Introduction

Sulfane sulfur is a chemical state of the sulfur atom with six valence electrons that are covalently bound to sulfur atoms (1, 2). Growing evidence supports the widespread existence of hydropersulfidated and polysulfidated proteins in all cell types, referred to as sulfane sulfur-binding proteins (SSBPs) (3). Protein sulfuration occurs via post-translational and co-translational pathways. Rhodanese is known to catalyze the production of sulfane sulfur and attach it to the thiol group of the protein itself using thiosulfate as a substrate (4). 3-Mercaptopyruvate sulfurtransferase is a rhodanese-like enzyme that uses 3-mercaptopyruvate as the preferred sulfur donor (5). Cystathionine β-synthase and cystathionine γ-lyase use cystine as a substrate and catalyze the production of sulfane sulfur-containing cysteine hydropersulfide (CysSSH)(6), whose terminal sulfane sulfur can be reversibly transferred to other thiols such as glutathione (GSH) or protein-SH to form GSH hydropersulfide (GSSH) or protein hydropersulfides (protein-SSH), respectively (7). Cysteinyl-tRNA synthetase 2 catalyzes the production of CysSSH from CysSH (8), thereby producing CysSSH-integrated nascent proteins. The biological function of sulfane sulfur has received considerable attention in redox biology because of its antioxidant/anti-electrophilic capacity. However, the role of sulfane sulfur in proteins is not fully understood; therefore, further mechanistic investigation is required. Although several SSBPs have been identified using various methods (6, 9), in the present study we used β-(4-hydroxyphenyl)ethyl iodoacetamide (HPE-IAM) (8) to derivatize the sulfane sulfur because we herein found that HPE-IAM has ability to extract sulfane sulfur atoms from SSBPs to form bis-S-HPE-AM adduct at a certain condition, thereby enabling quantitative analysis using LC-MS/MS with a stable isotope-labeled standard, bis-S34-HPE-AM.

In biological systems, cysteine-rich proteins can act as “redox switches” which sense accumulated oxidative stressors and free zinc ions, store excess metals, control the activity of metalloproteins, and serve as triggers for the activation of cellular redox signaling cascades (10). Metallothionein (MT), discovered in 1957 (11), is an important cysteine-rich metal-binding protein involved in three major biological processes: homeostasis of essential metals, detoxification of toxic metals, and protection from oxidative stress (12, 13). It is recognized that metal binding to MT is thermodynamically stable, but oxidation of the thiolate cluster readily leads to metal release and formation of intramolecular MT-disulfide linkages. Zinc ions released from zinc/thiolate clusters of MT are suggested to function as signaling molecules for cellular redox homeostasis (14). Simultaneously, reduction of MT-disulfide by cellular reducing agents can occur in a process called the “MT redox cycle” (12). However, the biochemical features of MT related to these functions have not been fully characterized. In addition, although the gas chromatography–flame photometric detector technique showed that MT isoforms contain sulfide ions (15, 16), it remains unclear if these sulfides are indeed sulfane sulfur atoms that act as essential factors in controlling protein redox states, thereby regulating cellular zinc homeostasis. Because of its constitutive expression, this study focused on MT3, which was originally identified as a growth inhibitory factor (GIF) in the human brain (17). This study aimed to clarify the existence and content of sulfane sulfur in GIF/MT3, the redox regulation of sulfane sulfur in holo- and apo-GIF/MT3 in association with zinc release, and the effect of sulfane sulfur on the thermostability and metal binding affinity of GIF/MT3. We found that sulfane sulfur atoms provide a redox-dependent switching mechanism for zinc/persulfide cluster formation in GIF/MT3.

Results

Existence of persulfide and polysulfide groups in apo-GIF/MT3

It is well recognized that GIF/MT3 is able to bind seven zinc ions. To determine if GIF/MT3 is an SSBP, we used an Escherichia coli expression system to prepare recombinant human Zn7GIF/MT3 protein, from which apo-GIF/MT3 was subsequently prepared (Fig. 1A). To detect sulfur modification in GIF/MT3, we attempted to first measure the molecular weight of the whole protein with and without bound zinc. Using Fourier transform ion cyclotron resonance (FT-ICR)-MALDI-TOF/MS, Zn7GIF/MT3 was mainly detected at m/z = 7071 (Fig. 1B), which corresponded to the mass of zinc-free apo-GIF/MT3 and indicated that zinc was removed during MS analysis. However, apo-GIF/MT3 showed several peaks at m/z = 7071, 7085, 7103, and 7117, with a main peak at m/z = 7053 (Fig. 1C) that corresponded to oxidized GIF/MT3 with nine intramolecular cysteine disulfide bonds, which presumably release nine molecules of H2. Thus, the peaks at m/z = 7085 (oxidized GIF/MT3 plus one sulfur atom), 7103 (apo-GIF/MT3 plus one sulfur atom), and 7117 (oxidized GIF/MT3 plus two sulfur atoms) suggested that oxidized apo-GIF/MT3 contains sulfane sulfur-like species that presumably exist as intramolecular cysteine trisulfide or tetrasulfide bridges. An increase in mass of 32 Da can also result from addition of two oxygen atoms, but we attributed it to one sulfur atom for reasons described later.

Detection of sulfane sulfur in GIF/MT3.

(A) Preparation of recombinant Zn7GIF/MT3 and oxidized apo-GIF/MT3 proteins. Recombinant human Zn7GIF/MT3 (10 μM) was incubated in HCl (0.1 N) at 37°C for 30 min and then replaced with 20 mM Tris-HCl (pH 7.5) buffer and incubated for 36 h at 37°C. After removal of low-molecular-weight molecules using 3 kDa centrifugal filtration, GIF/MT3-bound zinc content was measured using ICP-MS. (B) FT-ICR-MALDI-TOF/MS spectrum (positive-ion mode) of Zn7GIF/MT3. (C) FT-ICR-MALDI-TOF/MS spectrum (positive-ion mode) of oxidized apo-GIF/MT3. (D) Raman spectra of Zn7GIF/MT3, oxidized apo-GIF/MT3, and HPE-IAM-treated GIF/MT3 in the 250–800 cm−1 region. Optimized geometries for (E) α-domain and (F) β-domain models of apo-GIF/MT3 (assuming some cysteines with persulfide and tetrasulfide bonds as shown). Optimized geometries for (G) α-domain and (H) β-domain models of apo-GIF/MT3 (assuming some cysteines with disulfide bonds). (I) Calculated Raman spectra of apo-GIF/MT3 models with/without sulfane sulfurs. FT-ICR, Fourier transform ion cyclotron resonance.

Raman spectroscopy is used to detect bonding changes in proteins, including MTs (18, 19). The Raman shift of Zn7GIF/MT3 (Fig. 1D) contained a peak at 307 cm−1, which is attributable to both S-terminal and S-bridging ligands (e.g., S–Zn, S–Zn–S) (18). Also, the peaks at 761 cm−1 and 778 cm−1 presumably corresponded to cysteine–metal bonds (e.g., C–S–Zn) and backbone vibrations, respectively (18). Overall loss of zinc was indicated by the decrease in the intensity of these peaks in the Raman spectra of apo-GIF/MT3 and GIF/MT3 treated with HPE-IAM to consume sulfane sulfur atoms (Fig. 1D) and also confirmed using inductively-coupled plasma (ICP)-MS (Fig. 1A). The peak around 400 cm−1 is reported to correspond to vibrations of metal–S bridges (e.g., Zn–S– Zn) (18); however, loss of such a peak was not observed for apo-GIF/MT3 and HPE-IAM-treated GIF/MT3. The Raman peaks within the 510–520 cm−1 range reportedly indicate disulfide bonds in MT (18); in our spectra, an intense peak at 511 cm−1 was observed for apo-GIF/MT3 but not Zn7GIF/MT3 and HPE-IAM-treated GIF/MT3 (Fig 1D).

In general, the S–S bonds of polysulfides are strong Raman scatterers due to the high polarizability of the bonding and lone pair electrons at the two-coordinate sulfur atoms (20). It was also shown that S–S, S–S–S, and S–S–S–S structures exhibit different Raman shifts (21, 22) and the different Raman bands reported for polysulfide may correspond to different geometrical forms of the molecule. To confirm the origin of the Raman peak at 511 cm−1, quantum chemical calculations were made based on three-dimensional (3D) homology modeling, as described later, of apo-GIF/MT3 structures with and without persulfides; the free cysteines and their persulfides were assumed to be protonated and some of the neighboring cysteines formed disulfides or tetrasulfides, depending on the model. The details of the model structures (Fig. 1E–H) and the calculation schemes are described in the Experimental procedures section. Figure 1I shows the calculated Raman spectra of apo-GIF/MT3 with thiol (–SH) groups and disulfide (S–S) bonds (apo-GIF/MT3_S2 model), and of apo-GIF/MT3 persulfide (–SSH) groups and tetrasulfide (S–S–S–S) bonds (apo-GIF/MT3_S4 model). Although the theoretical and experimental Raman spectra exhibited different overall shapes, owing to computational limitations, it is clear that the peak near 511 cm−1 was markedly more intense for the apo-GIF/MT3_S4 model than the apo-GIF/MT3_S2 model. The normal mode vectors were evaluated, and the resulting assignments of these peaks are summarized in Table S1. The peaks mainly corresponded to the stretching and bending of disulfide and tetrasulfide bonds. The commensurate increase in peak intensity with the number of S–S bonds was consistent with the fact that the apo-GIF/MT3_S4 model has several S–S and S–S–S–S bonds, while the apo-GIF/MT3_S2 model has only S–S bonds. The Zn-binding models with/without persulfide also showed that the peaks around 500 cm−1 were almost lost in Zn7GIF/MT3 without persulfide (Fig. S1 and Table S2), indicating that the peak near 488 cm−1 (Fig. 1I) for Zn7GIF/MT3 corresponded to the S–S structure of persulfide. Taken together, these results suggest the existence of sulfane sulfur atoms in both Zn7GIF/MT3 and apo-GIF/MT3.

Determination of sulfane sulfur atoms in Zn7GIF/MT3

HPE-IAM is a relatively inert electrophile that allows the detection of sulfur atoms (e.g., H2S) by forming a bis-S-β-(4-hydroxyphenyl)ethyl acetamide (bis-S-HPE-AM) adduct (8). Our rationale was that if GIF/MT3 is an SSBP, the interaction of HPE-IAM with Zn7GIF/MT3 should eventually form a bis-S-HPE-AM adduct that can be quantified using LC-MS/MS with the stable isotope-labeled standard bis-S34-HPE-AM (Fig. 2A). Small molecules such as H2S were removed during the purification of Zn7GIF/MT3 to exclude their contribution to the measured bis-S-HPE-AM adduct concentration. In a preliminary examination, a negligible amount of sulfane sulfur in Zn7GIF/MT3 could be detected after 36 h incubation with HPE-IAM at 37°C. Stillman and coworkers reported that it was difficult for N-ethylmaleimide to access an apo-MT isoform at 37°C because of its folded structure, whereas heat treatment allowed such an electrophile to covalently bind the protein (23). Therefore, as expected, the amount of sulfane sulfur detected in Zn7GIF/MT3 depended on the HPE-IAM concentration (plateauing at 5 mM), the amount of Zn7GIF/MT3 (up to 10 µM), and the reaction temperature and duration (Fig. 2B–D). We performed the reaction with 5 mM HPE-IAM at 60°C for 36 h. Under these optimized conditions, each MT isoform (each containing 20 cysteine residues) possessed approximately 20 sulfane sulfurs (Fig. 2E). None of the Cys-to-Ala mutants of GIF/MT3 possessed sulfane sulfur (Fig. 2E), indicating that all 20 sulfane sulfurs were bound to cysteine residues of Zn7GIF/MT3. Although the form of binding (e.g., 20 RSSH, 10 RSSSH, RSS20SR, 2 RSS10SR) was not identified, persulfide (20 RSSH) was suggested to be formed rather than polysulfide for reasons described in the discussion section.

Sulfane sulfur assay optimization and quantification of MT sulfane sulfur content.

(A) Schematic showing the detection of sulfane sulfur in Zn7GIF/MT3. (B) Sulfane sulfur detected in Zn7GIF/MT3 after incubation with the indicated concentrations of HPE-IAM at 60°C for 36 h. (C) Sulfane sulfur detected in Zn7GIF/MT3 after incubation with 5 mM HPE-IAM at 60°C for 36 h. (D) Sulfane sulfur detected in Zn7GIF/MT3 after incubation with 5 mM HPE-IAM at 37°C or 60°C for the indicated times. (E) Sulfane sulfur detected in human Zn7MT1, Zn7MT2, Zn7GIF/MT3, wild-type (WT) Zn7GIF/MT3, and apo-GIF/MT3 with all Cys residues mutated to Ala (all C/A), each incubated with 5 mM HPE-IAM at 60°C for 36 h. Sulfane sulfur content was measured using LC-MS/MS. HPE-IAM, β-(4-hydroxyphenyl)ethyl iodoacetamide.

Redox-based GIF/MT3 recycling system during oxidative stress

To explore the functional role of sulfane sulfur in GIF/MT3, we examined the stability of sulfane sulfur in the protein with or without bound zinc. Freshly prepared Zn7GIF/MT3 and apo-GIF/MT3 possessed almost the same amount of sulfane sulfur (Fig. 3A). Unexpectedly, sulfane sulfur content in Zn7GIF/MT3 remained unchanged for up to 28 days in 20 mM Tris-HCl (pH 7.5) at 37°C (data not shown). In contrast, in apo-GIF/MT3, sulfane sulfur content decreased markedly within 12 h of incubation, and the addition of zinc blocked any further decrease (Fig. 3A). This suggests that zinc ions are rapidly re-coordinated by the persulfide group in apo-GIF/MT3, thereby stabilizing sulfane sulfur atoms. To examine the possibility of forming intramolecular cysteine tetrasulfide, which is stable and cannot react with iodoacetamide in the absence of a reducing agent (24), apo-GIF/MT3 left in 20 mM Tris-HCl (pH 7.5) for 36 h (i.e., oxidized apo-GIF/MT3) was incubated with the reducing agent tris(2-carboxyethyl)phosphine (TCEP). The presence of free SH/SSH groups in oxidized apo-GIF/MT3, determined using 5,5′-ditiobis-(2-nitrobenzoic acid) (DTNB) (25), was negligible but increased following TCEP incubation, leading to a complete recovery of sulfane sulfur atoms (Fig. 3B). These observations led us to assume that the time-dependent disappearance of persulfide in apo-GIF/MT3 (Fig. 3A) was not due to the oxidative degradation of sulfane sulfur but rapid closure of a ring that can be cleaved by TCEP (Fig. 5C). Moreover, our method, based on TCEP-mediated reduction of tetrasulfide and subsequent trapping of sulfane sulfur atoms by HPE-IAM, was validated using the model compounds N-acetylcysteine-tetrasulfide (Fig. 4A) and diallyltetrasulfide (Fig. 4A and 4B). In the absence of TCEP, minimal amounts of bis-S-HPE-AM adducts were detected in all the compounds examined. However, incubation with TCEP resulted in the stoichiometric detection of sulfane sulfur but not oxidized-N-acetylcysteine and diallyl disulfide, suggesting that sulfane sulfur was stably trapped by HPE-IAM during the 36 h TCEP incubation. A possible mechanism of reaction between tetrasulfide compounds and HPE-IAM is shown in Fig. 4C. Thus, we confirmed that sulfane sulfur atoms of cysteine tetrasulfide in apo-GIF/MT3 could be preserved after zinc release and oxidation.

Sulfane sulfur stability in apo-GIF/MT3 and its restoration by a reducing agent.

(A) Stability of sulfane sulfur in apo-GIF/MT3 incubated with or without (Cont) zinc. To prepare apo-GIF/MT3, Zn7GIF/MT3 was incubated in 0.1 M HCl for 30 min, then the buffer was replaced with 20 mM Tris-HCl (pH 7.5). To examine the stability of sulfane sulfur in apo-GIF/MT3, freshly prepared apo-GIF/MT3 (2 µM) with or without added zinc ions were incubated at 37°C for up to 24 h. (B) Effect of tris(2-carboxyethyl)phosphine (TCEP) on sulfane sulfur binding and free SH/SSH groups in oxidized apo-GIF/MT3. To prepare oxidized apo-GIF/MT, Zn7GIF/MT3 was incubated in HCl (0.1 N) at 37°C for 30 min and then replaced with 20 mM Tris-HCl (pH 7.5) buffer and incubated for 36 h at 37°C. The resulting oxidized apo-GIF/MT3 protein (10 µM) was incubated with 0, 1, 10, 50, or 100 mM TCEP in 20 mM Tris-HCl (pH 7.5) at 37°C for 1 h, then low-molecular-weight molecules were removed by 3 kDa ultrafiltration for 6 times. Sulfane sulfur content was determined using LC-ESI-MS/MS, and the concentrations of free SH/SSH groups were measured using Ellman’s reagent.

Reactivity of HPE-IAM with tetrasulfide derivatives as models of tetrasulfide bridges in apo-GIF/MT3.

(A) Reactivity of HPE-IAM with N-acetylcysteine (NAC) derivatives. Oxidized NAC (oxiNAC), NAC-trisulfide (NAC-S1), and NAC-tetrasulfide (NAC-S2) (each 10 µM) were incubated with HPE-IAM (5 mM) at 60°C for 1 or 36 h with or without TCEP (1 mM). (B) Reactivity of HPE-IAM with diallyl polysulfide derivatives. Diallyl disulfide (DADS), diallyl trisulfide (DATS), or diallyl tetrasulfide (DATetraS) (each 10 µM) were incubated with HPE-IAM (5 mM) at 60°C for 1 or 36 h with or without TCEP (1 mM). (C) Scheme showing possible reactions of tetrasulfide derivatives with HPE-IAM and TCEP. Bis-S-HPE-AM, bis-S-β-(4-hydroxyphenyl)ethyl acetamide.

Redox-dependent release of zinc ions and recycling of sulfane sulfur in GIF/MT3.

(A) Quantitation of zinc ions released from Zn7GIF/MT3 by H2O2 and S-nitroso-N-acetylpenicillamine (SNAP). To examine the release of zinc ions by H2O2 and SNAP, Zn7GIF/MT3 (10 µM) was treated with H2O2 (1 or 5 mM) or SNAP (1 or 5 mM) in 100 mM Tris-HCl (pH 7.5) at 25°C for 30 min. After removing H2O2/SNAP using 3 kDa ultrafiltration for 4 times, free SH/SSH groups and sulfane sulfur content in GIF/MT3 were determined. (B) Free SH/SSH content in Zn7GIF/MT3, determined by H2O2 or SNAP treatment after incubation with TCEP. To examine the interaction of Zn7GIF/MT3 with H2O2 or NO, Zn7GIF/MT3 (10 µM) was incubated with H2O2 (1 or 5 mM) or SNAP (1 or 5 mM) in 100 mM Tris-HCl (pH 7.5) at 25°C for 30 min. After removing H2O2/SNAP using 3 kDa ultrafiltration for 4 times, the resulting proteins (5 µM) were incubated with TCEP (50 mM) in 100 mM Tris-HCl (pH 7.5) at 37°C for 1 h. After removing TCEP using 3 kDa ultrafiltration for 5 times, sulfane sulfur content was determined using LC-ESI-MS/MS and the concentrations of free SH/SSH groups were measured using Ellman’s reagent. (C) Proposed reactions between a zinc/persulfide cluster in GIF/MT3 and H2O2 or NO.

Several reports have indicated that oxidative modification of MTs results in the release of zinc involved in zinc signaling (26, 27). Incubation with H2O2 and S-nitroso-N-acetylpenicillamine (SNAP), a nitrosonium ion donor, induced zinc release from Zn7GIF/MT3 (Fig. 5A). Under these conditions, the numbers of free SH/SSH groups and sulfane sulfur atoms in GIF/MT3 were also decreased by H2O2 and SNAP treatment. However, subsequent TCEP treatment nearly restored the original levels of free SH/SSH and sulfane sulfur (Fig. 5B). The persulfide in apo-GIF/MT3 appeared to be resistant to TCEP-induced release of sulfane sulfur, although tetrasulfide was not. Overall, it seems likely that sulfane sulfur in Zn7GIF/MT3 acts as a reserve of sulfur to be modified under physiological oxidative stress and a component of the redox-active closed-ring structure regulated by reductants (Fig. 5C).

The interaction of sulfane sulfur species with KCN to yield thiocyanate and thiol products (cyanolysis) has been used as evidence of the presence of protein hydropersulfides (28). Therefore, we used KCN to eliminate the sulfane sulfur atoms from Zn7GIF/MT3. KCN treatment decreased the sulfane sulfur atom content of Zn7GIF/MT3 by approximately 75% (Fig. 6A). After removing KCN, the reducing agent TCEP was subsequently added because intramolecular cysteine disulfide/tetrasulfide bridges can be formed under the condition. TCEP did not recover the level of sulfane sulfur in GIF/MT3 (Fig. 6A), indicating that KCN indeed removed sulfane sulfur from GIF/MT3. In addition to eliminating the sulfane sulfur atoms, KCN treatment also reduced the zinc content of GIF/MT3 (Fig. 6B). To examine the role of sulfane sulfur in zinc retention, sulfane sulfur-diminished apo-GIF/MT3 was incubated with zinc after TCEP treatment to reconstruct zinc-bound GIF/MT3. Re-coordination of zinc ions to KCN-treated apo-GIF/MT3 was incomplete compared with KCN-untreated apo-GIF/MT3 (Fig. 6B), implying that the sulfane sulfur is an essential zinc ligand in apo-GIF/MT3 and that an asymmetric SSH or SH ligand is insufficient for native zinc binding (Fig. 6C).

Contribution of sulfane sulfur in GIF/MT3 to zinc binding.

(A) To eliminate sulfane sulfur in Zn7GIF/MT3 by cyanolysis, Zn7GIF/MT3 (10 µM) was reacted with KCN (75 mM) in 100 mM Tris-HCl (pH 7.5) at 37°C for 14 h. After removal of KCN, the resulting protein was incubated with TCEP (10 mM) in 100 mM Tris-HCl (pH 7.5) at 37°C for 1 h. After removal of TCEP, sulfane sulfur content in GIF/MT3 was determined using LC-ESI-MS/MS. (B) Comparison of zinc binding capacity of GIF/MT3 before and after cyanolysis. Zn7GIF/MT3 (10 µM) was incubated with KCN (75 mM) in 100 mM Tris-HCl (pH 7.5) at 37°C for 14 h. After removal of KCN, the resulting protein was incubated with TCEP (10 mM) in 100 mM Tris-HCl (pH 7.5) at 37°C for 1 h. After removal of TCEP, the resulting protein (5 µM) was incubated with zinc chloride (50 µM) in 50 mM Tris-HCl (pH 7.5) at 37°C for 1 h. Low-molecular-weight molecules were removed using 3 kDa ultrafiltration after each step. Protein-bound zinc content was determined using ICP-MS. *p < 0.05 and **p < 0.01.

Reduction of apo-GIF/MT3 by thioredoxin

Thioredoxin (Trx) is a master enzyme that reduces disulfide bonds in cellular proteins (29). Holmgren previously reported that E. Coli Trx predominantly catalyzes S–S bond cleavage of insulin (Km ∼ µM) rather than low-molecular-weight substances such as cystine and oxidized GSH (30). Surprisingly, apo-GIF/MT3 (Km = 30 nM, Kcat = 31,536 min−1, Kcat/Km = 1051 × 106 M−1min−1) was a much more efficient substrate than insulin (Km = 1,192 nM, Kcat = 19,114 min−1, Kcat/Km = 16 × 106 M−1min−1) (Fig. 7A and B), whereas Trx was unable to reduce Zn7GIF/MT3 (Fig. 7C), as was the case for TCEP (Fig. 6A). Therefore, we hypothesized that the zinc/persulfide clusters in Zn7GIF/MT3 may block the interaction of the protein with Trx and that the zinc ions bound to GIF/MT3 may act as a repressor of Trx-mediated S–S bond cleavage. In addition, apo-GIF/MT3 was a poor substrate for Trx-related proteins 14 (TRP14) and 32 (TRP32) (Fig. 7C). Furthermore, HPE-IAM trapping assay analysis confirmed that the Trx/Trx reductase (TR) system recovered sulfane sulfur content in apo-GIF/MT3 (Fig. 7D) but not in the low-molecular-weight (<3 kDa) fraction (data not shown). These observations indicate that Trx is a powerful enzyme that cleaves the tetrasulfide bond in apo-GIF/MT3 and that persulfide in apo-GIF/MT3 seems to be resistant to Trx as well as TCEP. Notably, a small amount of sulfane sulfur in apo-GIF/MT3 was observed even in the absence of Trx and TR, thereby supporting our conclusion (Fig. 1E–I) that some persulfides or their deprotonated forms exist in apo-GIF/MT3. This may be a unique SSBP-related feature of GIF/MT3.

Reduction of apo-GIF/MT3 by thioredoxin (Trx) and subsequent regeneration of sulfane sulfur.

(A) Velocity (V) of Trx-catalyzed reduction of oxidized apo-GIF/MT3 substrate (S). Oxidation of NADPH was followed by measuring the absorbance of NADPH at 340 nm. (B) Comparison of substrate reduction by NADPH and the thioredoxin system. (C) NADP+ formation upon incubation of: oxidized apo-GIF/MT3 with Trx/TR, TRP14/TR, or TRP32/TR; and Zn7GIF/MT3 with Trx/TR. (D) Regeneration of sulfane sulfur in oxidized apo-GIF/MT3 after incubation with the Trx/TR system. TR, Trx reductase; TRP14, Trx-related protein 14; TRP32, Trx-related protein 32.

3D modeling of GIF/MT3 with sulfane sulfur atoms

We generated a 3D homology model of human Zn7GIF/MT3 using the Molecular Operating Environment (MOE) software and the Protein Data Bank (PDB) structures 4MT2 and 2F5H as templates (Fig. S2). Then we created a 3D structure of sulfane sulfur-bound Zn7GIF/MT3 (one sulfane sulfur per cysteine residue), Zn7S20GIF/MT3 (Fig. 8A), which was also used for Raman spectra modeling (Fig. 1E-I). The predicted 3D structure of Zn7S20GIF/MT3 was almost the same as that of Zn7GIF/MT3 (Fig. 8A), with the root-mean-square deviation of atom positions being only 0.789 Å. Similar results were obtained for Zn7MT1 and Zn7MT2 (Fig. S3). Zn7GIF/MT3 contains a cyclohexane-like Zn3Cys9 cluster in the β domain and a bicyclononane-like Zn4Cys11 cluster in the α domain (31). The structures of both clusters were mostly maintained even when all thiol groups were changed to persulfides by adding one sulfane sulfur atom to each (Fig. 8B). Schematic structures of the generated Zn7GIF/MT3 with or without sulfane sulfurs are shown in Fig. S4. Addition of two sulfane sulfur atoms, corresponding to cysteine trisulfide, disrupted each cluster structure (cf. Fig. S5 and Fig. 8B). When they contained one sulfane sulfur in each cysteine, the thermostability scores of MT1, MT2, and GIF/MT3 in the presence of zinc ions were higher than those in the absence of zinc ions (Table S3), indicating that these ions are key to the thermostability of MT isoforms, including those containing sulfane sulfur atoms. The thermostabilities and Cd7, Cu7, Hg7, and Zn7 binding affinities of S20GIF/MT3 were more favorable than the corresponding values of the sulfane sulfur-free protein (Table 1). Conversely, placing more than one sulfane sulfur on each cysteine residue decreased the thermostability and zinc binding affinity (Fig. 8C). Collectively, these results indicate that zinc ions contribute to protection against persulfide oxidation and MT thermostability, while sulfane sulfur atoms participate in cysteine tetrasulfide formation, marked enhancement of metal binding affinity, and rearrangement of zinc ions. Therefore, our study provides evidence for an interdependence of zinc and sulfane sulfur and for unique structural and functional roles of the persulfide groups in GIF/MT3.

Structural modeling of sulfane sulfur in GIF/MT3 using MOE, and a reaction scheme for sulfane sulfur-based zinc/persulfide cluster.

(A) Comparison of three-dimensional structures of Zn7GIF/MT3 (pink) and Zn7S20GIF/MT3 (green). (B) Cyclohexane-like Zn3Cys9 cluster in the GIF/MT3 homology model, and bicyclononane-like Zn4Cys11 cluster derived from PDB structure 2F5H with (lower) or without (upper) sulfane sulfur. Yellow, orange, and gray spheres indicate cysteine residues, sulfane sulfur, and zinc ions, respectively. (C) Thermostability and zinc binding affinity scores of GIF/MT3 with different numbers of sulfane sulfurs at each cysteine residue. (D) A proposed model for redox-dependent hold-and-release regulation of zinc ions by GIF/MT3.

Thermostability and metal binding affinity scores of growth inhibitory factor (GIF)/metallothionein-3 (MT3) with or without sulfane sulfur. Values were calculated using the Protein Design module of the Molecular Operating Environment (MOE) software.

To confirm the presence of SSBPs in mouse brain, we attempted to isolate them from the high-molecular-weight fraction (>3 kDa) of the cytosol using diethylaminoethyl (DEAE)-Sepharose CL-6B column chromatography. Surprisingly, an abundance of SSBPs were detected, and approximately half of them were tightly bound to the column and eluted in buffer containing 0–0.4 M NaCl (Fig. 9A). Although SSBPs from other proteins with iron/sulfur clusters may have also been detected, this possibility remains to be explored in future studies. Eluate corresponding to the peak concentration of SSBPs (fractions 40 to 44) was further separated using Sephacryl S-100 column chromatography (Fig. 9B), which resolved two major SSBP-related peaks. We collected eluate corresponding to the latter (fractions 40 to 43), which contained proteins with high SSBP content and a mass of approximately 13 kDa, even though its total protein concentration was low. These proteins were then separated using Blue Sepharose chromatography (Fig. 9C). While proteins that bound tightly to the Blue Sepharose resin did not contain sulfane sulfur, an SSBP that eluted in fractions 3 to 5 migrated as a single band (16 kDa) using SDS-PAGE (data not shown). This 16 kDa SSBP was confirmed to be GIF/MT3 using nano ultra-performance LC-MS/MS (Table S4).

Separation of sulfane sulfur-binding proteins from mouse brain cytosol using column chromatography.

(A) Diethylaminoethyl Sepharose CL-6B column. (B) Sephacryl S-100 column. (C) Blue Sepharose column. Triangles, closed circles, and dotted lines indicate sulfane sulfur, protein, and NaCl concentrations, respectively. Portions of each fraction were incubated with 5 mM of HPE-IAM in 20 mM Tris (pH 7.5) at 37°C for 30 min and the sulfane sulfur content was determined from the bis-S-HPE-AM adduct concentration measured using LC-MS/MS. Protein concentration was determined using the bicinchoninic acid assay. Isolation of sulfane sulfur-binding protein was performed as described in the Experimental procedures.

Discussion

MT isoforms are believed to possess a zinc/thiolate cluster characterized by strong Zn–S bonds but facile release of zinc ions under oxidative stress (12, 13). Here, we developed a reliable assay involving prolonged (36 h) incubation with HPE-IAM at 60°C to extract sulfane sulfur from Zn7GIF/MT3 and isotope-dilution LC-MS/MS analysis. The present study provided evidence that MTs are SSBPs containing a sulfane sulfur atom on each of their 20 cysteine residues, which form a zinc/persulfide cluster. Although Capdevila et al. previously showed evidence for existence of sulfide ions in recombinant MT1, MT2, and MT4, they detected only one to four sulfide ions liberated from MTs as H2S gas using gas chromatography–flame photometric detection in strongly acidic conditions (15). These observations suggest that unlike our assay, this method is likely to underestimate the sulfane sulfur content of proteins. While our assay has difficulty detecting sulfane sulfur in oxidized polysulfide bridges such as cysteine tetrasulfide, which is supported by a recent observation (24), a TCEP cleavage step enabled this problem to be overcome (Fig. 4C).

Sulfane sulfur modification of MTs appears to be universal because similar sulfane sulfur contents were observed in recombinant human MT1, MT2, and GIF/MT3 (Fig. 2E). Although MTs have been mainly studied in vertebrates, their diversity and distribution have been widely reported (32). So far, three functional MT forms (reduced apoprotein, oxidized apoprotein, and metalated protein) are known. In this current study, we propose that sulfane sulfur is another key factor involved in regulation of MT function that may have major implications for several biological functions.

Oxidation of sulfane sulfur in GIF/MT3 is a fascinating mechanism of zinc release that does not involve direct thiol oxidation. There is little doubt that zinc release from the zinc/persulfide cluster in GIF/MT3 will be sensitive to mild oxidative stress because the pKa value of cysteine persulfide is lower than that of cysteine (33). However, formation of cysteine tetrasulfides following zinc release from the oxidized GIF/MT3 (Fig. 8D) represents a paradigm shift in GIF/MT3 biochemistry. The sulfane sulfur atoms of MT-tetrasulfide are stably retained and can reacquire zinc after they are reduced, as shown in Fig. 8D. Tetrasulfides, whose presence in apo-GIF/MT3 was shown (Fig. 1C and 1D), are presumably formed in response to structural frustration of the disulfide form, as reported for the sulfide-responsive transcriptional repressor, SqrR (24). In our preliminary study, we failed to directly identify cysteine tetrasulfide during reaction of apo-GIF/MT3 with pronase because alkaline hydrolysis of polysulfide makes it unstable in water (34, 35). We therefore speculate that cysteine tetrasulfide groups exist in an acidic local environment of apo-GIF/MT3 and that Trx rapidly interacts with and cleaves tetrasulfide S–S bonds because of their markedly low pKa values, resulting in the regeneration of persulfide groups.

It is believed that the function of the sulfane sulfur moiety in proteins is to protect cysteine thiols from irreversible oxidation (e.g., to sulfinic acid and sulfonic acid) because such oxidative modifications of cysteine persulfides can be reversed by Trx-mediated reduction (36). In other words, sulfane sulfurs act as “sacrificial” sulfur atoms. However, in this study, we discovered that sulfane sulfur has a higher affinity for zinc than thiol (Fig. 8C and Table 1) and is stored in non-sacrificial tetrasulfide groups when oxidized (Fig. 8D). As a result, tetrasulfides in oxidized-apo-GIF/MT3 are reduced by the Trx system, with Trx being regenerated to a reduced form by NADPH and TR, thereby enabling reacquisition of zinc ions by the persulfide moiety. In contrast, Trx has been proposed to reduce albumin-persulfide (37, 38). A possible explanation for this discrepancy is that apo-GIF/MT3-persulfide is rapidly changed into a different conformation that is topologically resistant to Trx reduction. In other words, Trx may be substrate-specific.

While our proposed mechanism of MT redox regulation is consistent with that proposed by Maret et al. (13), discovery of sulfane sulfur in MTs explains unknown features of MT redox biochemistry. Maret and coworkers showed that approximately 50% of MT existed in the apo form in the rat brain, although they did not examine specific isoforms (39). A reasonable explanation for this observation is that reduced apo-MT can undergo redox-coupled reactions with oxidized proteins (40), leading to the formation of apo-MT-tetrasulfide, which loses its zinc ion-binding capability. GIF/MT3 is a constitutive form predominantly expressed in the brain (41) and protects against Alzheimer’s disease (42, 43). Notably, several studies have indicated that Trx acts as a protection factor in Alzheimer’s disease (44, 45). Although the involvement of GIF/MT3 and Trx in regulating this disorder has not been elucidated, Trx-mediated reduction of apo-GIF/MT3 may lead to the reduction of unknown proteins that might suppress the onset of Alzheimer’s disease because of the high antioxidant capabilities of apo-MT persulfides. Further studies are required to identify the redox-coupled protein dynamics associated with the reduced form of apo-GIF/MT3 and their relevance to the molecular basis of Alzheimer’s disease.

To our knowledge, this is the first study to perform 3D structural modeling of an SSBP with or without sulfane sulfur. Our structural modeling studies revealed that, like Zn7GIF/MT3, the seven zinc ions of Zn7S20GIF/MT3 were tetrahedrally coordinated by the array of 20 sulfane sulfurs but not by cysteine thiols, thereby forming two zinc/persulfide clusters (Fig. 8B). As shown in Figs. 8A and S3, cyclohexane-like Zn3S9 and bicyclononane-like Zn4S11 clusters were conserved even in the presence of 20 sulfane sulfurs without affecting the overall structure of the MTs. Nevertheless, sulfane sulfur is important for both metal binding affinity and protein stability (Table 1) and thus MT function. We suggest that the 20 sulfane sulfurs are evenly distributed among 20 cysteine residues in GIF/MT3 for the following reasons: i) zinc binding of Zn7GIF/MT3 was suggested to involve a C–S–S–Zn rather than Zn–S–Zn structure (Fig. 1D); ii) addition of two or three sulfane sulfurs to each cysteine residue in Zn7GIF/MT3 decreased its stability (Fig. 8C); iii) the polysulfide form of sulfane sulfur seems to have difficulty maintaining zinc/sulfur clusters in GIF/MT3 (Fig. S5). However, one of the limitations of our study is that we did not directly obverse such zinc-persulfide cluster itself.

Because protein sulfuration occurs during nascent protein translation, SSBPs appear to be ubiquitous in cells. In fact, we previously reported that a variety of cellular proteins were per/poly-sulfidated, as determined using a tag-switch-tag assay. We have recently characterized several SSBPs such as GSH S-transferase P1 (GSTP1) (9), dynamin-related protein 1 (Drp1), alcohol dehydrogenase 5 (ADH5), glyceraldehyde-3-phosphate dehydrogenase (GAPDH), ethylmalonic encephalopathy 1 (ETHE1) (8), and now MT1, MT2, and GIF/MT3. As shown in Fig. 9, the present assay also confirmed that there are numerous SSBPs in addition to GIF/MT3 in the cytosol of the mouse brain. Notably, 3,207 zinc-binding proteins in the human proteome have been identified with three and four zinc ligands, with 40% of the latter category consisting of Cys4 coordination (46). Once oxidants react with thiols in a zinc finger domain, zinc is released from the coordination site, resulting in inhibition of the zinc finger protein function. However, disulfide formation in the zinc finger domain is reversed by reducing agents such as GSH.

We speculate that sulfane sulfur is a key component of such a “zinc redox switch”, enabling it to provide high-affinity for zinc and protection against excess oxidative/electrophilic stress. Supporting our notion, zinc finger proteins such as tristetraprolin (47), androgen receptor (48), and prolyl hydroxylase (49) were reported to undergo persulfidation by H2S. In this context, H2S inhibits enzymatic activity of tristetraprolin and androgen receptor, but increases enzymatic activity of prolyl hydroxylase. A possible explanation for this difference is that excess exogenous H2S may cause protein polysulfidation, thereby disturbing the native protein structure. Our findings provide structural and mechanistic insights into the role of sulfane sulfur in hold-and-release regulation of zinc ions by zinc-binding proteins. A future research goal is to investigate the universal role of sulfane sulfur atoms in redox regulation of all zinc-finger proteins.

In conclusion, we have provided evidence that S-sulfuration based on addition of sulfane sulfur plays a central role in hold-and-release regulation of zinc by GIF/MT3. Our study has further revealed a fascinating redox-dependent switching mechanism of a zinc/persulfide cluster involving formation of a cystine tetrasulfide bridge. We believe that our findings open new directions of research in redox and metals biology.

Materials and Methods

Materials

DEAE Sepharose CL-6B, Sephacryl S-100, Blue Sepharose 6 Fast Flow, Glutathione Sepharose 4 Fast Flow, and Benzamidine Sepharose 4 Fast Flow were obtained from GE Healthcare (Uppsala, Sweden). HPE-IAM was obtained from Molecular Biosciences (Boulder, CO, USA). Human recombinant thioredoxin and insulin were purchased from Wako Pure Chemical Industries (Osaka, Japan). TR from rat liver (TrxB) was obtained from Sigma-Aldrich (St. Louis, MO, USA). pGEX-4T-1 cells were obtained from GE Healthcare. All other reagents and chemicals used were of the highest grade available.

Protein expression and purification

Vector pEX-K4J2 containing human cDNA of MT1A, MT2, MT3, or mutant GIF/MT3 (all Cys-to-Ala) between the BamHI and XhoI sites was obtained from Eurofins Genomics (Tokyo, Japan). The cDNAs were excised using BamHI and XhoI and ligated into the corresponding sites of pGEX-4T-1, a glutathione S-transferase (fusion expression vector. An overnight culture of E. Coli BL21 containing 1% v/v pGEX-4T1-1/cDNA vector in fresh Luria-Bertani medium was grown at 37°C for 2 h, then ZnCl2 (final concentration of 500 µM) and isopropyl-1-thio-β-D-galactopyranoside (final concentration of 100 µM) were added to induce the expression of the fusion protein. After 5 h incubation at 37°C, cells were pelleted by centrifugation at 5,000 × g for 10 min at 4°C and resuspended in 5% of the original volume of buffer A (20 mM Tris-HCl [pH 7.5], 150 mM NaCl), then lysed using mild sonication at 4°C. Triton X-100 was added to a final concentration of 1% v/v, and the suspension was mixed gently at approximately 20°C for 1 h to facilitate protein solubilization. After centrifugation at 105,000 × g for 1 h, the supernatant was applied at a flow rate of 2 mL/min to a Glutathione Sepharose column (5.5 cm × 1.5 cm i.d.) pre-equilibrated with buffer A. The column was washed with 100 mL of buffer A, then syringe-filled with 10 mL thrombin solution (400 U/mL in buffer A; Wako, Osaka, Japan) and incubated overnight at room temperature. After incubation, the target proteins and thrombin were eluted using buffer A. The eluate was filtered using a 3 kDa Amicon Ultra centrifugal filter unit (Millipore) following centrifugation with buffer C (20 mM Tris-HCl [pH 7.5], 500 mM NaCl) to concentrate the fractions and exchange the buffer. To remove thrombin, the concentrated sample was applied at a flow rate of 2 mL/min to a Benzamidine Sepharose 4 Fast Flow column (3.9 cm × 1.5 cm i.d.) pre-equilibrated with buffer C. The eluted sample was filtered eight times using a 3 kDa Amicon Ultra centrifugal filter unit with buffer B to exchange the buffer and remove small molecules, then stored at −80°C. The amino acid sequences of the obtained recombinant proteins are shown in Fig. S6.

Protein assay

The cytoplasmic protein concentration in mouse brain was determined using the bicinchoninic acid assay with bovine serum albumin as a standard. The concentrations of GIF/MT3 protein were determined by measuring the absorbance of apo-GIF/MT3 at 220 nm using an extinction coefficient of 53,000 M−1cm−1 (50). To produce apo-GIF/MT3, Zn7GIF/MT3-containing buffer was exchanged with 0.1 M HCl by ultrafiltration. Briefly, protein solution (0.5 mL) was added to an Amicon Ultra centrifugal filter unit. After 30 min centrifugation at 14,000 × g, the filtrate was discarded and 0.1 M HCl (0.45 mL) was added to the retentate. This procedure was repeated two times, and the final retentate was exchanged with 20 mM Tris-HCl (pH 7.5) buffer and used for further studies.

Protein isolation

Animal housing, husbandry, and euthanasia were conducted according to the guidelines of the Animal Care and Use Committee of the University of Tsukuba. Approximately 50 C57BL/6 mice (10–20 weeks-old, ≈1:1 male/female), kindly provided by Prof. S. Takahashi (University of Tsukuba), were anesthetized by intraperitoneal injection of 200 mg/kg phenobarbital. Their brains were perfused with cold saline and then homogenized with four volumes of buffer A (20 mM Tris [pH 7.5], 150 mM NaCl). The homogenate was centrifuged at 9000 × g for 10 min at 4°C and the resulting supernatant was centrifuged at 105,000 × g for 1 h to obtain the cytosol. The cytosolic fraction was filtered and buffer-exchanged 27 times using a 3 kDa Amicon Ultra centrifugal filter unit and centrifugation at 5,000 × g for 30 min at 4°C with buffer B (20 mM Tris [pH 7.5]). To isolate SSBPs, the resulting high-molecular-weight fraction, containing 442 mg protein in 69 mL solution, was applied to a DEAE Sepharose CL-6B column (4.1 cm × 2.5 cm i.d.) pre-equilibrated with buffer B. The column was washed with buffer B at a flow rate of 1 mL/min, then SSBPs were eluted using 200 mL buffer B with a linear gradient of 0–0.4 M NaCl and 5 mL fractions were collected. The major SSBP-containing fractions (fractions 40–44 in Fig. 9A) were filtered using a 3 kDa Amicon Ultra centrifugal filter unit and centrifugation at 14,000 × g for 30 min at 4°C with buffer A seven times to concentrate the protein and exchange the buffer. The concentrated fraction (4.5 mL) was applied to a Sephacryl S-100 column (71 cm × 2.5 cm i.d.) previously equilibrated with buffer A and eluted with buffer A at a flow rate of 1 mL/min and 5 mL fractions were collected The major SSBP-containing fractions with low total protein concentration (fractions 40–43 in Fig. 9B) were combined and filtered, as described above, with buffer B. The concentrated fraction (1 mL) was applied to a Blue Sepharose column (8.4 cm × 2.5 cm i.d.) previously equilibrated with buffer B. The loaded column was washed with buffer B, then SSBPs were eluted a flow rate of 1 mL/min using 200 mL buffer B with a linear gradient of 0–0.4 M NaCl and collected in 10 mL fractions. Eluate containing SSBP (fractions 3–5 in Fig. 9C) was concentrated to a volume of 0.2 mL using Amicon Ultra centrifugal filter units. The resulting material was used for sulfane sulfur detection, SDS-PAGE with silver staining, and western blotting. All operations were performed at 4°C. Protein-bound sulfane sulfur was measured by determining bis-S-HPE-AM concentration after incubation of the protein with HPE-IAM. The incubation mixture (100 µL) consisted of 5 mM HPE-IAM and protein in buffer B. The reaction was performed at 37°C for 30 min and the yield of the bis-S-HPE-AM adduct was determined using liquid chromatography-electrospray ionization-tandem mass spectrometry (LC-ESI-MS/MS), as described later in detail.

Identification of proteins

To identify SSBP in the brain, the isolated protein (75 µg) was incubated with 20 mM dithiothreitol in 50 mM ammonium bicarbonate at 50°C for 1 h, then incubated with 50 mM iodoacetamide in 50 mM ammonium bicarbonate at room temperature for 30 min, and finally digested with trypsin (1.2 µg) at 37°C overnight. The tryptic digests (2.5 µL) were loaded in direct injection mode onto a nanoAcquity ultra-performance LC system (Waters, Milford, MA, USA) equipped with a BEH130 nanoAcquity C18 column (100 mm × 75 μm, 1.7 μm i.d.) held at 35°C. Mobile phases A (0.1% v/v formic acid) and B (0.1% v/v formic acid in acetonitrile) were linearly mixed at a flow rate of 0.3 μL/min using a gradient system as follows: 3% B for 1 min; linear increase to 40% B over 65 min; linear increase to 95% B over 1 min; constant 95% B for 9 min; linear decrease to 3% B over 5 min. The total running time, including initial conditioning of the column, was 90 min. The eluted peptides were transferred to the nanoelectrospray source of a quadrupole TOF-MS instrument (Synapt High Definition Mass Spectrometry system, Waters) via a Teflon capillary union and pre-cut PicoTip (Waters). ESI was used with a capillary voltage of 3 kV and sampling cone voltage of 35 V. Low (6 eV) or elevated (step from 15 to 30 eV) collision energy was used to generate either intact peptide precursor ions (low energy) or peptide product ions (elevated energy). The source temperature was 100°C, and the detector was operated in the positive-ion mode. Data were collected in the m/z = 300–2000 range using an independent reference spray and the NanoLockSpray interference procedure in which Glu-1-fibrinopeptide B (m/z = 785.8426) was infused via the NanoLockSpray ion source and sampled every 10 s for external mass calibration. Data were collected using MassLynx software (v4.1, Waters). ProteinLynx Global Server Browser (v2.3, Waters) was used to identify the protein based on its peptide mass fingerprints.

Measurement of zinc concentration

Each sample was added to an acid-washed test tube containing nitric acid (0.3 mL) and H2O2 (0.1 mL) and digested at 130°C for 2 d in an aluminum dry bath block. The evaporated samples were dissolved in deionized distilled water, and zinc concentrations were measured using ICP-MS (ICPMS-2030, Shimadzu, Japan). A ZnSO4 solution was used as a concentration standard.

FT-ICR-MALDI-TOF/MS

Recombinant human Zn7GIF/MT3 was incubated with 0.1 N HCl at 37°C for 30 min and then exchanged with 20 mM Tris-HCl (pH 7.5) buffer at 37°C for 36 h to prepare oxidized apo-GIF/MT3. Low-molecular-weight molecules were then removed using a 3 kDa Amicon Ultra centrifugal filter unit. Zn7GIF/MT3 or apo-GIF/MT3 (0.5 µL) in 20 mM Tris-HCl (pH 7.5) were mixed with a solution of α-cyano-4-hydroxycinnamic acid matrix (0.5 µL, 60% v/v acetonitrile, 0.2% v/v trifluoroacetic acid) and then dispensed into 384-well plates. The crystals obtained on the plate were analyzed using FT-ICR-MS (7T solariX, Bruker Daltonics, Billerca, MA, USA) equipped with a MALDI source operating in positive ion mode. Analytical conditions were as follows: m/z range, 1000–10,000; number of scans averaged, 3; accumulation time, 2.00 s; polarity, positive.

Raman Spectroscopy

Recombinant Zn7GIF/MT3 was incubated with 0.1 N HCl for 30 min and then replaced with 20 mM Tris-HCl (pH 7.5) buffer for 36 h at 37°C (apo-GIF/MT3) or HPE-IAM (5 mM) in 20 mM Tris-HCl (pH 7.5) for 36 h at 60°C. Then, low-molecular-weight molecules were removed using a 3 kDa Amicon Ultra centrifugal filter unit. The resulting protein was concentrated to ≈4 mg/mL using a 5 kDa centrifugal concentrator (Vivaspin; Sartorius, Gottingen, Germany). For drop-deposition Raman spectroscopy, 0.5 μL of each protein sample was first dried onto a hydrophobic quartz coverslip for up to 15 min under vacuum. Spectra were then collected from the “coffee ring” of each drop, where proteins were found in the absence of bulk salt, using a Raman microscope system with a charge-coupled-device detector (InVia, Renishaw, New Mills, UK). Each sample was excited using a 785 nm diode laser focused through a Leica 50× (0.75 numerical aperture) short-working-distance air objective, with ≈100 mW power incident on each sample. The laser was focused onto the sample using an on-screen camera. WiRE software (v4.1, Renishaw) was used for spectral acquisition, data collection, and cosmic ray removal. The Raman system was calibrated against the 520 cm−1 reference peak of silicon prior to each experiment. All spectra were processed using the IrootLab plugin (0.15.07.09-v) in MATLAB (The MathWorks, Inc., MA, United States). The background was carefully subtracted from the spectra using blank quartz spectra, then the background-corrected spectra were smoothed using a wavelet denoising function. Fluorescence was removed by fitting and subtracting a fifth-order polynomial, and the ends of each spectrum were anchored to the axis using a rubber-band-like function before intensity normalization.

Detection of protein-bound sulfane sulfur

LC-ESI-MS/MS analysis with HPE-IAM was used to determine the levels of protein-bound sulfane sulfur. Some reagents such as H2O2, SNAP, TCEP, and KCN were filtered through a 3 kDa Amicon Ultra centrifugal filter unit prior to use. A high-molecular-weight cytosolic fraction from mouse brain or purified MT protein solution was incubated with HPE-IAM under the appropriate conditions to yield bis-S-HPE-AM adducts. Incubation with HPE-IAM at temperatures >60°C was not suitable because it yielded false-positives for sulfane sulfur in protein-free negative controls. The resulting solutions were filtered through a 3 kDa Amicon Ultra centrifugal filter unit to obtain low-molecular-weight fractions containing bis-S-HPE-AM adducts. HPE-AM adducts were diluted four-fold with 0.1% v/v formic acid containing known amounts of isotope-labeled internal standard (bis-S34-HPE-AM6) and the sulfane sulfur concentrations were determined using LC-ESI-MS/MS. A triple quadrupole mass spectrometer (EVOQ Qube, Bruker) coupled to an ultra-high-performance LC system (Advance, Bruker) was used to perform LC-ESI-MS/MS. Sulfane sulfur-derived bis-S-HPE-AM was separated using a YMC-Triart C18 column (50 mm × 2.0 mm i.d.) at 40°C. Mobile phases A (0.1% v/v formic acid) and B (0.1% v/v formic acid in methanol) were linearly mixed at a flow rate of 0.2 mL/min using a gradient system as follows: 3% B for 3 min; linear increase to 95% B over 12 min; constant 95% B for 1 min; linear decrease to 3% B. MS spectra were obtained using a heated ESI source with the following settings: spray voltage, 4000 V; cone temperature, 350°C; heated probe temperature, 250°C; cone gas flow, 25 psi; probe gas flow, 50 psi; nebulizer gas flow, 50 psi.

Measurement of free SH/SSH content

Ellman’s reagent (DTNB) was used to estimate the concentration of sulfhydryl groups in GIF/MT3 by comparison with a standard curve of the sulfhydryl-containing compound GSH. Briefly, after removal of low-molecular-weight molecules, GIF/MT3 protein (1 µM) was incubated with DTNB (500 µM) in 100 mM Tris-HCl (pH 8.0) and 1 mM EDTA at room temperature for 5 min, and the absorbance at 412 nm was measured. A putative reaction scheme for DTNB with RSSH is shown in Fig S7.

NADPH consumption

To study the kinetics of reduction of human apo-GIF/MT3 by Trx, 200 µL reaction mixtures containing 100 mM KPi (pH 7.5), 100 µM NADPH, 1 µg human Trx (0.5 µM), 0.7 µg rat TrxB (50 nM), and the concentrations of oxidized apo-GIF/MT3 indicated in Fig. 7A were used. To study the reduction of human apo-MT3 or human insulin by Trx, 200 µL reaction mixtures containing 100 mM KPi (pH 7.5), 100 µM NADPH, 1 µg human Trx (0.5 µM), 0.7 µg rat TrxB (50 nM), and the concentrations of oxidized apo-GIF/MT3 or human insulin indicated in Fig. 7B were used. To compare the reduction of human apo-GIF/MT3 or Zn7GIF/MT3 by Trx, TRP14, or TRP32, 200 µL reaction mixtures containing 100 mM KPi (pH 7.5), 100 µM NADPH, 6 µg of human Trx, TRP14, or TRP32, 1 µg of rat TrxB, and 6 µg of oxidized apo-GIF/MT3 or Zn7GIF/MT3 were used (Fig. 7C). Reactions were performed at room temperature and NADPH oxidation was monitored by measuring the absorbance of NADP+ at 340 nm. To restore sulfane sulfur in apo-MT3 after incubation with the Trx/TR system (Fig. 7D), apo-GIF/MT3 (5 µM) was incubated with Trx (6 µM), TrxB (72 nM), and NADPH (100 µM) at 25°C for 30 min in 100 mM KPi (pH 7.5) and then with 5 mM HPE-IAM. Sulfane sulfur content in apo-GIF/MT3 was determined using LC-ESI-MS/MS after 3 kDa filtration, with the peak intensity obtained without apo-GIF/MT3 being subtracted from that obtained with the complete mixture.

Homology modeling of MT isoforms

Homology modeling of human GIF/MT3 was performed using MOE software (2018.01; Chemical Computing Group ULC, 1010 Sherbrooke St. West, Suite #910, Montreal, QC, Canada, H3A 2R7, 2018). To construct a model of GIF/MT3 (National Center for Biotechnology Information reference sequence: NP_005945.1), the crystal structure of rat MT2 (PDB code: 4MT2) and the NMR structure of the α domain of human GIF/MT3 (PDB code: 2F5H) were used as templates. Following the alignment of the primary structures (Fig. S2A), the sequence similarities of the templates were 67.7% and 100% compared with the β domain and α domain of GIF/MT3, respectively. The metals in the templates were changed as desired or deleted to model apo-GIF/MT3. To construct the GIF/MT3 model, 100 independent models of the target protein were built using the segment-matching procedure in MOE. Refinement of the model with the lowest generalized Born/volume integral (GVBI) was achieved by energy minimization of outlier residues in Ramachandran plots generated within MOE. The final model of GIF/MT3 exhibited a 3D structure similar to those of MT2 and the α domain of GIF/MT3 (Fig. S2B). The same method was used to construct homology models of human MT1A and MT2, with rat MT2 as the template for MT1, and both rat MT2 and the α domain of human MT2 (PDB code: 1MHU) as templates for MT2 (Fig. S3).

Generation of sulfane sulfur-bound 3D model of MT

All cysteine residues in the homology model of MT were replaced with cysteine persulfide or polysulfides by performing a residue scan using the Protein Design module of MOE, and the resultant changes in metal binding affinities and complex stabilities were evaluated. The orientation of cysteine persulfide was manually modified to increase its interaction with the metals. Supplementary data file containing homology model of GIF/MT3 with replacement of all cysteine residues by cysteine persulfide in PDB format (*.pdb) was linked to the article (Data S1).

Protein thermostability and metal-binding affinity scoring

We assessed the influence of sulfane sulfur on protein unfolding free energy using the Protein Design module of MOE, which computed a stability scoring function, ΔΔGs, based on the GBVI and weighted surface area:

where ΔEvdw is the AMBER van der Waals interaction energy, ΔEcoul is the AMBER Coulomb interaction energy, ΔEsol is the change in solvation energy calculated using the GBVI, and ESS is the change in energy due to the presence of a disulfide bond. ΔSAsc and ΔSApol are the changes in the side-chain and polar surface areas, respectively. α is a scaling factor accounting for configurational entropy effects, and ΔGsuWT→Mut is the change in stability of the unfolded states. The affinity score was also calculated using MOE software as the difference between the ΔΔGs values of the protein, free zinc, and metal–protein complex.

Quantum chemistry calculations

Since the whole structure of the GIF/MT3 is quite large, we divided MT3 into two domains (α-domain and β-domain) in the quantum chemistry calculations in order to assign the observed Raman spectra. We have independently constructed α-domain and β-domain models of apo-GIF/MT3 with disulfide bonds between neighboring cysteines or tetrasulfide bonds. These models are referred to as apo-MT3_S2 and apo-MT3_S4, respectively, and are shown in Fig. 1E–H. The initial structures were taken from the results of the homology modeling by MOE (see Fig. 8A). H atoms were placed instead of Zn-S bonds in the models. To consider apo-MT3 models, the nearest S atoms are supposed to form disulfide or tetrasulfide bond. The Raman spectra were computed by frequency calculation. All quantum chemical calculations were carried out at B3LYP/6-31G(d) level by GAUSSIAN16 (Revision C.01, Gaussian, Inc., Wallingford CT, 2016). After obtaining the Raman spectra for the α- and β-domains, these spectra are summed to obtain the Raman spectra of the apo-GIF/MT3 as illustrated in Fig. 1I. The corresponding Zn-binding models were constructed and evaluated the Raman spectra with the same manner.

Statistical analysis

All reported data represent the mean ± SD of three independent experiments, except for the MOE calculations. The statistical significance of pair-wise differences was assessed using Student’s t-test. p < 0.05 was considered to indicate a statistically significant difference, and p < 0.01 was considered highly significant.

Acknowledgements

We thank Prof. T. Sawa (Kumamoto University, Japan) for kind donation of NAC derivatives and Prof. E. S. J. Arnér (Karolinska Institutet, Sweden) for kind donation of TRP14 and TRP32.

Funding

This work was supported by Grants-in-Aid for Scientific Research from the Ministry of Education, Culture, Sports, Science, and Technology of Japan (#18H05293 to Y.K.; #20H04340, #22H04799, and #22H05555 to Y.S.).

Author contributions

Y.Shinkai, Y.D., and Y.K. designed the experiments. Y.Shinkai and Y.D. performed the experiments and analyzed the results, except for the Raman analysis. G.D. and S.M. performed the Raman analysis. T.M. and Y. Shigeta performed the computational analysis. M.A.,T.S., M.N., T.I., and T.A. provided useful information and theoretical support. Y.Shinkai wrote the original draft of the manuscript. Y.Shinkai, S.M., J.F., Y.Shigeta, and Y.K. edited the manuscript. Y.K. supervised the study. All authors read and approved the final manuscript.

Competing interests

Authors declare that they have no competing interests.

Data and materials availability

All data are available in the main text or the supplementary materials.

Supplementary Materials

Supplementary material for this article is available.

Fig. S1. Zn-binding GIF/MT3 models and calculated Raman spectra. Fig. S2. Homology modeling of GIF/MT3.

Fig. S3. 3D structural models of human Zn7MT1A and Zn7MT2 Fig. S4. Schematic structures of Zn7GIF/MT3 and Zn7S20GIF/MT3.

Fig. S5. Zn3Cys9 and Zn4Cys11 clusters containing the polysulfide form of sulfane sulfur. Fig. S6. Amino acid sequences of human MTs and GIF/MT3 mutant

Fig. S7. A putative reaction scheme for DTNB with RSSH. Table. S1. Peak assignments for apo-GIF/MT3 model structures

Table. S2. Peak assignments for Zn7S20GIF/MT3 and Zn7GIF/MT3 model structures Table. S3. Thermostability score of sulfane sulfur-bound MT isoforms with or without Zn. Table. S4. Fragment sequences of a mouse brain sulfane sulfur-binding protein, determined using nano-UPLC-MS.

Data. S1. Pdb file of Zn7S20GIF/MT3 generated by homology modelling.