Abstract
Copper is an essential enzyme cofactor in bacteria, but excess copper is highly toxic. Bacteria can cope with copper stress by increasing copper resistance and initiating chemorepellent response. However, it remains unclear how bacteria coordinate chemotaxis and resistance to copper. By screening proteins that interacted with the chemotaxis kinase CheA, we identified a copper-binding repressor CsoR that interacted with CheA in Pseudomonas putida. CsoR interacted with the HPT (P1), Dimer (P3), and HATPase_c (P4) domains of CheA and inhibited CheA autophosphorylation, resulting in decreased chemotaxis. The copper-binding of CsoR weakened its interaction with CheA, which relieved the inhibition of chemotaxis by CsoR. In addition, CsoR bound to the promoter of copper-resistance genes to inhibit gene expression, and copper-binding released CsoR from the promoter, leading to increased gene expression and copper resistance. P. putida cells exhibited a chemorepellent response to copper in a CheA-dependent manner, and CsoR inhibited the chemorepellent response to copper. Besides, the CheA-CsoR interaction also existed in proteins from several other bacterial species. Our results revealed a mechanism by which bacteria coordinately regulated chemotaxis and resistance to copper by CsoR.
Introduction
Chemotaxis is a widespread ability of motile bacteria to direct their movement towards higher concentrations of beneficial chemicals or lower concentrations of toxic chemicals1, 2. Chemotaxis plays a vital role in bacterial exploration and adaptation to complex environments3,4. The chemotaxis signaling pathway is extensively studied in the enteric bacteria Escherichia coli and Salmonella enterica serovar Typhimurium2,5. In E. coli, the chemotaxis system consists of five methyl-accepting chemotaxis proteins (MCPs) and six core components (the kinase CheA, the response regulator CheY, the coupling protein CheW, the methylesterase CheB, the phosphatase CheZ, and the methyltransferase CheR). In response to decreased attractant or increased repellent, methylated MCPs and the coupling protein CheW activate CheA autophosphorylation6,7. The phosphorylated CheA (CheA-P) is a phosphodonor for the response regulator CheY and the methylesterase CheB. After CheY accepts the phosphate group from CheA, it binds FliM and FliN of the motor-switch complex, resulting in a switch in the flagellar rotational direction and bacteria tumbling8. Meanwhile, on a slower timescale, phosphorylated CheB demethylates the active MCPs, thus reducing their ability to activate CheA, leading to decreased levels of phosphorylated CheY and less tumbling9. The phosphatase CheZ contributes to signal termination by removing the phosphoryl group from phosphorylated CheY, and the methyltransferase CheR contributes to signal adaptation by catalyzing the methylation of MCPs2,5.
Among the bacterial chemotaxis system components, the kinase CheA is a five-domain enzyme central to the chemotaxis signaling pathway10,11. The five domains (P1-P5) of CheA each have distinct functions. The P1 domain (HPT domain) contains the phosphoryl-accepting histidine that becomes phosphorylated, the P2 domain (CheY-binding domain) docks the response regulator proteins CheY and CheB, the P3 domain (Dimer domain) dimerizes the CheA protein, the P4 domain (HATPase_c domain) binds ATP and catalyzes phosphoryl transfer to the histidine residue on P1, and the P5 domain (CheW-binding domain) couples CheA to other chemotaxis components by binding both CheW and the chemoreceptors10,11. Except for interacting with the components in chemotaxis system, CheA is reported to interact with proteins from other systems. For example, in the plant pathogen Xanthomonas oryzae pv. oryzicola, CheA interacts with and phosphorylates the response regulator VemR to regulate bacterial virulence, motility, and EPS production12. In Vibrio parahaemolyticus, a polarly localized protein ParP interacts with CheA and prevents its dissociation from chemotaxis signaling arrays, facilitating proper chemotaxis and accurate inheritance of these macromolecular chemotactic machines13. In Comamonas testosteroni, CheA interacts with and phosphorylates the response regulator FlmD, resulting in decreased biofilm formation14. In Azospirillum brasilense with two chemotaxis signaling systems, the kinase CheA from each chemotaxis signaling system physically interacts with the CheY response regulator of another system15. In Pseudomonas aeruginosa, CheA interacts with the phosphodiesterase DipA to regulate its subcellular localization and activity, leading to individual cell heterogeneity and motility behavior diversity in bacterial populations16. These studies suggest that the CheA-mediated crosstalk between chemotaxis and other systems coordinates complex behaviors in diverse bacteria.
In most living organisms, copper is an essential cofactor for enzymes involved in fundamental processes such as respiration and photosynthesis17,18. However, copper also has toxic effects on cells, and bacteria have several strategies to increase their resistance to copper20,21. The direct bacterial response associated with copper resistance is highly conserved and generally involves (a) sensing of the increased copper concentration by sensors, (b) activation of bespoke transcriptional networks, (c) overproduction of copper efflux pumps that secrete copper out of the cells, and (d) recruitment of copper-binding and copper-oxidizing proteins that prevent copper from interacting with cellular components22–26. In addition to the above copper resistance strategies, bacteria can avoid copper stress through chemotaxis. For example, in Caulobacter crescentus, the reactive oxygen species derived from cytoplasmic copper ions mediate the bacterial chemotaxis to copper, and a potential cytoplasmic MCP McpR regulates bacterial chemotaxis in response to cellular copper content, enabling bacteria to escape from copper-rich environment27,28. However, unlike the widely reported mechanisms of copper resistance in diverse bacterial species, the mechanism(s) of bacterial chemotaxis to copper is poorly studied. Besides, it remains unclear how bacteria coordinate chemotaxis and resistance to copper.
Since the kinase CheA plays a central role in chemotaxis signaling, identifying CheA-interacting proteins would extend the knowledge of chemotaxis regulation. In this study, by screening proteins that interacted with CheA in Pseudomonas putida, we obtained 16 novel CheA-interacting proteins. Among the 16 proteins, CsoR, a copper-binding transcription regulator, inhibited the autophosphorylation of CheA, leading to decreased chemotaxis. Meanwhile, CsoR functioned as a DNA-binding repressor to inhibit the expression of copper-resistance genes. Copper-binding of CsoR relieved its inhibition of gene expression and chemotaxis.
Results
Identification of new CheA-interacting proteins in P. putida
We performed a pull-down assay to identify protein(s) interacting with CheA. Purified 6 × His-tagged CheA bound onto a Ni-NTA agarose column was used as “bait” protein to pull out potential CheA-interacting “prey” protein(s) from whole cell lysate of P. putida KT2440, and a blank Ni-NTA agarose column was used as a negative control. All “prey” proteins from the CheA-binding column and control column were collected, resolved by SDS–PAGE (Fig. 1a), and analyzed by mass spectrometry (MS). In MS analysis, 43 proteins showed a significantly higher amount in the CheA-binding column than in the control column (Log2(fold change) > 2) (Fig. 1b, Table S1). As expected, the “bait” protein CheA showed the highest amount, with a Log2(fold change) value close to 8. Meanwhile, the response regulator CheY and the phosphatase CheZ (two proteins known to be associated with CheA) also showed high Log2(fold change) values. In addition to these three proteins (CheA, CheY, and CheZ), the remaining 40 proteins were considered potential new CheA-interacting proteins.
To verify the above result, we performed bacterial two-hybrid (BTH) assay to test the interactions between CheA and the 40 proteins. The results from the BTH assay revealed that 19 proteins showed apparent interaction with CheA, including PP_2969 (CsoR), PP_1612 (Eno), PP_4111 (FusB), PP_5046 (GlnA), PP_1074 (GlpR), PP_4728 (GrpE), PP_0853 (IspG), PP_1877 (MsrC), PP_2378 (NfuA), PP_1023 (Pgl), PP_5006 (PhaD), PP_0691 (ProB), PP_0148, PP_1644, PP_2683, PP_3177, PP_3227, PP_3501, and PP_4460 (Fig. 1c). Meanwhile, the rest 21 proteins displayed no significant interaction with CheA in BTH assay (Fig. S1a and S1b), suggesting that they were false positive results in the pull-down assay. We further tested the interactions between CheA and the 19 proteins in P. putida using bimolecular fluorescence complementation (BiFC) assay. The results displayed that except three proteins (PP_2683, PP_3227, and PP_4460) showed no apparent interaction with CheA, the other 16 proteins displayed obvious interaction with CheA in the BiFC assay (Fig. 1d, Fig. S2). Collectively, using pull-down, BTH, and BiFC assays, we identified 16 new CheA-interacting proteins in P. putida, including CsoR, Eno, FusB, GlnA, GlpR, GrpE, IspG, MsrC, NfuA, Pgl, PhaD, ProB, PP_0148, PP_1644, PP_3177, and PP_3501.
Effect of CheA-interacting proteins on bacterial chemotaxis
Since CheA played a crucial role in bacterial chemotaxis, we wondered whether the 16 CheA-interacting proteins were involved in regulating chemotaxis. Thus, we overexpressed each of the 16 proteins in wild-type P. putida and tested the chemotaxis ability. The wild-type P. putida harboring empty vector (WT+pVec) was used as the control. Chemotaxis ability was assessed using semisolid nutrient agar plates on which bacteria formed large colonies (swimming zone) by generating and following attractant gradients leading outward from the colony origin29. Growth of the 16 strains in liquid medium showed a similar trend as that of the control strain (Fig. S3), suggesting that the 16 proteins had no noticeable effect on bacterial growth. As shown in Fig. 2a, five strains (WT+pcsoR, WT+pispG, WT+pnfuA, WT+pphaD, and WT+pPP_1644) displayed smaller colony than the control strain (WT+pVec), indicating a weaker chemotaxis ability in these five strains. The other 11 strains showed a similar chemotaxis ability as WT+pVec. These results suggested that five CheA-interacting proteins (CsoR, IspG, NfuA, PhaD, and PP_1644) inhibited chemotaxis in P. putida.
CsoR and PhaD inhibit CheA autophosphorylation
CheA has autophosphorylation activity, and it can phosphorylate its cognate response regulator11. To test whether phosphate transfer existed between CheA and the 16 proteins, we performed a phosphate transfer assay using purified proteins and [32P]ATP[γP]. We successfully purified 14 out of the 16 proteins but failed to purify two proteins (GlpR and PP_3177) after several attempts. Thus, the two proteins were not included in the phosphate transfer assay. The results showed that CheA exhibited a strong autophosphorylation signal after incubation with [32P]ATP[γP] for 45 min (Fig. S4a). Then, each of the 14 proteins or CheY (positive control) was added to phosphorylated CheA to investigate the phosphate transfer. The addition of CheY to phosphorylated CheA led to a labeling of CheY and a reduction in the phospholabeling of CheA (Fig. S4a), indicating a phosphate transfer happened between CheA and CheY. However, no labeling of the 14 target proteins was observed, and there was no apparent change in the phospholabeling of CheA after adding each of the 14 proteins (Fig. S4a), suggesting no phosphate transfer happened between CheA and the 14 tested proteins.
Then, we wondered whether the 14 proteins influenced CheA autophosphorylation. To answer this question, we mixed CheA with each of the 14 proteins before adding the substrate [32P]ATP[γP]. The mixture containing CheA and bovine serum albumin (BSA) was used as a negative control. As shown in Fig. 2b, CsoR/PhaD significantly decreased the phospholabeling of CheA. In contrast, the other 12 proteins and BSA had no apparent influence on the phospholabeling of CheA. We further tested the impact of CsoR/PhaD on CheA autophosphorylation with a more detailed assay, in which CheA was mixed with an increased amount of CsoR/PhaD. The results showed that CheA phospholabeling decreased as CsoR/PhaD increased. In contrast, the increase of BSA had no obvious influence on CheA phospholabeling (Fig. 2c and 2d). These results indicated that CsoR and PhaD inhibited CheA autophosphorylation. It was also possible that CsoR and PhaD degraded the substrate[32P]ATP[γP] in the reaction mixture, resulting in decreased CheA autophosphorylation. To test this possibility, we examined whether CsoR and PhaD had ATPase activity. The known ATPase FleQ was used as a positive control, and BSA was used as a negative control. The results showed that adding FleQ into the reaction mixture caused a decrease in ATP level (Fig. S4b), indicating the existence of ATPase activity. Meanwhile, the addition of CsoR/PhaD exhibited no apparent influence on ATP level as the addition of BSA (Fig. S4b), suggesting that CsoR and PhaD had no ATPase activity.
In the chemotaxis signaling pathway, CheA transfers the phosphate group to the response regulator CheY to modulate flagellar rotation2,5. Since CsoR and PhaD interacted with CheA, we wondered whether CsoR/PhaD influenced the phosphate transfer between CheA and CheY. Thus, we incubated CsoR/PhaD with the phosphorylated CheA before adding CheY to the reaction mixture. The results revealed that CheA phospholabeling in the CsoR/PhaD-adding group reduced to a similar level as that in the group without CsoR/PhaD (Fig. S4c), implying that CsoR/PhaD had no apparent influence on the phosphate transfer between CheA and CheY.
The domains of CheA involved in interacting with CsoR and PhaD
To further explore how CsoR and PhaD affect CheA autophosphorylation, we determined the domain(s) of CheA involved in interacting with CsoR and PhaD. Similar to the E. coli CheA, the P. putida CheA consists of five domains with distinct functions (Fig. 3a). We constructed five truncated CheA variants, with each missing one domain (termed CheAΔHPT/CheAΔYB/CheAΔDim/CheAΔHATPase/CheAΔWB) (Fig. 3a). Then we performed BTH assay to test the interaction between CsoR/PhaD and each of these truncated CheAs. The results revealed that three truncated CheAs (CheAΔHPT, CheAΔDim, and CheAΔHATPase) showed no interaction with CsoR and PhaD. In comparison, the other two truncated CheAs (CheAΔYB and CheAΔWB) interacted with CsoR and PhaD with a similar intensity as the wild-type CheA did (Fig. 3b and 3c), indicating that the HPT (P1), Dimer (P3), and HATPase_c (P4) domains were essential for interacting with CsoR and PhaD, while the YB (P2) and WB (P5) domains were not required to interact with CsoR and PhaD. To further test this result, we cloned each of the five domains into a BTH vector and tested the interaction between CsoR/PhaD and each of the five domains. The result showed that the Dimer domain (DimCheA) interacted with CsoR and PhaD like the whole-length CheA did (Fig. 3b and 3c). The HPT domain (HPTCheA) and the HATPase_c domain (HATPaseCheA) showed a weaker interaction with CsoR and PhaD. Meanwhile, the YB domain (YBCheA) and the WB domain (WBCheA) displayed no interaction with CsoR and PhaD (Fig. 3b and 3c). Together, these results revealed that the Dimer domain (P1) of CheA played a significant role, the HPT (P3) and HATPase_c (P4) domains played a minor role, while the CheY-binding (P2) and CheW-binding (P5) domains played no role in the interaction between CheA and CsoR/PhaD. Since the three domains involved in interacting with CsoR/PhaD were also essential for CheA autophosphorylation activity10,11, CsoR/PhaD might inhibit CheA autophosphorylation by inhibiting the function of the three domains.
CsoR is a copper-binding transcriptional repressor for copper-resistance genes
Of the two proteins that inhibit CheA autophosphorylation, CsoR is annotated as a metal-binding transcriptional repressor30. The homolog of CsoR in Mycobacterium tuberculosis binds to copper and regulates the expression of copper-resistance genes31,32. However, the metal-binding ability and the function of the P. putida CsoR were not experimentally characterized. Thus, we tested the metal-binding ability of the P. putida CsoR using MicroScale Thermophoresis (MST). Six metal ions were involved in the assay, including copper (Cu2+), zinc (Zn2+), nickel (Ni2+), cobalt (Co2+), cadmium (Cd2+), and magnesium (Mg2+). The results revealed that CsoR bound to three out of the six tested metal ions (Cu2+, Zn2+, Ni2+), and the binding to Cu2+ was the strongest with a calculated binding constant (Kd) of 5.5 ± 1.98 μM. In contrast, the binding to Ni2+ and Zn2+ was weak (with Kd value of 125 ± 38 μM and 253 ± 42 μM, respectively) (Fig. 4a). Meanwhile, CsoR showed no apparent binding to Co2+/Cd2+/Mg2+ under the same condition (Fig. 4a). We further constructed a csoR deletion mutant (ΔcsoR) and investigated the effect of csoR deletion on the expression of copper-resistant genes using quantitative real-time PCR (qRT-PCR). Three key copper-resistant-related genes (copA-I, copA-II, and copB-II) from two copper-resistant-related operons were chosen as targets in qRT-PCR. The results showed that csoR deletion (ΔcsoR+pVec) led to a weak but significant increase (about 1.3-fold) in the expression of the three genes, and complementation (ΔcsoR+pcsoR) decreased the expression of the three genes (Fig. 4b). The addition of CuCl2 (final concentration 10 μM) induced the expression of the three genes (about 5-fold) (Fig. 4b). However, no noticeable difference in gene expression level was observed between WT+pVec and ΔcsoR+pVec, as well as between ΔcsoR+pVec and ΔcsoR+pcsoR (Fig. 4b), implying that CsoR was not required for the copper-induced genes expression. Besides, the deletion of cheA (ΔcheA+pVec) displayed no obvious effect on the expression of the three genes in either the presence or absence of copper (Fig. 4b). Together, these results demonstrated that CsoR functioned as a copper-binding repressor for copper-resistant genes in P. putida.
Previous studies reported that CsoR bound the promoter of target genes to inhibit gene expression31,33. We further tested the interaction between CsoR and the promoter of copA-I using electrophoretic mobility shift assay (EMSA). The fragment of copA-I promoter exhibited a stepwise increase in the shifted DNA amount (CsoR-DNA complex), with the CsoR protein amount increasing from 5 to 20 μM (Fig. 4c).
Adding Cu2 to the reaction mixture decreased the CsoR-DNA complex (Fig. 4c), indicating that Cu2+ inhibited the interaction between CsoR and promoter DNA. Besides, Ni2+, Zn2+, and Cd2+ also exhibited an inhibitory effect on the interaction between CsoR and promoter DNA, but to a much lower extent compared with Cu2+ (Fig. 4d). Meanwhile, Co2+ and Mg2+ displayed no obvious effect on the CsoR-DNA interaction (Fig. 4d). These results showed that CsoR was a promoter-binding transcriptional repressor, and binding to metal (especially copper) decreased the interaction between CsoR and promoter DNA.
Copper inhibits the interaction between CheA and CsoR
Since CsoR interacted with CheA and bound copper, we wondered whether copper affected the interaction between CheA and CsoR. Thus, we investigated the interaction between CheA and CsoR under different CuCl2 concentrations using MST. As revealed in Fig. 5a, CheA showed strong interaction with CsoR in the absence of Cu2+ (Kd= 0.17 ± 0.1 μM), and the addition of Cu2+ (20 and 200 μM) led to increased binding constant (0.59 ± 0.2 μM and 2.15 ± 0.97 μM), indicating that copper decreased the interaction between CheA and CsoR. A similar trend was observed in the pull-down assay, in which the amount of CsoR bound by CheA gradually decreased with the concentration of Cu2+ increased from 2 to 20 μM (Fig. 5b).
A previous study on M. tuberculosis CsoR revealed three residues that played a vital role in copper-binding31. The alignment assay showed that the three residues were conserved among CsoR homologs from several bacterial species, including the P. putida CsoR (Fig. S5a). To test the role of the three residues in copper-binding, we individually replaced each of the three residues (Cys40, His65, and Cys69) with alanine and tested the copper-binding ability of these mutated CsoRs (CsoRC40A, CsoRH65A, and CsoRC69A). MST results showed that the CsoRC69A displayed significantly decreased copper-binding ability compared to wild-type CsoR. In contrast, CsoRC40A and CsoRH65A showed a slight decrease in copper-binding ability compared with that of the wild-type CsoR (Fig. S5b), suggesting that the Cys69 residue of CsoR played a critical positive role in copper-binding. Besides, the results from EMSA also supported this conclusion, in which the mutation of C69A, but not C40A/H65A, noticeably inhibited the effect of Cu2+ on CsoR-DNA interaction (Fig. S5c and S5d). BTH assay revealed that the three point-mutated CsoRs interacted with CheA with a similar intensity to the wild-type CsoR (Fig. S5e). Results from the pull-down assay showed that the addition of Cu2+ significantly decreased the amount of CsoRC40A and CsoRH65A bound by CheA, but had less effect on the amount of CsoRC69A bound by CheA under the same condition (Fig. 5b). Together, these results revealed that copper bound CsoR and inhibited its interaction with CheA.
Copper relives the inhibition of CsoR on bacterial chemotaxis
Since CsoR interacted with CheA and inhibited its autophosphorylation, and copper hindered the interaction between CheA and CsoR, we speculated that copper might relieve the inhibition of CsoR on CheA autophosphorylation. To test this hypothesis, we added CsoR and copper to the reaction mixture containing CheA and then analyzed the autophosphorylation of CheA using [32P]ATP[γP]. CsoR alone significantly inhibited CheA autophosphorylation, while adding CsoR and copper showed weaker inhibition on CheA autophosphorylation (Fig. 5c). Besides, CsoRC69A showed similar inhibitory effects on CheA autophosphorylation in the presence and absence of Cu2+ (Fig. 5c), indicating that binding with CsoR was the prerequisite for Cu2+ to relieve the inhibition of CsoR on CheA autophosphorylation.
We further tested the effect of CsoR on chemotaxis in the presence of copper using the semisolid plate. As shown in Fig. 5d, in the absence of Cu2+, the overexpression of point-mutated CsoR (CsoRC40A/CsoRH65A/CsoRC69A) led to a similar decrease (about 40%) in chemotaxis as the overexpression of wild-type CsoR. In comparison, in the presence of 200 μM Cu2+, the inhibitory effect of CsoR/CsoRC40A/CsoRH65A overexpression on chemotaxis was weaker (about 20%). However, the inhibitory effect of CsoRC69A overexpression on chemotaxis was not affected by Cu2+ (Fig. 5d). These results demonstrated that binding copper relieved the inhibition of CsoR on bacterial chemotaxis.
CsoR inhibits chemorepellent response to copper
Excess copper is toxic to cells, and bacteria avoid high copper concentrations through chemotaxis. Since CsoR interacted with CheA and inhibited chemotaxis, we wondered about the role of CsoR in bacterial chemotaxis to copper. Thus, we tested the chemotaxis response of P. putida to copper gradient and the role of CsoR and CheA in this response using semisolid plates. The copper gradient was achieved by placing an agar plug containing 200 mM CuCl2 in the center of a semisolid plate, and bacterial cells were spotted two centimeters away from the plug to test their chemotaxis to Cu2+. An agar plug without CuCl2 was also placed in the center of a semisolid plate and used as a negative control. As shown in Fig. 6a, the swimming zone of all tested strains was a circle shape in the control plate without CuCl2. However, all swimming zones showed an oval shape in the plate with CuCl2 gradient (Fig. 6a), in which the bacterial movement distance near the plug (D1) was short, and the movement distance from the plug (D2) was long, indicating that the strains showed chemorepellent response to CuCl2. The RI value (Response index value, RI=D1/(D1+D2)) was further calculated to characterize the strength of the chemorepellent response to CuCl2. The results showed that WT+pcsoR displayed a higher RI value (0.428 ± 0.015) than WT+pVec (0.373 ± 0.021) (Fig. 6b). Meanwhile, ΔcsoR+pVec showed a lower RI value (0.324 ± 0.013) than WT+pVec, and complementation increased the RI value to wild-type level (Fig. 6b). These results suggested that CsoR inhibited the chemorepellent response to copper. Besides, both cheA deletion mutant (ΔcheA+pVec) and cheA csoR double deletion mutant (ΔcsoRΔcheA+pVec) displayed no chemotaxis ability in either the presence or absence of copper gradient (Fig. 6a and 6b), indicating that CsoR inhibited chemotaxis ability in a CheA-dependent manner.
Using time-lapse microscopy experiments and cell-tracking analysis, we further examined the bacterial chemorepellent response to Cu2+. In the control group without chemokine (Cu2+ gradient), cells of all tested strains swam randomly in all directions (Fig. 6c). The center of mass (defined as the average of all single cell endpoints, and it reflects the movements of target strain and the strength of chemotaxis response) of all tested strains showed no apparent difference (Fig. 6d). In the group with chemokine (Cu2+ gradient), cells of WT+pVec, WT+pcsoR, ΔcsoR+pVec, and ΔcsoR+pcsoR migrated towards the lower concentration of Cu2+ (Fig. 6c). In comparison, cells of ΔcheA+pVec and ΔcsoRΔcheA+pVec still swam randomly in all directions (Fig. 6c), indicating that P. putida cells showed a chemorepellent response to Cu2+ in a CheA-dependent manner. The center of mass value of WT+pcsoR (13.85 ± 1.92 μm) was smaller than that of WT+pVec (21.77 ± 3.60 μm) (Fig. 6d). Meanwhile, the center of mass value of ΔcsoR+pcsoR (14.16 ± 1.41 μm) was smaller than that of ΔcsoR+pVec (21.39 ± 2.02 μm) (Fig. 6d), suggesting that CsoR inhibited bacterial chemorepellent response to Cu2+. The velocities (cell migration speeds) of cells from WT+pcsoR, ΔcsoR+pVec, and ΔcsoR+pcsoR were similar to that from WT+pVec both in the presence and absence of Cu2+ gradient, implying that CsoR had no evident influence on bacterial migration speed. In contrast, the velocities of cells from ΔcheA+pVec and ΔcsoRΔcheA+pVec were lower than that from WT+pVec (Fig. 6e), indicating that CheA played a positive role in bacterial migration speed. Together, these results demonstrated that CsoR inhibited the chemorepellent response to copper in a CheA-dependent manner.
The interaction between CheA and CsoR exists in several bacterial species
The role of CsoR in regulating copper resistance has been reported in several bacterial species, including Acidithiobacillus caldus33, Bacillus subtilis34, Bradyrhizobium diazoefficiens35, Corynebacterium glutamicum36, Listeria monocytogenes37, M. tuberculosis31, Staphylococcus aureus38, Streptomyces lividans39, and Thermus thermophilus40. BLAST results showed that four of the nine above species (A. caldus, B. diazoefficiens, B. subtilis, and L. monocytogenes) had both cheA and csoR on their genomes. Besides, in addition to P. putida, cheA and csoR coexist in other Pseudomonas species, including Pseudomonas fluorescens, Pseudomonas syringae, and Pseudomonas stutzeri. We wondered whether the CheA-CsoR interaction also occurred between proteins from these strains. Thus, we tested the interaction between CheA and CsoR of the same strain via BTH assay. The result showed that the CheA-CsoR interaction existed between proteins from A. caldus, B. subtilis, P. syringae, and P. stutzeri (Fig. 7). However, CheA and CsoR from B. diazoefficiens, L. monocytogenes, and P. fluorescens showed no apparent interaction (Fig. 7). Besides, the intensity of CheA-CsoR interaction was more vigorous between the two proteins from B. subtilis, but weaker between that from A. caldus, P. syringae, and P. stutzeri (Fig. 7). These results suggested that except in P. putida, the interaction between CheA and CsoR also existed in other bacterial species.
Discussion
Integrating components from different systems provides a straightforward mechanism for coordinating signaling from various systems. This study identified an interaction between the chemotaxis kinase CheA and the copper-responsive transcriptional repressor CsoR in P. putida. Further analysis revealed that CsoR inhibited bacterial chemotaxis via interacting with CheA and hindering its autophosphorylation. Meanwhile, CsoR regulated copper resistance by modulating the expression of copper-resistance genes. Together with previous reports41–43, we proposed a potential model to describe the function of CsoR in regulating copper resistance and bacterial chemotaxis. As shown in Fig. 8, under low copper levels, CsoR molecules exist mainly in none copper-binding status (free CsoR) in the cell, and the free CsoR forms tetramer and binds to promoters of copper-resistance genes (such as copA-I), leading to repressed gene transcription and copper resistance ability. Meanwhile, the free CsoR interacts with CheA and inhibits its autophosphorylation, decreasing bacterial chemotaxis ability. Under high copper levels, more copper-binding CsoR molecules exist, and copper-binding changes the conformation of the CsoR tetramer and releases CsoR from promoters, leading to increased gene transcription and copper resistance. Besides, the copper-binding of CsoR decreases the interaction between CsoR and CheA, which relieves the inhibition of CsoR on CheA autophosphorylation, resulting in increased chemotaxis ability.
In classical chemotaxis signaling, MCP on the cell membrane senses external signaling molecules and regulates bacterial chemotaxis by mediating CheA autophosphorylation activity5,7. MCPs can directly bind diverse external signaling molecules, such as amino acids, dipeptides, sugars, tricarboxylic acid cycle intermediates, aromatic molecules, and inorganic phosphate44. However, there are only a few reports on the relationship between MCP and metal ions45–47, and no evidence supports that MCP senses metal ions by direct binding. It is possible that bacteria sense and trigger chemotaxis to metal ions differently from that they sense and trigger chemotaxis to external signaling molecules like amino acids. Our results provide a mechanism by which bacteria sense copper and regulate chemotaxis via the copper-responsive repressor CsoR. Through the interaction between CsoR and CheA, bacteria coordinately regulated chemotaxis and resistance to copper stress, which would favor the bacteria to better adapt to complex environments. Besides, the interaction between CsoR and CheA was not limited to the proteins from P. putida, and it was also found in proteins from several other bacterial species (Fig. 7), implying that the regulation of chemotaxis and resistance to copper via the interaction between CsoR and CheA might be a widespread regulatory mechanism.
Although the P. putida CsoR functioned as a copper-responsive regulator to modulate the expression of copper-resistance genes, its effect on gene expression was much weaker than its homologous protein in other bacterial species. In M. tuberculosis, B. subtilis, C. glutamicum, L. monocytogenes, and S. aureus, deletion of csoR resulted in an about 10-fold increase in the expression of target genes in the absence of copper32,34,36,37,38. In contrast, deletion of csoR in P. putida led to a slight but reproducible increase (about 1.3-fold) in gene expression in the absence of copper (Fig. 4b). This difference might be attributed to the existence of several key regulators that activated the expression of copper-resistance genes in response to copper in P. putida, such as CueR and CopR. CueR positively regulated the expression of cueA, encoding a copper-transporting P1-type ATPase that played a crucial role in copper resistance48. CopR was essential for expressing several genes implicated in cytoplasmic copper homeostasis, such as copA-II, copB-II, and cusA49,50. The existence of these positive regulators makes the function of CosR a secondary or even dispensable insurance in the expression of copper-resistance genes. Consistent with this, there is no CosR homolog in P. aeruginosa, and copper homeostasis in P. aeruginosa is mainly controlled by CueR and CopR50,51.
Through pull-down, BTH, and BiFC assays, we obtained 16 new CheA-interacting proteins involved in different physiological processes (Table S1). Among the 16 proteins, five proteins (CsoR, IspG, NfuA, PhaD, and PP_1644) inhibited bacterial chemotaxis on semisolid plates (Fig. 2a). Our study here focused on the physiological role of CsoR-CheA interaction. Still, the function of other interactions remained unclear. PhaD is a TetR family transcriptional regulator that behaves as a carbon source-dependent activator of the pha cluster related to polyhydroxyalkanoates (PHAs) biosynthesis52,53. Bacterial PHAs are isotactic polymers synthesized under unfavorable growth conditions in the presence of excess carbon sources. PHAs are critical in central metabolism, acting as dynamic carbon reservoirs and reducing equivalents54. The interaction between PhaD and CheA leads one to speculate that there might be some connection between PHA synthesis and bacterial chemotaxis. Another CheA-interacting protein, PP_1644, also attracts our interest. PP_1644 is annotated as a NAD(P)H dehydrogenase involved in cyclic electron transport and respiration processes. Exploring the physiological role of the interaction between CheA and these proteins in the future helps to reveal the association between the chemotaxis process and other physiological metabolisms.
Materials and Methods
Bacterial strains and growth conditions
All strains and plasmids used in this study are listed in Supplementary Table S2. Unless specifically mentioned, E. coli strains were grown in lysogeny broth (LB) medium at 37°C. P. putida KT2440 and its derivative strains were cultured at 28°C in LB medium or chemically defined M9 minimal medium supplemented with 40 mM glucose as carbon source. Antibiotics were used, when required for plasmid maintenance or transformants screening, at the following concentrations: kanamycin (50 mg/L), carbenicillin (50 mg/L), chloramphenicol (25 mg/L), and gentamycin (20 mg/L for E. coli or 40 mg/L for P. putida).
Plasmid and strain construction
The routine cloning of DNA fragments into plasmid was performed by following a T5 exonuclease-dependent method55. Briefly, a 14 base pairs (bp) homologous end was added to the 5’ of primer during synthesizing. Amplified DNA fragments and linearized plasmid containing the same homologous end were incubated in a reaction buffer containing T5 exonuclease (0.04 U) and left at 30℃ for 40 min before transforming into E. coli competent cells. Primers used for plasmid construction are listed in Supplementary Table S3. All cloning steps involving PCR were verified by commercial sequencing (Tsingke, Wuhan, China).
Gene deletion mutant was constructed by homologous recombination using the suicide plasmid pBBR401. For example, to construct a markerless P. putida csoR deletion mutant, ~800 bp from the chromosomal regions flanking csoR (upstream region and downstream region) were PCR-amplified. The PCR products were cloned into pBBR401 to create pBBR401-csoRUP-DOWN. Then, the final plasmid was transferred to P. putida by electroporation. The integration strain was selected on plates containing gentamicin. After subculturing the integration strain in LB medium without antibiotics six times (12 h each time), single colonies were obtained by plate streaking. Then, colonies losing gentamicin resistance were kept for further verification. The csoR delete mutant was confirmed by PCR and sequencing.
To generate a csoR/cheA overexpression plasmid, a DNA fragment containing the complete csoR/cheA was PCR amplified. The product was cloned into expressional vector pBBR403 to yield pBBR403-csoR/cheA. The expression of csoR/cheA on pBBR403-csoR/cheA was controlled by an inducible tac promoter. To construct a vector for target protein expression and purification, we amplified and cloned the target gene into pET-28a with 6 × His tag or pHS-Strep with Strep II tag. Overlapping PCR was used to create point mutations of CsoR. To construct a C40A point mutation in CsoR, we amplified two fragments with two primer pairs (CsoRC40A s1/CsoRC40A a1 and CsoRC40A s2/CsoRC40A a2). The CsoRC40A a1 and the CsoRC40A s2 shared reverse complementary sequences containing the point mutation in which the original TGC codon of arginine was replaced by GCC of alanine. The two fragments were mixed in a 1:1 ratio to perform overlapping extension. The final PCR product was cloned into pET-28a and pBBR403. The mutation in csoR was confirmed by sequencing.
Expression and purification of His/Strep II-tagged proteins
For the expression of His/Strep II-tagged protein, overnight culture of E. coli BL21 carrying the construct of target proteins was 1:100 diluted into LB medium and incubated for 4 h at 37°C. Then, 0.4 mM IPTG (isopropyl-D-thiogalactopyranoside) was added to induce protein expression. After 4 h incubation at 16°C, cells were harvested and resuspended in lysing buffer (10 mM Tris-Cl [pH 7.8], 300 mM KCl, and 10% (w/v) glycerol). The harvested cells were lysed using a pressure cell breaking apparatus, and cell debris was removed by centrifugation at 15000 rpm for 20 min. The supernatants were then filtered through a 0.22-μm-pore-size filter and loaded onto a Ni-NTA Resin column (for His-tagged protein) or Strep-Tactin Resin column (for Strep II-tagged protein). Target proteins were eluted using an imidazole gradient (50/100/150/200mM imidazole for His-tagged protein) or 50 mM biotin (for Strep II-tagged protein) and then dialyzed overnight against lysing buffer to remove imidazole. The concentrations of obtained proteins were determined using BCA assay.
Protein-protein pull-down assay
Protein-protein pull-down assay was used to identify CheA-interacting protein and test the effect of copper on CheA-CsoR interaction. Briefly, 6 × His/Strep II-tagged CheA was induced and loaded to a Ni-NTA/Strep-Tactin column as described above. Then, overnight cultured wild-type KT2440/BL21 strain expressing CsoR was harvested, lysed, and filtered before adding to the same column. For the pull-down assay to identify CheA-interacting protein, the same volume of wild-type extract was added to a blank Ni-NTA column as a negative control. For the pull-down assay to test the effect of copper on CheA-CsoR interaction, various amounts of CuCl2 were mixed with the cell extract containing CsoR before being added to the Strep-Tactin column. Then, the columns were sealed and incubated at 4°C with 40 rpm shaking. After 2 h incubation, the supernatant was removed, and the columns were washed with lysing buffer containing 20 mM imidazole (for Ni-NTA column) or lysing buffer (for Strep-Tactin column) to wash the unspecific binding protein away. Then, elution buffer containing 250 mM imidazole (for the Ni-NTA column) or 50 mM biotin (for the Strep-Tactin column) was added to wash down all proteins on the column. The eluted proteins were collected and resolved by 12.5% SDS–PAGE followed by Coomassie blue staining and mass spectrometry analyses.
Mass spectrometry (MS)-based protein sequencing
After Coomassie blue staining of eluted proteins obtained from pull-down assay, the whole lane of the experimental or control sample was excised from gels and prepared for MS analysis. Protein from the excised gels was extracted with a Micro Protein PAGE Recovery Kit (Sangon Biotech, China) following the operating instructions. Then, trypsin digestion of extracted protein was performed with 1 g trypsin (Promega, USA) and incubated at 37°C overnight. The digestion was terminated by adding trifluoroacetic acid (TFA). Then, desalting was subsequently performed using Zip-tip (Merck Millipore, Ireland). Peptides were eluted from the Zip-tip with 50 μL of matrix solution (5 mg/mL α-cyano-4-hydroxycinnamic acid, 50% acetonitrile, 0.1% TFA). The supernatant was collected and concentrated to a final volume of 10 μL in a centrifugal concentrator.
The samples were analyzed using the MALDI-TOF/TOF mass spectrometer (Applied Biosystems, USA). Mass spectra were recorded in the positive-ion mode, averaging 2500 laser shots per spectrum. Mass spectra (excluding trypsin autolytic peptides and other known background ions) were searched against the P. putida proteome from the UniProt database to identify the proteins. The search was performed using trypsin digestion, allowing two missed cleavages, specifying carbamidomethyl-Cys as a fixed modification, and setting a peptide mass tolerance of ± 1.6 Da. The global false discovery rate (FDR) cutoff for peptide and protein identification was set to 0.01. An intensity-based absolute quantification (iBAQ) algorithm was used to rank the relative abundance of different proteins as previously described56. iBAQ percentage of specific proteins in the experimental sample (iBAQ_T (%)) and control sample (iBAQ_CK (%)) were used to represent relative protein concertation. Log2 (iBAQ_T/iBAQ _CK) fold change of ≥ 2 or ≤2 and a P value of ≤ 0.05 was considered significantly different.
Bacterial two-hybrid (BTH) assay
For bacterial two-hybrid analysis of protein-protein interactions of P. putida proteins expressed in E. coli, each ORF was cloned in-frame with the T18 and T25 fragments of adenylate cyclase ORF in vectors pUT18C and pKT25. Primers used to amplify each ORF are listed in Table S3. The resulting vectors were co-transformed into E. coli BTH101 and plated onto LB agar plate supplemented with 50 mg/L carbenicillin, 50 mg/L kanamycin, 40 mg/L 5-bromo-4-chloro-3-indolyl-b-D-galactopyranoside (X-gal), and 0.5 mM IPTG, and incubated at 28°C for 48 h. Three co-transformants for each assay were cultured to stationary phase in LB broth at 28°C, then spotted onto an LB agar plate supplemented as above, and incubated for 60 h at 28°C. Plates were then scanned on a Tanon 2500 scanner. The LacZ activity of spotted colonies was measured using o-nitrophenyl-β-galactopyranoside (ONPG) as substrate, as described before57. The experiments were repeated three times with three technical repeats per sample, and the data are presented as Miller units.
Bimolecular fluorescence complementation (BiFC) assay
BiFC was used to analyze protein-protein interactions as previously described58. Briefly, to determine the interaction between two interested proteins (such as CheA and CsoR), CheA was fused to KN151 (the N-terminal of mLumin), and CsoR was fused to LC151 (the C-terminal of mLumin), yielding a recombinant plasmid pBBR403-CheA-KN151-CsoR-LC151. Then, the recombinant plasmid was transformed into the wild-type P. putida strain. Transformants were picked and cultured in LB medium containing 40 mg/L gentamycin and 0.5 mM IPTG for 24 h at 28℃. Then, images of the dark-filed and bright field of the transformant cells were obtained using FV1000 CLSM (Olympus, Japan) equipped with a 100×/1.4 oil immersion objective lens. Besides, the transformant cells were washed twice with 0.9% NaCl, and then fluorescence intensities and OD600 were measured using a Spark microplate reader (Tecan, Switzerland). Fluorescence intensity and OD600 were detected using the black and transparent microplate, respectively. The excitation and the emission wavelength to detect fluorescence were 587 nm and 620 nm, respectively, and the experiment was repeated twice with triplicates.
Microscale thermophoresis (MST) assay
MST was performed to analyze the interaction between two proteins or proteins and metal ions. Briefly, to test the interaction between CsoR and copper. A green fluorescent protein (GFP) encoding gene was fused to the end of csoR in pET-28a-csoR to achieve fusion expression. The fusion protein CsoR-GFP was induced and purified as described above in protein induction and purification. The obtained CsoR-GFP was dialyzed with MST buffer (50 mM Tris-HCl [pH 7.8], 150 mM NaCl, 0.05% Tween 20). The MST assay was performed on a Monolith Instrument NT.115 device using standard treated capillaries (NanoTemper Technologies, Germany). The concentration of CsoR-GFP was constant at 250 nM, and the CuCl2 concentration was varied from 0.031 to 1000 μM with a 2-fold gradient. The experiment was recorded using the Nano-BLUE fluorescent detector. Measurements were performed in MST buffer. The MO. Affinity Analysis software (version 2.3) was used to calculate the dissociation constant (Kd) from triplicate reads of measurements.
In vitro phosphorylation assays
For the autophosphorylation reaction, purified CheA (3 μM) was incubated in phosphorylation buffer containing 50 mM Tris–HCl [pH 7.5], 15 mM MgCl2, and 50 mM NaCl. The reaction was initiated by adding 0.03 μCi of [32P]ATP[γP] (PerkinElmer, USA) to the mixture. SDS-PAGE loading buffer containing SDS and EDTA was added to the mixture to terminate the reaction at the indicated time. To test the effect of target proteins on CheA autophosphorylation, target protein (10 μM) was mixed with CheA (3 μM) for 10 min before adding [32P]ATP[γP]. To test the transphosphorylation reaction, CheA was autophosphorylated before CheY/target protein (10 μM) was added to the mixture, and the reaction mixture was incubated at 30°C for different time intervals before being terminated with SDS-PAGE loading buffer. Samples were heated at 95°C for 5 min and then resolved by 12.5% SDS– PAGE. After drying of the gels, products were visualized by autoradiography.
RNA extraction and real-time RT-PCR (qRT-PCR) assay
P. putida cells were cultured in M9 minimal medium supplemented with 40 mM glucose as carbon source for 24 h. Then, cells were harvested and washed thrice with sterilized phosphate buffer saline (PBS) before being divided into two equal parts. One part was resolved with fresh M9 medium and another with M9 medium containing 10 μM CuCl2. After 30 min incubation, cells were harvested for RNA extraction using a total RNA extraction reagent (Vazyme R401-01, China) as recommended by the manufacturer. 1 μg extracted RNA was digested with DNase I and reverse transcribed to cDNA using a reverse transcription kit (Takara RR047A, Japan), and cDNA was used as the template for qRT-PCR analysis. The qRT-PCR assay was performed using Power SYBRTM Green PCR mix (Applied Biosystems 4367659, USA) and analyzed using a QuantStudio™ 3 Real-Time PCR System (Applied Biosystems, USA). The rpoD gene was selected as an internal control. The primers used in qRT-PCR analysis are listed in Supplementary Table S3. All experiments were performed thrice with three technical repeats per sample.
Electrophoretic mobility shift assay (EMSA)
EMSA was used to test the interaction between CsoR and copA-I promoter DNA. Equal amounts of DNA (60 ng) were added to binding reactions with various quantities of CsoR in binding buffer (10 mM Tris-Cl [pH 7.8], 50 mM KCl, 20 mM MgCl2, 5% glycerol, 20 μL total reaction volume). CsoR was incubated with promoter DNA for 20 min at room temperature. Reaction mixtures containing Cu2+ were performed as described above, except CuCl2 was incubated with CsoR for 10 min before adding DNA. All reaction solutions were loaded onto 5% acrylamide gel and electrophoresed at 150 V for 40 min in 0.5 × TBE buffer (45 mM Tris-Cl [pH 7.8], 45 mM borate, 1 mM EDTA). Gels were stained with ethidium bromide before being digitized using a scanner (Tanon 2500, China).
Bacterial chemotaxis assay
The chemotaxis ability of P. putida strains was assessed by using semisolid plate and µ-slide Chemotaxis plate (Ibidi 80326, Germany). For the method with semisolid plates, an agar plug (1% agar) containing 200 mM CuCl2 was placed in the center of a LB semisolid plate (0.25% agar) and left at room temperature for 12 h to achieve a CuCl2 gradient on the semisolid plate. An agar plug without CuCl2 was also placed in the center of a semisolid plate and used to test bacterial chemotaxis without copper. For the assay to investigate the effect of copper on bacterial chemotaxis, 200 μM CuCl2 (final concentration) was mixed with semisolid LB before making a semisolid plate. Overnight growth P. putida cells were washed and resuspended with fresh M9 medium and adjusted to the same optical density (OD600 = 0.5). Then, 2 μL of resuspended cultures was spotted 2 centimeters away from the agar plug/plate center, and the plate was incubated for 16 h (for the control plate) or 18 h (for the copper-containing plate) at 28 °C before digital photographs were taken. The distance from the point of inoculation to the edge of the colony growth closest to the agar plug (D1) and the distance from the point of inoculation to the edge of the colony growth farthest from the agar plug (D2) were measured. The response index (RI) value was calculated to characterize the bacterial response to CuCl2 as previously described29. The RI was calculated using the following equation: RI = D1/(D1 + D2). RI values greater than 0.52 and less than 0.48 correspond to attractant and repellent responses, and intermediate values represent nonresponses.
For the method with µ-slide Chemotaxis plate (a commercially available microfluidic device with a channel connecting two reservoirs), the reservoirs were filled with the two bacterial solutions (with or without CuCl2) following a modified version of the manufacturer’s “Fast Method” protocol. Briefly, overnight cultures were inoculated with M9 medium and grown at 28 °C, 180 rpm, until they reached an optical density (OD600) between 0.3 and 0.35. 1 ml of bacterial culture was washed twice with fresh M9 medium by centrifugation (3 min at 3000 rpm), and finally diluted to a target OD600 of 0.015 with fresh M9 supplemented with 0.01% Tween 20, with or without 2 mM CuCl2 for injection into the chemotaxis device. First, the entire device was overfilled with buffer free of CuCl2 or bacteria through the filling ports, and then the central channel’s ports were closed with plugs. About 65 µl was removed from one reservoir, replaced by 65 µl of CuCl2-free bacterial solution, and then this reservoir’s ports were closed. Finally, all liquid was removed from the other reservoir and replaced with a bacterial solution containing CuCl2. For control measurements, neither bacterial solution contained CuCl2. Phase contrast microscopy recordings were obtained at room temperature on a Nikon Ti-E inverted microscope using an sCMOS camera (PCO Edge 4.2) and a 40 x objective lens. Recordings were obtained starting from 20 min after filling the device. Three 15 s-long recordings of cells in the observation area were obtained at 15 fps. Then, single-cell tracking analysis was performed using ImageJ’s Manual Tracking and Chemotaxis Tool plugins.
Statistical analysis
Statistical analyses were performed using Graph-Pad Prism (version 9.0.0). Student’s t-test or an analysis of variance (ANOVA) was used to analyze the significance of differences in LacZ activity, fluorescence intensity, swimming zone diameter, gene expression, response index, center of mass, and velocity. A P value less than 0.05 was considered statistically significant.
Acknowledgements
This work was supported by the National Natural Science Foundation of China [42020104003 and 31900054] and the Fundamental Research Funds for the Central Universities [2662022SKQD002].
Competing interests
The authors declare no competing interests.
Data availability
Relevant data supporting the critical findings of this study are available within the article and the Supplementary Information file. The absorbance, microscopic photographs, gels, plates, and EMSA data generated in this study have been provided in the Source data file.
Supplementary Information
Fig. S1 Detect the interaction between CheA and the 40 proteins using BTH. CheA was cloned into T25a (a) and T18C (b). Blue indicates protein-protein interaction, and white indicates no interaction in the colony after 60 h of incubation. A colony containing T25a-zip and T18C-zip plasmids was used as a positive control (CK+), and a colony containing empty T25a and T18C plasmids was used as a negative control (CK-).
Fig. S2 Detect the interaction between CheA and indicated proteins using BiFC. Representative images for each pair of proteins were shown. Jun-KN151+Fos-LC151 and KN151+LC151 were used as CK+ and CK-, respectively. RFP channel images (fluorescent field), bright field images, and overlay images of the same field are shown. Scale bar = 2 μm.
Fig. S3 Growth curve of the 16 overexpression strains and wild-type strain in liquid LB broth (100 mL in a 250 mL triangular glass flask, at 28°C with 180 rpm shaking). The optical density at 600 nm (OD600) was used to characterize the growth of bacterial cells in the medium.
Fig. S4 Role of target proteins in the CheA-mediated transphosphorylation. (a) Transphosphorylation between CheA and the 14 proteins. Target proteins were added to the phosphorylated CheA and incubated for 10 s before adding termination buffer. CheY was added as a positive control. (b) ATPase activity of indicated proteins. The amount of remaining ATP after incubation with 10 μM indicated proteins for 30 min. BSA was used as a negative control. The asterisks represent statistically significant differences between FleQ and BSA (**P < 0.01). “ns.” represents no statistically significant between the indicated protein and BSA. (c) Effect of CsoR and PhaD on the transphosphorylation between CheA and CheY. The PT time in seconds (2 s and 10 s) represents the time of transphosphorylation. The bands of CheA, CheY, CsoR, and PhaD on the gel were indicated with arrows. The relative autoradiograph intensity of the CheA band was calculated using Image J software, shown below each lane.
Fig. S5 Role of the three conserved residues in the Cu2+-binding ability of CsoR. (a) P. putida CsoR and CsoR homologs of indicated bacterial species are aligned using an online ClustalW server (https://www.genome.jp/tools-bin/clustalw). The number above the sequence represents the amino acid order of S. saprophyticus CsoR. The identical residues are shown as white on red letters. Similar residues are shown in red in blue boxes. Asterisks indicated the three conserved residues involved in Cu2+-binding. The sequence identity of CsoR homologs to the P. putida CsoR was calculated. (b) MST analysis of the interaction between wild-type and mutated CsoRs and Cu2+. Wild-type/mutated CsoR (250 nM) was incubated with increasing concentrations of Cu2+. (c and d) Effect of point mutation on the binding of CsoR to copA-I promoter in the presence of Cu2+ in the EMSA assay. Free DNA and CsoR-DNA complex are indicated. (e) Detect the interaction between CheA and point-mutated CsoR using BTH. The LacZ activities of colonies are shown below. The result is the average of three independent assays. The data represent mean values with standard deviations. “ns.” represents none statistically significant between indicated strain and CK- strain analyzed by Student’s t-test.
Table S1 Target proteins identified in a pull-down assay. iBAQ_T (%) and iBAQ_CK (%) represent the percentage of certain proteins in experimental and control samples, respectively. The P values are for three technical replicates. Protein names and descriptions are based on the annotated genome as indicated at http://www.pseudomonas.com.
Table S2 Strains and plasmids used in this work.
Table S3 Primers used in this work.
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