A novel chlorination-induced ribonuclease YabJ from Staphylococcus aureus

The characteristic fold of a protein is the decisive factor for its biological function. However, small structural changes to amino acids can also affect their function, for example in the case of post-translational modification (PTM). Many different types of PTMs are known, but for some, including chlorination, studies elucidating their importance are limited. A recent study revealed that the YjgF/YER057c/UK114 family (YjgF family) member RidA from Escherichia coli shows chaperone activity after chlorination. Thus, to identify the functional and structural differences of RidA upon chlorination, we studied an RidA homolog from Staphylococcus aureus: YabJ. The overall structure of S. aureus YabJ was similar to other members of the YjgF family, showing deep pockets on its surface, and the residues composing the pockets were well conserved. S. aureus YabJ was highly stable after chlorination, and the chlorinated state is reversible by treatment with DTT. However, it shows no chaperone activity after chlorination. Instead, YabJ from S. aureus shows chlorination-induced ribonuclease activity, and the activity is diminished after subsequent reduction. Even though the yabJ genes from Staphylococcus and Bacillus are clustered with regulators that are expected to code nucleic acid-interacting proteins, the nucleic acid-related activity of bacterial RidA has not been identified before. From our study, we revealed the structure and function of S. aureus YabJ as a novel chlorination-activated ribonuclease. The present study will contribute to an in-depth understanding of chlorination as a PTM.


Introduction
Post-translational modification (PTM) is a biochemical process where amino acids of proteins are covalently modified after translation. PTMs are critical regulators of proteins' physiochemical properties, functions, and interactions with other proteins or nucleic acids. They are rapid, specific, and highly controlled modifications involved in cellular processes, such as enzyme activity, protein turnover, and protein localization [1]. More than 200 different types of PTMs have been identified, such as phosphorylation, glycosylation, ubiquitination, nitrosylation, methylation, acetylation, lipidation, and proteolysis [2]. Although PTMs play fundamental roles in the regulation of numerous pathways of cells, many types of PTMs still remain to be elucidated. Furthermore, various studies about different types of PTMs are reported each year, including chlorination [3]. Chlorination activates chaperone activity of Hsp33 through partial unfolding of its C-terminal redox-switch domain [4]. β-lactoglobulin, α-amylase, and BSA are other examples of proteins that gain chaperone activity after chlorination [5]. A recent study also revealed that Escherichia coli RidA from the YjgF/YER057c/UK114 family (YjgF family hereafter) exhibits chlorination-induced chaperone activity [5]. Given that chlorination can activate protein functions, it suggests that chlorination is an important PTM that is closely involved with cellular networks [6][7][8].
The YjgF family is divided into eight subfamilies according to NCBI Conserved Domain Database: RidA and Rid1-Rid7 (see cd00448: YjgF YER057c UK114 family). An organism may have RidA and other helices form links between two layers. The topology of SA YabJ is β1-β2-β3-α1-α2-β4-α3-β5-α4-β6. (B) The SA YabJ trimer is shown in a ribbon representation from top view. Chain A is colored in cyan, chain B is colored in magenta, and chain C is colored in gray. β-strands are packed in the center area and α-helices cover the surface area. (C) Potential surface charge of the crystal structure of SA YabJ, calculated with UCSF Chimera, where surfaces are colored between −10 kcal/mole (red) and +10 kcal/mole (blue) (1 kcal = 4.184 kJ). The one side of the hole is positively charged (from top view) and the other side is negatively charged (from bottom view). Three pockets of the surface are indicated as arrows. (D) Cross-section of SA YabJ. A 10Å-diameter hole is located in the middle and the deep pocket of one monomer is shown.
Rid family proteins [9]. Several crystal structures of YjgF family members have been solved, showing common features. Most are ball-like trimers with a hole in the center, formed by β-strands, with one pocket on each monomer, formed by loops. The six footprint residues (Tyr 17 , Ser 30 , Asn 88 , Arg 105 , Cys 107 , and Glu 120 in E. coli RidA) are positioned in the pocket on each monomer and are used as a position-specific scoring matrix to differentiate the Rid subfamilies. These six footprint residues are expected to be functional sites. For example, the Rid4-Rid7 subfamilies, which lack Arg 105 , do not show any deaminase activity. Almost all other subfamily members have deaminase activity that removes reactive enamine/imine intermediates during branched chain amino acid biosynthesis pathways and accelerates the release of ammonia [10,11]. Therefore, the family was recently suggested to be renamed Rid (reactive intermediate/imine deaminase). The typical RidA subfamily members are found in diverse organisms, such as Bacillus subtilis (YabJ), Drosophila melanogaster (DUK114), and Rattus norvegicus (L-PSP). Besides deamination, other functions of the RidA subfamily include maintenance of the mitochondrial genome (Saccharomyces cerevisiae, YER057C), translation inhibition (human hp14.5), and chaperone activity (E. coli RidA and D. melanogaster DUK114) [9,12].
Gene clustering in prokaryotes indicates a functional relationship, and bacterial RidA subfamily genes are usually clustered with pyrimidine or arginine metabolism genes [13]. Unlike other bacterial RidA subfamily member genes, those from Bacillus and Staphylococcus species show unique genetic profiles [14]. The gene encoding RidA in Bacillus and Staphylococcus is clustered with spoVG, forming the yabJ-spoVG bicistronic operon. In Bacillus and Staphylococcus species, RidA is encoded from the gene yabJ; therefore, the RidA proteins encoded by these genes are subsequently termed YabJ ( BS YabJ and SA YabJ hereafter). yabJ and spoVG transcription depends heavily on σ B , a large regulon of genes involved in many different cellular processes [15]. Although σ B controls the expression of multiple genes, including virulence factors, gene regulators, and antibiotic resistance, the σ B promoter is not directly responsible for this regulation. Rather, σ B -dependent regulation is controlled by downstream regulatory elements such as the yabJ-spoVG operon. Indeed, inactivation of the Staphylococcus yabJ-spoVG operon causes a reduction in nuclease, protease and lipase activity, and resistance to antibiotics [16,17]. The two proteins encoded from the bicistronic operon are expected to work as regulators by interacting with nucleic acids. Even though BS YabJ represses the function of purR, which encodes adenylosuccinate synthetase, the mechanism has not yet been revealed [18].
Here, we elucidated the crystal structure of SA YabJ from Staphylococcus aureus Mu50 and its function as a ribonuclease after chlorination. Because yabJ is clustered with another DNA-binding protein gene in the yabJ-spoVG operon, and using the domain prediction for YabJ in the UniProtKB database, SA YabJ is predicted to have a nuclease function. Although the structures of many RidA homologs are solved, only L-PSP has shown ribonuclease activity [19]. The hp14.5 has translation inhibition activity, although the mechanism is still unclear [20]. Considering that mammalian RidA homologs primarily show nucleic acid-related activity amongst many homologs and liver perchloric acid extracted L-PSP and trichloroacetic acid extracted hp14.5 show higher activity than recombinant L-PSP and hp14.5, YabJ is predicted to go through chlorination as a PTM. To gain further insight into the function of SA YabJ, we verified whether chlorination was possible and ribonuclease activity assays were conducted. Chlorination was reversible with a reducing agent, and SA YabJ shows ribonuclease activity after chlorination and loses activity when reduced. In addition, we identified important residues for the ribonuclease activity by site-directed mutagenesis. The present study presents a ribonuclease that is activated following chlorination and the novel discovery of the nuclease function of YabJ. Our structural and functional research regarding chlorination of SA YabJ will promote a better understanding of this type of PTM.

Cloning, expression, and purification
An expression plasmid for SAV0497 (yabJ) from S. aureus Mu50 was constructed using ligation-independent cloning (LIC) as previously described [21][22][23]. The resulting construct has 17 additional residues (MHHHHHHENLYFQ-GAAS) that encode an N-terminal hexa-histidine tag, TEV cleavage site, and GAAS residues for LIC cloning. To prepare mutants (C103A, pocket-forming sites mutant: Y16H18K39R101C103K111A), the EZchange Site-directed Mutagenesis kit (Enzynomics, Korea) was used. The sequences of the cloned genes were confirmed by DNA sequencing (results not shown). The recombinant plasmids were transformed into E. coli BL21 (DE3). Cells were grown at 37 • C in LB medium supplemented with ampicillin (50 μg/ml) until the OD 600 reached 0.5. Recombinant protein expression was induced by the addition of IPTG to 0.5 mM, and the cells were allowed to grow for an additional 4 h at 37 • C. The cells were harvested by centrifuging at 4500 g at 4 • C. For each protein, cell pellet was resuspended in lysis buffer (50 mM Tris/HCl, pH 7.5, and 500 mM NaCl) and disrupted using an Ultrasonic processor (Cole-Parmer, U.S.A.) at 4 • C. The cell lysate was centrifuged at 20000 g for 1 h at 4 • C. The cleared supernatant was purified by binding to an Ni-NTA (Ni 2+ -nitrilotriacetate) affinity column (Qiagen, Germany; 3 ml of resin per liter of cell lysate) and eluted with binding buffer containing 200 mM imidazole. Further purification and buffer exchange were achieved by size-exclusion chromatography using a Superdex 75 (10/300 GL) column (GE Healthcare Life Sciences, U.S.A.) that was previously equilibrated with 50 mM Tris/HCl, pH 7.5, and 200 mM NaCl. The purity of recombinant SA YabJ was estimated to be over 95% by SDS/PAGE. The purified SA YabJ was concentrated to 10 mg/ml by ultrafiltration in 10000 Da molecular-mass cut-off spin columns (Millipore, U.S.A.). The absorbance at 280 nm was measured, and Sequence alignment of SA YabJ with YabJ from B. subtilis (59% sequence identity), Mmf1 from S. cerevisiae (42% sequence identity), RidA from E. coli (50% sequence identity), L-PSP from rat (38% sequence identity), and hp14.5 from human (42% sequence identity). Identical residues are colored white on a red background and similar residues are red on a white background. Secondary-structure elements (springs, α-helices; arrows, β-strands) are represented above and the sequences are numbered. The six footprint residues are marked as (#). The residues enclosed with black boxes in L-PSP and hp14.5 are expected to go through PTM and additionally marked as (᭡). The figure was constructed using ESPript (http://espript.ibcp.fr) [73].  Crystallization, X-ray data collection, and structure determination Crystals of SA YabJ were grown by the hanging-drop vapor diffusion method at 293 K using 24-well VDX plates (Hampton Research, U.S.A.). Initial crystallization conditions were established using screening kits from Hampton Research (Crystal Screens I and II, Index, PEG/Ion, and MembFac) and from Emerald BioSystems (Wizard I, II, III, and IV). For the optimal growth of the SA YabJ crystals, each hanging drop was prepared on a siliconized coverslip by mixing 1 μl of 10 mg/ml protein solution and 1 μl of precipitant solution (25% (w/v) PEG3350 and 100 mM Tris/HCl, pH 8.5) and this drop was equilibrated against a 1-ml reservoir of precipitant solution. The condition yielded needle-shaped crystals that grew to dimensions of 1.2 mm × 0.4 mm × 0.4 mm in 10 days. For crystal freezing, the crystals were transferred to a cryoprotectant solution with 30% glycerol in the crystallization conditions for several minutes before being flash frozen in a stream of nitrogen gas at 100 K. Diffraction data were collected on ADSC Quantum 315r CCD detector system (Area Detector Systems Corporation, U.S.A.) at the BL-5C experimental station of the Pohang Light Source, Korea. The crystal was rotated by 1 • for each image, and the raw data were processed and scaled using the program suite HKL2000 [24]. Further data analysis was carried out using the CCP4 suite [25]. The crystal belonged to space group P2 1 and contained six molecules per asymmetric unit. Data collection statistics are summarized in Table 1.
To determine the structure of SA YabJ, molecular replacement was used with the program MolRep within the CCP4 suite using the structure of homolog YabJ from B. subtilis (PDB code: 1QD9) as a search model [26]. The sequence identity of the two proteins is 59%. Refinement of the crystal structure was done through iterative cycles of model building using COOT, followed by refinement of the models with Refmac5 and phenix.refine [27][28][29][30][31][32]. A 5% portion of the data was set aside before the refinement for the R free calculations [33]. Solvent molecules became apparent in the later stages of refinement. Refinement was pursued until no further decrease in R free was observed. The final models exhibited good stereochemical geometry when the overall geometry was validated with PROCHECK [34]. Refinement statistics are summarized in Table 1. Structural alignments were carried out using the program PyMOL (http://www.pymol.org) and USCF chimera (http://www.cgl.ucsf.edu/chimera), which were then used for the construction and generation of all figures [35]. Protein interfaces, surfaces, and assemblies were calculated using the PISA server at the European Bioinformatics Institute (http://www.ebi.ac.uk/pdbe/prot int/pistart.html) [36].

Protein chlorination and oxidation
Hypochlorous acid (HOCl) was prepared from sodium hypochlorite (NaOCl) (Sigma, U.S.A.). Ten percent of the NaOCl solution was diluted to 200 mM in 50 mM Tris/HCl, pH 7.5. For complete chlorination of SA YabJ, 1 mM SA YabJ was incubated for 30 min at room temperature in HOCl with a molar ratio of SA YabJ:HOCl of 1:10. After treatment, excess HOCl was removed by extensive dialysis with 50 mM Tris/HCl, pH 7.5. The control solution consisted of the same SA YabJ with a buffer, which was incubated under the same conditions. The chlorinated SA YabJ (1 mM) was processed with 10 mM DTT to reduce the chlorinated state. Subsequently, DTT was removed by extensive dialysis with 50 mM Tris/HCl, pH 7.5.
For complete oxidation of SA YabJ, 1 mM SA YabJ was incubated for 30 min at room temperature in H 2 O 2 (Sigma, U.S.A.) with a molar ratio of SA YabJ:H 2 O 2 of 1:10. Excess H 2 O 2 was removed by extensive dialysis with 50 mM Tris/HCl, pH 7.5. The chlorination and oxidation state of SA YabJ was determined by MS and native PAGE.

PAGE
SDS/PAGE was conducted according to the Laemmli method using a 12% (w/v) polyacrylamide gel [37]. The samples were treated with 1% (w/v) SDS and 5% (v/v) 2-mercaptoethanol at 100 • C for 5 min before electrophoresis in a vertical Mini Gel system (Bio-Rad, U.S.A.). The proteins were stained with Coomassie Brilliant Blue R250 (Thermo Scientific, U.S.A.). Additionally, for the separation of native SA YabJ, native PAGE was performed and analysis was conducted using 12% (w/v) polyacrylamide gel without either SDS or 2-mercaptoethanol. Native PAGE was performed in 25 mM Tris/HCl, pH 8.3, and 192 mM glycine. The staining was performed as for SDS/PAGE.

Mass spectroscopy
Mass analysis was performed on a nano-HPLC system (Dionex Ultimate 3000 RSLCnano System, Thermo Scientific, U.S.A.) coupled with a hybrid quadrupole-orbitrap mass spectrometer (Q-Exactive, Thermo Scientific, U.S.A.) at the National Instrumentation Center for Environmental Management (NICEM, Seoul National University, Korea). Protein samples (10 μl) were loaded on to a C 8 reverse-phase column (INNO5, Young Jin Biochrom, Korea). A room temperature gradient from 0.1% formic acid in water (solvent A) to 0.1% formic acid in acetonitrile (solvent B) was used for HPLC. The total run time for each sample was 20 min. The molecular mass of the protein was generated from several multiply charged peaks using the Xcalibur 2.2 software (Thermo Scientific, U.S.A.).

CD
CD spectra were collected using a Chirascan series spectrometer equipped with a temperature controller (Applied Photophysics, U.K.) [38]. The protein samples were prepared in 50 mM Tris/HCl, pH 7.5 and 200 mM NaCl. The CD spectra were recorded with a step size of 1.0 nm, a bandwidth of 1 nm, and an averaging time of 2 s. Measurements were performed in a 1-mm path length quartz SUPRASIL cell (Hellma, Germany) using 10 μM concentration of SA YabJ at room temperature. Three scans were applied continuously and the data were averaged. The CD spectra were smoothed and processed after blank subtraction using Pro-Data Viewer software (Applied Photophysics, U.K.). The change in molar ellipticity [θ] was calculated using the following equation, where θ is in millidegrees, path length (l) is in millimeters, and C is the molar concentration of protein:

Chaperone activity assay
To monitor the chaperone activity, citrate synthase was employed as a substrate [39,40]. Initially, to identify foldase chaperone activity, 75 μg of citrate synthase (Sigma, U.S.A.) was mixed with a solution of 100 mM Tris/HCl, pH 8.0, 20 mM DTT, and 6 M guanidinium chloride. The citrate synthase mixture (75 μg of citrate synthase, 100 mM Tris/HCl, Mass spectroscopy of native and chemical-treated SA YabJ in the same order as (A). A major peak was observed at 16008 Da in native SA YabJ spectrum, corresponding to the calculated mass of SA YabJ. After the treatment of HOCl, a major peak was observed at 16332 Da, in addition to multiple peaks with ∼35.45 Da intervals, indicating discreet additions of chloride ions. Another set of peaks with ∼35.45 Da intervals is observed, implying simultaneous oxidation and chlorination occurs. Two main peaks with an approximate 16 Da mass difference appear when the HOCl-treated SA YabJ is reduced, indicating most chlorinated residues are reduced but some oxidized residues are not reduced. A similar spectrum is observed for H 2 O 2 -treated SA YabJ. pH 8.0, 6 M guanidinium chloride, and 20 mM DTT) was incubated for 1 h at 25 • C; consequently, the citrate synthase in this solution was denatured. After incubation, refolding of citrate synthase was achieved by 100-fold dilution with a solution of 100 mM Tris/HCl, pH 8.0 containing 5 μM SA YabJ. Hsp31 from S. aureus was used for positive control and buffer containing citrate synthase was used for negative control [41]. The diluted solution was mixed with 100 mM Tris/HCl, pH 8.0, 1 mM DTNB (5,5 -dithiobis [2-nitrobenzoic acid]), 0.2 mM MnCl 2 , 0.4 mM oxaloacetic acid, and 0.3 mM acetyl-CoA to detect the activity of citrate synthase. After mixing, only the active refolded enzyme could catalyze the breakdown of acetyl-CoA into the acetyl group and CoA. The CoA reacts with DTNB, which acts as a coloring agent, and this produces a yellow TNB (5-thio-2-nitrobenzoic acid)-CoASH compound that is detectable at 412 nm using a Multi-Mode microplate reader (SpectraMax M5e, Molecular Devices, U.S.A.) [42].
An aggregation prevention assay for chaperone activity was performed using citrate synthase mentioned above. Citrate synthase (30 μM) (Sigma, U.S.A.) was denatured in 4.5 M guanidinium chloride, 50 mM Tris/HCl, pH 7.5 at room temperature overnight. A total of 0.3 μM citrate synthase aggregation was monitored in 50 mM Tris buffer (pH 7.5) containing 5 μM SA YabJ at 30 • C. Hsp31 from S. aureus was used as a positive control. The emission and excitation wavelengths were set at 360 nm [5].

Ribonuclease activity assay
Purified, recombinant SA YabJ was incubated at 37 • C for 30 min with the nucleic acid substrates: dsDNA, ssDNA, and ssRNA. Nucleic acid substrates (30 μM) were mixed with 0, 30, 60, and 120 μM SA YabJ in 50 mM Tris/HCl, pH 7.5 and 150 mM NaCl to a final volume of 5 μl. The total solutions were loaded on to 0.8% agarose gels in TBE buffer, and the results were visualized using a Gel Doc (Bio-Rad, U.S.A.). The nucleic acid used in the present study was an expected promoter of the spoVG gene of the yabJ-spoVG operon. In detail, oligomers used for the agarose gel assay were AATAAAACAGAGAGATATATACTATAGGG (29 nts) as ssDNA, dsDNA for the same sequence, and AAUAAAACAGAGAGAUAUAUACUAUAGGG (29 nts) as ssRNA [43].
The ribonuclease activity assay was complemented by a fluorescence assay using the RNase Alert assay kit (IDT, U.S.A.) [44,45]. A fluorophore is covalently linked to one end and a quencher on the other end of a synthetic RNA. When a ribonuclease cleaves the synthetic RNA of a fluorophore-quencher pair, the separated fluorophore emits green fluorescence at 520 nm following excitation at 490 nm. SA YabJ and mutants (C103A and pocket-forming sites mutant) were incubated at 37 • C with the substrate (50 pmol) in 20 mM Tris/HCl, pH 7.0 and RNaseAlert buffer for 30 min. The resulting fluorescence (RFU) was monitored in a continuous assay format using a Multi-Mode microplate reader (SpectraMax M5e, Molecular Devices, U.S.A.).
The crystal structure reveals that SA YabJ exists as a compact homotrimer, which is consistent with the results of size-exclusion chromatography (Figures 1B and 3A). The ball-like trimeric structure forms a hole in the center area with a diameter of approximately 10Å, with ∼20 water molecules positioned in the interior. The interface buries ∼988Å 2 of surface per subunit (13.7% of the subunit surface). The β-strands (β2-β6) form a central barrel with a hollow center that does not completely permeate the protein, and all α-helices are located around the perimeter, solvent exposed ( Figure 1B). On its trimeric interface, there are numerous residues that contribute hydrogen bonds between the subunits, including Ser 18 , Thr 21  The surface electrostatic potential map shows that positively charged residues predominate at the entry of the center cavity, and negatively charged residues are dominant on the opposite side. Two highly conserved glutamate residues, Glu 116 and Glu 118 , are responsible for this negative charge. Each monomer has a deep pocket on its surface. In the trimeric structure, the depth of each pocket is limited by the β5 strand of the adjacent monomer ( Figure 1C,D).

Structural comparison of S. aureus YabJ with other proteins
The overall fold of SA YabJ shows high structural similarity to other members of the YjgF family [46][47][48][49][50][51]. SA YabJ is classified as a member of the typical RidA subfamily by sequence analysis, and all six footprint residues (Tyr 16 , Ser 29 , Asn 87 , Arg 101 , Cys 103 , and Glu 116 ) are conserved. The absolutely conserved arginine (Arg 101 in SA YabJ) in RidA and Rid1-Rid3 subfamilies has proven to be crucial for the catalysis of imine hydrolysis subfamilies. This arginine is not conserved in the members of Rid4-Rid7 subfamilies, and imine hydrolysis is not catalyzed by these proteins [9]. In the crystal structure of SA YabJ, all six footprint residues are positioned toward the deep pocket on the surface, where they are known to be involved in ligand binding (Figure 2). In the co-crystal structures of 2-oxobutanoate-bound E. coli TdcF and pyruvate-bound Arabidopsis thaliana RidA, ligands are co-ordinated in these pockets, interacting with arginine, cysteine, serine, and glutamate residues [52,53].
The SA YabJ structure was submitted to the DALI server (http://ekhinda.biocenter.helsinki.fi/dali server) to obtain structural homologs [54]. Since only mammalian RidA proteins are known to show nucleic acid-related activity, the structure is compared with mammalian L-PSP from rat and hp14.5 from human. For L-PSP from rat, one serine residue (Ser 2 ), three lysine residues (Lys 13 , Lys 60 , and Lys 67 ), and one threonine residue (Thr 74 ) are expected to have PTMs, as acetylation, succinylation, and phosphorylation, respectively [55][56][57]. These five residues are all surface exposed and conserved in human hp14.5. Additionally, one of the six footprint residues, Cys 103 in SA YabJ is replaced by alanine in both mammalian RidA proteins. This indicates that bacterial and mammalian RidA may perform different functions ( Figure  2). At present, many structures from the YjgF family have been solved and most of them share the tightly packed trimeric structure mediated through the β-strands of each monomer. Despite the conserved quaternary structures throughout the YjgF family, several disparate metabolic functions are revealed. Therefore, detailed structural insights would produce significant contributions to our understanding of the biological functions of the YjgF family proteins.

Chlorination of S. aureus YabJ
Proteins of the YjgF family are mostly highly acid-stable, evidenced by L-PSP and hp14.5, members of the RidA subfamily [49]. These proteins are prepared as soluble proteins in perchloric acid-treated rat liver and trichloroacetic acid extracts from human mononuclear phagocyte (MNP), respectively [19,20,57]. They both inhibit protein synthesis and L-PSP is also a ribonuclease. Interestingly, acid-extracted, native L-PSP, and hp14.5 show higher activity compared with their recombinant counterparts [20,58]. E. coli RidA shows chaperone activity after incubation with HOCl [5]. These previous studies show that chlorination plays a role in the physiology of RidA subfamily proteins. Protein chlorination causes alterations in protein structure via side chain or peptide bond amino group modification, and a corresponding functional change follows in several cases [59][60][61]. As other members of the RidA subfamily show high stability in acidic solution and chlorination, SA YabJ is predicted to be stable during chlorination. To study whether SA YabJ shows any functional changes upon chlorination, like E. coli RidA, chlorination of SA YabJ was performed.
The chlorination state in solution is monitored by size-exclusion chromatography, PAGE, and mass spectroscopy. A single, intense peak with a molecular mass of ∼50 kDa in size-exclusion chromatography indicates the presence of homogeneous SA YabJ trimer. Native PAGE shows a single band, although SDS/PAGE separates SA YabJ into two bands at 50 and 16 kDa, indicating trimer and monomer. Because the chemical detergent SDS affects protein oligomeric state, trimeric structure is dissociated during SDS/PAGE. After 30 min of chlorination at room temperature, a single peak splits and broadens in size-exclusion chromatography. This result corroborates the native PAGE, which shows a thick, spread band. SDS/PAGE indicates only one band at the monomer position. The chlorination propensity of SA YabJ was reversible. When the chlorinated SA YabJ is reduced with 10 mM DTT, the same result as native SA YabJ is observed. This chlorinated and reduced SA YabJ recovers a single intense peak in size-exclusion chromatography, trimeric conformation in SDS/PAGE, and the spread band on native PAGE becomes condensed. To discriminate the effects of chlorination from oxidation, the same experiment was conducted on oxidized SA YabJ. A single peak is  mM Tris/HCl pH 8.0). The buffer with citrate synthase (ᮀ) contained additional 0.75 μg of denatured citrate synthase. Hsp31 (᭹) was used for the chaperone reference [41]. No chaperone activity was observed with SA YabJ before (᭺) and after (᭡) chlorination. (B) Aggregation prevention assay. Aggregation of citrate synthase was measured by light scattering at 30 • C. The citrate synthase was observed alone in a buffer (ᮀ), or mixed with 5 μM SA YabJ before (᭺) and after (᭡) chlorination. Hsp31 that was used for the positive control (᭹) inhibits aggregation. Values are the mean of three separate determinations.
observed from size-exclusion chromatography and PAGE shows a similar result to SA YabJ or chlorinated and reduced SA YabJ ( Figure 3A). The chlorination state was also identified using mass spectroscopy. Based on the calculated mass of recombinant SA YabJ of 16008.9 Da, a single peak at 16008 Da corresponds to native SA YabJ. On the other hand, after chlorination, the major peak is shifted to the right, indicating that several amino acids of SA YabJ are covalently modified. Oxidation occurs simultaneously during chlorination with HClO, and a number of peaks appeared in the mass spectrum. The major peaks show intervals of ∼35.45 Da, which correspond to the addition of multiple chlorine atoms. After reduction in chlorinated SA YabJ, chlorinated residues are reduced but oxidized residues remain. Mass spectra of chlorinated and reduced SA YabJ and oxidized SA YabJ are similar, indicating two main peaks with a mass difference of ∼16 Da ( Figure 3B).

Chaperone activity was not observed in S. aureus YabJ
Chaperones are a functionally related group of proteins that assist in protein folding. Depending on the molecular weight, chaperones are classified into subfamilies. When the molecular weight is 34 kDa or less, they are called small heat shock proteins (sHSP) [62]. sHSP are often predicted to undergo dynamic assembly into oligomers, and perform chaperone activities by interacting with substrates [63]. Regulation is essential for ensuring proper physiological activity of these chaperones, and structural changes due to PTM are crucial for controlling their interactions with target proteins [64]. For example, Hsp33 undergoes structural rearrangement and is activated as a chaperone after exposure of HOCl [4]. A 20-kDa DJ-1 exhibits enhanced activity toward α-synuclein when its cysteine is oxidized to Cys-SO 2 H [65]. From our previous study, the 18-kDa SAV1875 lost its chaperone activity after its cysteine was fully oxidized from Cys-SO 2 H to Cys-SO 3 H [66]. Also, E. coli RidA shows chlorination-induced aggregation prevention chaperone activity [5]. Since SA YabJ is defined as a member of the RidA subfamily, displaying similar structural characteristics, chaperone activity was expected by chlorination in the same manner as E. coli RidA. However, both native and chlorinated SA YabJ do not show chaperone function in respects of the foldase activity or aggregation prevention activity ( Figure 4). This result is surprising, considering the high degree of sequence and structural similarity between SA YabJ and E. coli RidA; both sharing 50% homology, comprising trimeric structures with an RMSD value of 1.1Å, and displaying similar surface structures and charge distributions. Size-exclusion chromatography predicts E. coli RidA to be multimerized after the chlorination, but SA YabJ does not seem to form any higher oligomer ( Figure 3A). Although the trimeric structure is supposed to be dissociated, SA YabJ was highly stable after chlorination. In addition, CD revealed that the secondary structure of dominant α-helices is well preserved after chlorination ( Figure 5). Therefore, trimeric structure or higher oligomeric state might be the requisite to the chaperone activity of RidA subfamily proteins.

Ribonuclease activity of S. aureus YabJ
The overall fold and trimeric structure of SA YabJ are well conserved throughout YjgF family members. However, the gene distribution of yabJ in Staphylococcus and Bacillus species is unusual [16]. Only Staphylococcus and Bacillus species have the yabJ-spoVG operon that encodes YjgF family protein YabJ and multifunctional protein SpoVG. The inactivation of the yabJ-spoVG operon produces strong attenuation of nuclease, protease, and lipase function. The regulation of this operon is mainly associated with SpoVG rather than YabJ, and the strong-binding affinity of SpoVG and nucleic acids is verified [14,16]. Although there are known functions of BS YabJ, including deamination and repression of purA transcription, detailed studies on the function of YabJ with regard to nucleic acids are limited [18]. From the gene clustering information, previous functional studies, and nucleic acid-related studies with L-PSP and hp14.5, SA YabJ is predicted to have ribonuclease activity. However, native SA YabJ did not cleave any nucleic acid. Since L-PSP from perchloric acid-treated rat liver reveals four times higher ribonuclease activity compared with recombinant L-PSP and hp14.5 extracted from trichloroacetic acid shows higher protein synthesis inhibition activity than the recombinant hp14.5, chlorination is speculated to affect the interaction with nucleic acids [19,20].
Chlorinated SA YabJ was tested for ribonuclease activity. On gel electrophoresis, chlorinated SA YabJ displays the highest cleavage activity against ssRNA molecules and weak activity on ssDNA. However, chlorinated SA YabJ does not cleave dsDNA. The specificity on ssRNA corresponds previous observations in mammalian RidA proteins [19]. Native SA YabJ does not show nuclease activity toward any type of nucleic acid ( Figure 6A). As chlorination is reversible, ribonuclease activity of chlorinated SA YabJ decreases after reduction. SA YabJ that was reduced by DTT after chlorination was no longer able to degrade ssRNA on gel electrophoresis (data not shown). The fluorescence-quenching assay using random RNA corroborates the results of gel electrophoresis. Chlorinated SA YabJ showed a significantly higher initial rate of RNA cleavage compared with native or oxidized SA YabJ. DTT-reduction after chlorination subsequently reduced this gain in activity of SA YabJ, showing that chlorination, not oxidation, is essential for the ribonuclease activity of SA YabJ ( Figure 6B).

Structural insights into the interactions of chlorinated S. aureus YabJ with nucleic acids
Although SA YabJ shows an uncertain oligomeric state after chlorination, chlorinated SA YabJ was highly stable at high concentrations at room temperature. Although CD also revealed that the secondary structure was maintained, the protein did not crystallize after chlorination. Since ribonuclease activity is not observed in most RidA family proteins, there is a lack of studies that have focussed the ribonuclease function and structure relationship of RidA. A notable feature in the RidA monomer structure is a groove that forms a pocket when it becomes a trimer. The diameter of this groove is ∼20Å, which is a sufficient distance to accommodate nucleic acids. The surface electrostatic potential distribution of the groove shows a positively charged surface patch comprising Lys 78 , Lys 111 , and Arg 108 . The SA YabJ monomer structure implies possible interactions with nucleic acids physically and chemically.
The possible binding pocket of nucleic acids is detectable from the native SA YabJ crystal structure. To identify the location of the pocket, the SA YabJ structure was submitted to MetaPocket 2.0 (http://projects.biotec.tu-dresden.de/ metapocket/) [67,68]. Four putative pockets are detected, including the hole in the center area and the pocket on each monomer's surface ( Figure 7A). Ligand-bound crystal structures of other YjgF family members, E. coli TdcF, A. thaliana RidA, and human hp14.5, show that ligands are found in the pocket on the monomer's surface [52,53]. These studies suggest that the pocket on the monomer could be the SA YabJ binding site for nucleic acids.
Amino acids that can be easily modified after HOCl treatment are sulphur-containing cysteine and methionine, or amide-containing arginine, histidine, and lysine. In addition, other residues, such as tyrosine and tryptophan, are known to become chlorinated [69,70]. For example, tyrosine is chlorinated to 3-chlorotyrosine and chlorination of lysine can form monochloramines or dichloramines [69,71,72]. Lys 72 , Asn 81 , and Lys 122 interact with adjacent subunit residues (Glu 118 , Arg 108 , and Asn 23 , respectively) through charge-charge interaction on the trimeric interface ( Figure 7B). When SA YabJ is chlorinated, these residues might be affected by chlorination and the trimeric state would be destabilized. Residues Tyr 16 , His 18 , Lys 39 , Arg 101 , Cys 103 , and Lys 111 are in the flexible loop region and responsible for pocket formation. These residues are protruded toward the pocket and may be responsible for the altered characteristics following chlorination ( Figure 7C). To study the effect of these residues, we performed an additional ribonuclease activity assay using chlorinated C103A SA YabJ mutant and chlorinated pocket-forming sites mutant (Y16H18K39R101C103K111A). The fluorescence intensity was reduced in C103A SA YabJ, indicating Cys 103 performs an important role. The pocket-forming sites mutant lost ribonuclease activity ( Figure 7D). On the basis of the study, we suggest that residues around monomer pocket are important for chlorinated SA YabJ performing ribonuclease activity.

Discussion
Bacterial cells are prone to be exposed to a chlorinating milieu. Not only from household bleach, HOCl is produced during a host's phagocytic immune reaction, mainly from macrophages and neutrophils. HOCl is a highly reactive component, reacting with multiple chemical entities, such as proteins and fatty acids, and lead to suppression of DNA synthesis [6][7][8]71]. However, successful pathogens resist the host cellular defense as a function of structural or biochemical properties. Some proteins are modified and retained/converted their function under chlorination. For example, Hsp33, RidA, and DUK114 gain chaperone activity upon chlorination. Even though chlorination plays one of the most important roles in microbial killing, little is known about chlorination and bacterial response [4,5,12].
In the present study, we elucidate the structure and chlorination-related function of SA YabJ as a member of the YjgF family. The crystal structure of SA YabJ shows a homologous fold and trimeric structure, which are the pertinent traits of the YjgF family. Each monomer has a deep pocket on their surface, and there is a hole at the trimeric center. The presence of trimeric structure, pockets, and central hole are well conserved in other members of the YjgF family. The six footprint residues, which are used to differentiate YjgF subfamilies, are on a hole and pockets, implying the importance of structural features. Specifically, the amino acid composition of the pockets and hole structure of SA YabJ are similar to those of YabJ from B. subtilis. In addition, SA YabJ and BS YabJ share the same genetic array: the yabJ-spoVG gene cluster, which suggests that they might perform the same function. However, functional studies of BS YabJ are limited to deamination and inhibition of purA transcription.
We first identified SA YabJ as a ribonuclease that is activated after chlorination. Native SA YabJ did not show any ribonucleolytic activity. After chlorination, SA YabJ digests ssRNA efficiently, and also cleaves ssDNA to a lesser extent, but loses the activity when reduced. The loss of activity is due to the reduction in chlorinated SA YabJ as the difference was confirmed by size-exclusion chromatography and SDS/Native PAGE. In addition, we revealed that this gain of ribonuclease activity is specifically due to chlorination, not oxidation. This finding matches the fact that native L-PSP and hp14.5 show higher activity compared with recombinant proteins. The native L-PSP and hp14.5 were extracted using perchloric acid and trichloroacetic acid, respectively; conditions that permit chlorination of the proteins. Recombinant L-PSP and hp14.5 were, however, expressed in E. coli, and purified in buffers where chlorination was less likely.
This raises the question of exactly what modifications lead to SA YabJ gaining ribonucleolytic activity following chlorination. Mass spectroscopy shows an increase in more than 300 Da after chlorination, indicating that ∼11 amino acids can be affected from the protein's 126 amino residues. The result illustrates that chlorination and oxidation occur concurrently and various residues are influenced besides the sulphur-containing residues, methionine, and cysteine, as there are only four of these in total. From the mutants study, we have shown that Tyr 16 , His 18 , Lys 39 , Arg 101 , Cys 103 , and Lys 111 , which are predicted as the potential nucleic acid binding groove, are important for the chlorinated SA YabJ performing ribonuclease activity. Further investigation into the chlorination and activation of YabJ would further our understanding of the fundamentals of the chlorination PTM. In addition, the present study has led to the novel discovery of the chlorination-induced ribonuclease function of YabJ.

Accession number
Protein co-ordinate and structure factor have been deposited in the RCSB PDB under code 5YU2.