. Two microlitres of the reaction mixture was spotted and dried onto Cellulose PEI TLC plates (Selecto Scientific, USA). Plates were developed in running buffer, air-dried and exposed to a storage phosphor screen (GE Healthcare) and then the autoradiographic signals were recorded on a Typhoon FLA7000 (GE Healthcare).
Homology modelling and molecular docking analyses
The three-dimensional structure of the DHp-CA domain of RavS was generated by homology modelling methods. Homology modelling was carried out using Modeller 9.10 software. The known structures of CpxAHDC (4BIU), DivL (4EW8) and VraS (4GT8) were used for multiple template homology modelling.
The structure of c-di-GMP was extracted from the c-di-GMP-VCA0042 structure complex (PDB ID: 2RDE). The structure of DHp-CA was treated by adding hydrogen atoms, calculating the charge and combining nonpolar hydrogens. Docking calculations were carried out using Autodock 4.0 software. Affinity (grid) maps of 40 × 40 × 40 Å grid points were generated using the Autogrid program. After 100 calculations, the lowest energy conformation was chosen for c-di-GMP and protein interaction analysis.
S1 Fig. Molar ratio of RavA, RavR and RavS in X. campesris pv. campestris.
(a) Semi-quantitative western blotting test of different concentrations of purified protein and cellular RavA, RavR and RavS in X. ccampestris pv. campestris. Three biological replicates were performed with each comprising of three technical repeats. (b–d) Quantification of western blotting band intensities by Image J software in (a) (n = 3).
S2 Fig. Inactivation of ravS, ravR and ravA did not impact bacterial growth, production of extracellular enzymes and the oxidative stress response.
(a) Growth curves of bacterial strains. All strains were cultured overnight in NYG medium. The OD600 was measured at intervals of 2 h. Standard deviations are given for each data point (n = 3). (b–d) Production of extracellular enzymes of bacterial strains. (b) Extracellular protease. (c) Extracellular cellulase. (d) Extracellular amylase. (e) Resistance to oxidative stress. A 0.2-mL aliquot of each bacterial culture (OD600 = 0.8) was spread onto an NYG plate and dried at room temperature. Then 5 μL of 1.63 M H2O2 was inoculated onto a round filter paper. In (b–e) the plates were incubated at 28°C for 36 h. Average diameters of degradation or inhibition zones (n = 5) are shown in the figures.
S3 Fig. mRNA levels of the flagella-related and hrp genes in X. campesris pv. campestris.
(a) Genetic location of ravARS genes and flagella-associated genes. Arrows indicate direction of genes. (b) mRNA levels of flagella-related genes. (c) mRNA levels of hrp genes. (d) mRNA levels of hrpG gene in various strains. Transcription levels of fliC, fliD, motA, motB, flgA, flgB, flhA flhB, hrpD, hrpF and hrpG were quantified by qRT-PCR. In studying hrp gene expression, the bacterial cells were induced in the XVM2 medium. Three biological replicates each comprising of three repeats were performed. The average value and standard deviation are shown (n = 3). Asterisk indicates statistically significant (P ≤ 0.05), as measured by a two-tailed Student′s t-test.
S4 Fig. Epistasis analysis reveals that ravS is downstream of ravA-ravR in regulation.
Deletion of ravS or point mutation of the conserved phosphorylation site (ravSH500A) suppresses the mutational effects of ravA or ravR deletions. Representative pictures of virulence (a) swimming ability (b) and flagella development (c) are shown.
S5 Fig. EAL domain of RavR has phosphodiesterase activity.
(a) Synthesis of 32P-labelled c-di-GMP by tDGC cyclase in vitro. c-di-GMP was synthesized and labelled by using tDGC cyclase from [32P]GTP. Samples were analysed on thin-layer chromatography (TLC) plates. (b) RavR did not possess diguanylate cyclase (DGC) activity. None or 5 μM affinity purified proteins including GGDEF, RavR, RavRΔEAL or tDGC were added to the DGC reaction mixture with α-32P-labeled GTP. After incubation at 28°C for 60 min, samples were analysed by TLC assays. (c) Recombinant EAL-domain containing protein naturally forms homodimer. The purified EAL protein was separated by a molecular sieve and the molecular weight of each fraction was determined by analytic ultra-centrifugation. (d) Phosphorylation of RavR did not affect its PDE activity. The enzymatic reactions contained 25 μM 32P-labelled c-di-GMP were analysed by TLC. RavR or RavRD496A (5 μM), RavA (10 μM) and ATP (2 mM) were added as indicated. (e) Intensity of the signals in (d), measured by ImageJ. (f) Intracellular c-di-GMP concentrations of various strains detected by LC-MS/MS analysis. All the experiments were repeated independently three times.
S6 Fig. Both RavA and RavS have autokinase activity and transfer the phosphoryl group to RavR in a RavRD496 dependent manner.
(a) RavA phosphorylates RavR in vitro. Autophosphorylation of the histidine kinase RavA and its recombinant derivative RavAH164A in the presence of [γ-32P]ATP at room temperature for 10 min. RavA phosphotransfer to RavR was then carried out for 30 s. Assays contained 10 μM of soluble protein RavA or RavAH164A. Ten micromolar RavR or RavRD496A was added into the mixtures as indicated. The experiment was repeated three times. (b) RavA phosphorylated the recombinant protein RavRΔEAL in vitro. Assays contained 15 μM of soluble protein RavA or RavAH164A. Five micromolar RavRΔEAL or RavRΔEAL(D496A) was added as indicated. (c) RavSΔN but not RavSΔTrM possesses robust autophosphorylation activity. Five micromolar of RavSΔTrM or RavSΔN was added into the in vitro autophosphorylation mixture in the presence of [γ-32P]ATP at room temperature for 10 min. (d–f) Detection phosphorylated HK and RR using Phos-tag acrylamide gel. (d) RavA phosphorylates RavR or RavRΔEAL in vivo. RavA or RavAH164A was incubated with 2 mM ATP at 28°C for 15 min, respectively. RavR (or RavRD496A) or RavRΔEAL (or RavRΔEAL(D496A)) was then added into mixtures for 2 min. (e and f) RavS phosphorylates RavRΔEAL or RavREAL-AAA in vitro. RavSΔN was autophosphorylated with 2 mM ATP at 28°C for 15 minutes. Various recombinant RavR proteins, including RavRΔEAL, RavRΔEAL(D496A), RavREAL-AAA or RavREAL-AAA(D496A) were added and incubated for 30 min at 28°C. A total of 100 μM c-di-GMP were added as indicated. The reactions were stopped with 3 × SDS loading buffer and the products were separated by 8% or 12% acrylamide gels at 4°C, the gels were stained with Coomassie brilliant blue (d–f). Each experiment was repeated three times.
S7 Fig. c-di-GMP specifically binds to RavS to enhance the RavS-RavR phosphotransfer.
(a) Expression of truncated RavS and RavR proteins. Numbers indicate the sites of amino acid residues of RavS or RavR. (b) RavSΔN specifically interacts with fl-c-di-GMP. The interactions of RavSΔN, RavA, VgrS and RavRΔEAL with fl-c-di-GMP were measured by microscale thermophoresis (MST). Twenty nanomolar fluorescein-labelled nucleotides and increasing concentrations of proteins were co-incubated and potential interactions were measured by MST. The dissociation constant (Kd) was determined to estimate the binding affinity. Averages and standard deviations are shown (n = 3). (c) Time course analyses of the impact of c-di-GMP on the velocity of RavS-RavR phosphotransfer. Representative pictures in Fig 5B are shown. Each experiment was repeated three times.
S8 Fig. Substitution of Arg656 residue did not affect the stability of the recombinant RavS protein in vitro and in vivo.
(a), R656A substitution did not affect the thermal stability of recombinant DHp-CA protein of RavS. Thermal stability of DHp-CA or DHP-CAR656A was tested using Thermal shift assay (TSA). Three independent experiments were performed and a representative result is shown. The average and the standard deviation of three midpoints of melt curves were displayed. (b), R656A substitution did not affect the autokinase activity of RavSΔN. RavSΔN or RavSΔN(R656A) autophosphorylates in the presence of [γ-32P]ATP at room temperature for various minutes. In vitro phosphorylation assay was used to measure the autokinase activity. The experiment was repeated for three times. (c), ravSR656A point mutation did not affect the stability of RavS in cell. Western blotting was used to detect the RavS. Samples were separated on 8% SDS-PAGE gel. Each experiment was repeated independently three times.
S9 Fig. Overexpression of ravS (OE-ravS) but not ravSH500A rescues the swimming motility of the ravRΔEAL mutant.
(a) Overexpression of ravS in bacterial cells. RavS was detected by western blotting. RNAP was used as the loading control. The experiment was repeated three times. (b–i) Phenotypic characterization of the effect of ravS overexpression. WT-EV (harbouring a medium-copy, broad-host pBBR1MCS2 vector), ravRΔEALΔravS-EV, ravRΔEALΔravS::OE-ravS and ravRΔEALΔravS::OE-ravSH500A strains of X. campestris pv. campestris. (b–c) Bacterial virulence. Bacterial strains were inoculated onto plant leaves of Brassica olercaeae cv Zhonggan 11. The lesion length was recorded 10 d after inoculation (n = 30). (d) Production of extracellular polysaccharides (EPS). Bacterial strains were grown in TGM medium at 28°C for 72 h before EPS quantification, which was calculated as the dry weight of EPS vs. the dry weight of bacterial cells (n = 3). (e) Swimming motility. Bacterial strains were inoculated in NYG plates containing 0.15% agar and grown below 28°C for 28 h. Average diameters of the migration zones were measured (n = 10). (f) Flagella of bacterial strains. Bacterial flagella were observed by transmission electron microscopy (TEM) after negative staining. Representative images of each strain are shown. Upper panel: bacteria population profile; lower panel: a single bacterium. (g) Ratio of bacterial cells with flagella. For each strain, cells with flagella were counted (n = 100). (h) Flagellar length of bacterial strains (n = 30). (i) fliC mRNA level in bacterial strains. The amount of fliC mRNA was measured by qRT-PCR. Amplification of cDNA of tmRNA was used as the internal control. In (c–e) and (g–i), vertical bars represent standard deviations; asterisk: significant differences were tested by Student’s t-test (P ≤ 0.05). The experiment was repeated three times and a representative result is shown.
S1 Table. Bacterial strains and plasmids used in this study.
The authors thank Ms. Yao Wu and Ms. Jing-Nan Liang of IM-CAS for their help in using HPLC and TEM. We thank Prof. Zhao-Xun Liang for providing the tDGC recombinant strain.
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