DyP-Type Peroxidases: Recent Advances and Perspectives

In this review, we chart the major milestones in the research progress on the DyP-type peroxidase family over the past decade. Though mainly distributed among bacteria and fungi, this family actually exhibits more widespread diversity. Advanced tertiary structural analyses have revealed common and different features among members of this family. Notably, the catalytic cycle for the peroxidase activity of DyP-type peroxidases appears to be different from that of other ubiquitous heme peroxidases. DyP-type peroxidases have also been reported to possess activities in addition to peroxidase function, including hydrolase or oxidase activity. They also show various cellular distributions, functioning not only inside cells but also outside of cells. Some are also cargo proteins of encapsulin. Unique, noteworthy functions include a key role in life-cycle switching in Streptomyces and the operation of an iron transport system in Staphylococcus aureus, Bacillus subtilis and Escherichia coli. We also present several probable physiological roles of DyP-type peroxidases that reflect the widespread distribution and function of these enzymes. Lignin degradation is the most common function attributed to DyP-type peroxidases, but their activity is not high compared with that of standard lignin-degrading enzymes. From an environmental standpoint, degradation of natural antifungal anthraquinone compounds is a specific focus of DyP-type peroxidase research. Considered in its totality, the DyP-type peroxidase family offers a rich source of diverse and attractive materials for research scientists.


Introduction
General peroxidase research has seemed to wane in recent years, at least in part because peroxidases are ubiquitous and their generally accepted physiological role in plants-removing hydrogen peroxide (H 2 O 2 ) generated inside of cells and constructing a part of the cell wall such as lignin-has been long and thoroughly studied. In contrast, the research history of DyP-type peroxidases is in its early stages, with the first identification of the enzyme occurring only two decades ago. The first DyP-type peroxidase, dye decolorizing peroxidase (DyP) from Geotrichum candidum, was reported in 1999 [1,2]. The origin of this enzyme was later revised to Bjerkandera adusta [3]. In 2007, DyP-type peroxidases were recognized as being distinguishable from other known peroxidase and were defined as a novel peroxidase family-the DyP-type peroxidase family [4]. To date, DyP-type peroxidases have been found in a variety of organisms ( Figure 1). These enzymes also exhibit a varied distribution, functioning not only inside but also outside of cells. In prokaryotes, in particular, the cellular distribution ranges widely from intracellular to extracellular, including periplasmic space. Some secreted DyP-type peroxidases have a Tat (twin arginine translocation) signal, suggesting that they are Tat substrates [5][6][7][8][9][10]. Notably, all secreted DyP-type peroxidases with Tat signal belong to class I, as described in a later section. Moreover, EfeB and YwbN, which are representative DyP-type peroxidases as Tat substrates, reside in the periplasmic space and outside of the cell, respectively. They are homologs of each other and are inferred to play similar physiological roles [8,11]. Among eukaryotes, basidiomycetes have been a source of interesting findings on DyP-type peroxidases. Surprisingly, the DyP-type peroxidases in these organisms are all extracellular, similar to some other peroxidases from basidiomycete. If the main role of DyP-type peroxidases is to scavenge the H 2 O 2 generated inside of the cell or construct a part of cell tissues, it would be unnecessary to secrete the protein into the extracellular milieu. Therefore, secreted DyP-type peroxidases likely serve a function independent of removal of intracellular H 2 O 2 or construct the cell tissues. Interestingly, it appears that some DyP-type peroxidases exist as a cargo protein in encapsulin [12,13]. In particular, there is speculation that MtDyP (class P) provides defense against attacks of host cells. Several DyP-type peroxidases are summarized in outline form in Table 1.  In any case, research performed over the past decade has clarified the unique characteristics of DyP-type peroxidases, converging on the view that they do not exist solely to remove H 2 O 2 but instead have more important specific roles.

Characteristics Based on Tertiary Structure
In early-stage research, DyP-type peroxidases were categorized into classes A, B, C and D according to primary structural homologies (RedOxiBase). Although this orthodox classification is useful, it has limited value for studying catalytic mechanisms and active sites because the primary structure provides only amino acid sequence information. In contrast, tertiary structures define tangible entities that allow for detailed assessments of the relationship between structure and function among members of the DyP-type peroxidase family. In 2015, a new classification scheme was proposed for this family based on structure-based sequence alignments obtained using the multiple three-dimensional alignment tool, MATRAS [42]. Such tertiary structural analyses are apparently effective for further analysis because they revealed genuine structural homologies among different DyP-type peroxidases. Interestingly, this new scheme clearly reclassified the family into three new classes, combining classes C and D into a new class V (adVanced) and renaming classes A and B as classes I (Intermediate) and P (Primitive), respectively [42]. Throughout this review, we apply this new class I, P and V classification scheme. Typical structures of each of the three classes are shown on the right side of Figure 1.
contrast, tertiary structures define tangible entities that allow for detailed assessments of the relationship between structure and function among members of the DyP-type peroxidase family. In 2015, a new classification scheme was proposed for this family based on structure-based sequence alignments obtained using the multiple three-dimensional alignment tool, MATRAS [42]. Such tertiary structural analyses are apparently effective for further analysis because they revealed genuine structural homologies among different DyP-type peroxidases. Interestingly, this new scheme clearly reclassified the family into three new classes, combining classes C and D into a new class V (adVanced) and renaming classes A and B as classes I (Intermediate) and P (Primitive), respectively [42]. Throughout this review, we apply this new class I, P and V classification scheme. Typical structures of each of the three classes are shown on the right side of Figure 1. Figure 1. DyP phylogenetic tree. The tree was constructed with the maximum-likelihood method using RAxML-NG [61] with multiple sequence alignments of DyP amino acid sequences generated by the MAFFT [62] program. Percentages of bootstrap values obtained from 1000 bootstrap replicates are shown at the nodes. The best-fit model of evolution of the alignment was determined using ModelTest-NG [63]. Branches and labels of different phyla are shown in different Figure 1. DyP phylogenetic tree. The tree was constructed with the maximum-likelihood method using RAxML-NG [61] with multiple sequence alignments of DyP amino acid sequences generated by the MAFFT [62] program. Percentages of bootstrap values obtained from 1000 bootstrap replicates are shown at the nodes. The best-fit model of evolution of the alignment was determined using ModelTest-NG [63]. Branches and labels of different phyla are shown in different colors: green, actinobacteria; blue, firmicutes; red, proteobacteria; purple, cyanobacteria; orange, basidiomycota. Reference numbers for each DyP are shown in parentheses. Structures of representative DyPs of the three classes are shown on the right: Class I, DtPA (PDB ID: 6gzw); Class P, DtPB (PDB ID: 6yrj); Class V: DyP (PDB ID: 3afv).
The basic skeletal structure is common among the three classes and consists of a dimeric α + β barrel structure [42]. The structures of classes I and V are constructed based on class P, with some additional regions. Therefore, class P members have the smallest molecular size among the three classes, with members of a class V having the largest size. Notably, all important amino acid residues that define DyP-type peroxidases are included in the skeletal structure (i.e., class P), suggesting that basic functions are determined by this skeletal structure, with extra regions mediating additional functions. For instance, catalytic efficiencies (k cat /K m ) toward anthraquinone compounds are different among the three classes. As shown in Table 1, the catalytic efficiencies of most class V members (10 4 to 10 7 ) are the largest among the three classes. By comparison, catalytic efficiencies range from 10 3 to 10 6 for class I and from 10 2 to 10 5 for class P.

Catalytic Mechanism
The enzyme commission number for DyP is EC 1.11.1.19, which corresponds to a peroxidase group. Actually, in most cases, DyP-type peroxidases show typical peroxidase activity, such as that shown by horseradish peroxidase (HRP). Therefore, the catalytic cycle appears to be nearly the same as that of ubiquitous peroxidases [64]. As shown in Figure 2, general heme peroxidases cycle through resting, compound I and compound II states. The compound I formation process of DyP-type peroxidase is essentially inconsistent with that of classical heme peroxidases such as lignin peroxidase [4]. In the case of DyP-type peroxidase, resting and compound I states have been confirmed, but compound II is controversial. DyPA (class I) from Rhodococcus jostii shows a spectrum corresponding to compound II at pH 7.5 [21]. TcDyP (class I) from Thermomonospora curvata shows compound II at pH 7.8 with both H 2 O 2 and hydroquinone, but not with H 2 O 2 only [30]. Furthermore, compound II was not observed at pH 3, which is the optimum pH for dye decolorizing [30]. In support of this, Shrestha et al. reported that compound II was not observed at low pH in ElDyP (class P) from Enterobacter lignolyticus, suggesting that the catalytic cycle does not follow a typical two-step process [20]. The authors of this latter study suggested that the enzyme adopts a two-electron reduction process for compound I, as shown in Figure 3. Moreover, no exact compound II has yet been reported at low pH for DyPtype peroxidases belonging to classes P or V. Therefore, further study at low pH-the active pH for dye decolorization-is necessary regardless of whether the two-step catalytic cycle with sequential one-electron reduction of the enzyme occurs or not. On the other hand, excess H 2 O 2 deactivates DyP-type peroxidsaes, a property also characteristic of ubiquitous peroxidases.
in the skeletal structure (i.e., class P), suggesting that basic functions are determined by this skeletal structure, with extra regions mediating additional functions. For instance, catalytic efficiencies (kcat/Km) toward anthraquinone compounds are different among the three classes. As shown in Table 1, the catalytic efficiencies of most class V members (10 4 to 10 7 ) are the largest among the three classes. By comparison, catalytic efficiencies range from 10 3 to 10 6 for class I and from 10 2 to 10 5 for class P.

Catalytic Mechanism
The enzyme commission number for DyP is EC 1.11.1.19, which corresponds to a peroxidase group. Actually, in most cases, DyP-type peroxidases show typical peroxidase activity, such as that shown by horseradish peroxidase (HRP). Therefore, the catalytic cycle appears to be nearly the same as that of ubiquitous peroxidases [64]. As shown in Figure 2, general heme peroxidases cycle through resting, compound I and compound II states. The compound I formation process of DyP-type peroxidase is essentially inconsistent with that of classical heme peroxidases such as lignin peroxidase [4]. In the case of DyP-type peroxidase, resting and compound I states have been confirmed, but compound II is controversial. DyPA (class I) from Rhodococcus jostii shows a spectrum corresponding to compound II at pH 7.5 [21]. TcDyP (class I) from Thermomonospora curvata shows compound II at pH 7.8 with both H2O2 and hydroquinone, but not with H2O2 only [30]. Furthermore, compound II was not observed at pH 3, which is the optimum pH for dye decolorizing [30]. In support of this, Shrestha et al. reported that compound II was not observed at low pH in ElDyP (class P) from Enterobacter lignolyticus, suggesting that the catalytic cycle does not follow a typical two-step process [20]. The authors of this latter study suggested that the enzyme adopts a two-electron reduction process for compound I, as shown in Figure 3. Moreover, no exact compound II has yet been reported at low pH for DyP-type peroxidases belonging to classes P or V. Therefore, further study at low pHthe active pH for dye decolorization-is necessary regardless of whether the two-step catalytic cycle with sequential one-electron reduction of the enzyme occurs or not. On the other hand, excess H2O2 deactivates DyP-type peroxidsaes, a property also characteristic of ubiquitous peroxidases.   [20]. Left, compound I; center, ES complex; right, resting state. Oval denotes the heme plane in the enzyme. Asp is the catalytic residue. S and P denote substrate and product, respectively. In a general peroxidase, compound I changes to compound II with one electron reduction, as shown in Figure 2, but in this scheme, compound I of DyP-type peroxidases changes to the resting state directly through two-electron reduction.

Active or Binding Sites
DyP-type peroxidases show a broad range of substrate specificities, and several active sites have been proposed [31,43,49,65]. It is likely that the binding site(s) of most substrates are different from the H2O2 binding site. We will first focus on the H2O2 binding site, which is located at the distal site of the heme. As described previously, aspartic acid and arginine are absolutely conserved in the H2O2-binding site of most DyP-type peroxi- .+ Figure 3. Schematic diagram of two-electron oxidation of substrates by a DyP-type peroxidase, proposed in [20]. Left, compound I; center, ES complex; right, resting state. Oval denotes the heme plane in the enzyme. Asp is the catalytic residue. S and P denote substrate and product, respectively. In a general peroxidase, compound I changes to compound II with one electron reduction, as shown in Figure 2, but in this scheme, compound I of DyP-type peroxidases changes to the resting state directly through two-electron reduction.

Active or Binding Sites
DyP-type peroxidases show a broad range of substrate specificities, and several active sites have been proposed [31,43,49,65]. It is likely that the binding site(s) of most substrates are different from the H 2 O 2 binding site. We will first focus on the H 2 O 2 binding site, which is located at the distal site of the heme. As described previously, aspartic acid and arginine are absolutely conserved in the H 2 O 2 -binding site of most DyP-type peroxidases, whereas general peroxidases have histidine and arginine at this site [44]. In particular, aspartic acid (D) in the GXXDG motif, which is a well-known conserved region among DyPtype peroxidases, replaces the histidine in general peroxidases, accounting for the lower optimum pH of DyP-type peroxidases compared with general peroxidases [4,44]. A D171N point mutation in DyP (class V) from B. adusta results in the disappearance of compound I formation. This causes a drastic decrease in peroxidase activity [4], highlighting the critical importance of aspartic acid in GXXDG. In contrast, Singh et al. reported that the arginine in DyPB (class P) from R. jostii is essential for peroxidase activity [22]. It has similarly been found that the arginine in DtpB (class P) from Streptomyces lividans is also a key residue for peroxidase activity [25]. In this latter study, a serial femtosecond X-ray crystallography approach was used to determine how the distal heme site in DyP-type peroxidase can be tuned to choose either aspartic acid or arginine. In the case of YfeX (class P), the activity toward guaiacol and catechol is retained if the arginine is replaced with other amino acids, suggesting that this arginine may play a limited role [14]. Additionally, it has been reported that the distal aspartic acid of ElDyP (class P) is catalytically more important than the distal arginine and plays a key role in determining the acidic pH optimum of DyPs [20]. Similar effect depending on pH has been reported in a resurrect class V DyP [60].
As noted above, it is clear that DyP forms compound I, indicating two-electron oxidization using hydrogen peroxide. Actually, compound I of DtpB has been directly determined for a peroxidase carrying a porphyrin π cation radical [25]. Although compound I oxidizes various substrates, no reports provide direct evidence to show how and where substrates bind to it. This is one of the least clarified and essential characteristics of DyP-type peroxidases. The active sites of substrates other than H 2 O 2 are probably located apart from the distal heme region, which would otherwise limit access to bulky molecules, such as synthetic dyes. A likely hypothesis is that this site is located at the molecular surface of the enzyme, and that an electron is transferred from the distal area of the heme to the substrate via a long-range electron-transfer route [31,49,66]. A similar speculation has been raised for versatile peroxidases [67]. Several studies have shown that aromatic residues such as tryptophan and tyrosine accumulate and retain radicals, thereby serving as a point of substrate oxidation [19,31,49,66]. This hypothesis seems reasonable, although unfortunately there are no reports of a genuine enzyme-substrate (ES) complex between bulky substrates and aromatic residues in DyP-type peroxidases. In contrast, DMP (2,6-dimethoxyphenol), which is a general substrate for peroxidases, has been reported to associate with asparagine 313 at the molecular surface of DyP from B. adusta (class V), and a hydrogen-bonding network has been reported from there to the propionate of heme [43]. This network is similar to that of ascorbate peroxidase [68]. To date, this is the sole report of an ES complex for a DyP-type peroxidase. Although a Mn 2+ binding pocket was observed in an artificial N246A mutant of DypB [23], there was no report of an ES complex in the case of native DypB. Despite these advances, the location of the binding site for bulky substrates such as synthetic dyes, the representative substrates of DyP, has remained elusive.

Hydrolase
Some DyP-type peroxidases have been reported to have other functions besides peroxidase activity. One of the reaction products confirmed to arise from catalysis of Reactive blue 5-a representative anthraquinone dye-by DyP from Bjerkandera adusta is phthalic acid [44,45]. This indicates that the anthraquinone frame is degraded by hydrolysis. If this is the case, it is reasonable that DyP acts as a hydrolase because this hydrolysis would never proceed in the absence of H 2 O 2 , suggesting the necessity of forming H 2 O from H 2 O 2 .

The importance of H 2 O produced from H 2 O 2 is also reported for classical heme peroxidases and catalases. Jones reported that wet (H 2 O-containing) and dry (non-H 2 O-containing)
forms of compound I apparently play independent roles. He proposed a redox pathway switching mechanism, such that the states for the two electron-equivalent reduction of compound I are accessible in the dry form, but in the wet form only one-electron-equivalent processes are possible, unless the release of water can be stimulated [69]. The importance of a water molecule in the heme distal area was also reported for DtpB from S. lividans (class I) [25]. These reports suggested that H 2 O from H 2 O 2 might play a specific role in the catalytic mechanism. Together, these observations suggest that DyP from B. adusta is a bifunctional enzyme that exerts hydrolase activity using the H 2 O released by the peroxidase function. In contrast, Linde et al. have reported that spontaneous hydrolysis would occur if an anthracenetetrone was formed as an intermediate from an anthraquinone, given that the ubiquitous heme peroxidase HRP also decolorizes Reactive blue 5 [66]. Actually, HRP decolorizes Reactive blue 5, but there is no evidence that it degrades the anthraquinone frame because phthalic acid has thus far not been detected. It is probably the case that decolorization with HRP depends on degradation, not of the anthraquinone frame, but of an auxochrome group. Moreover, there are no reports that anthracenetetrone is generated as an intermediate for a DyP-type peroxidase. These two ideas are summarized in Figure 4.   [44]. Oval denotes the heme plane in the enzyme. B, Spontaneous hydrolysis generates phthalic acid, but predicted intermediates have not been detected [66].

Deferrochelatase or Iron Uptake
In 2009, Létoffé [44]. Oval denotes the heme plane in the enzyme. B, Spontaneous hydrolysis generates phthalic acid, but predicted intermediates have not been detected [66].

Deferrochelatase or Iron Uptake
In 2009, Létoffé et al. reported that EfeB (class I), a DyP-type peroxidase from Escherichia coli, functions as a deferrochelatase [70]. They observed that EfeB captures only iron without degradation of heme, which retains an intact tetrapyrrole skeleton. This phenomenon is quite different from that of heme oxygenase, which degrades the heme skeleton and then "picks out" the iron. This study created a profound impression on many researchers of DyP-type peroxidases. However, the corresponding function of FepB (class I), an EfeB homolog from Staphylococcus aureus, is obscure [11]. Moreover, YwbN (class I) from Bacillus subtilis, also a homolog of EfeB, shows no deferrochelatase activity, but does exhibit peroxidase activity [8]. Overall, whether DyP-type peroxidases have deferrochelatase activity remains a matter of controversy. Viewed from another standpoint, EfeB is a part of the EfeUOB operon, which encodes components of an iron transport system [29]. Interestingly, a similar operon has been found in both B. subtilis and S. aureus [8,11], and it has been proposed that both EfeB homologs are typical peroxidases that result in oxidation of Fe 2+ . Moreover, the efeB gene of B. subtilis is under additional control of several σ factors that are associated with the cell envelope stress response, suggesting a key role in the life-cycle of the organism [8]. Collectively, these studies suggest that the relationship between iron uptake and the role of DyP-type peroxidases must be critical to bacterial viability because iron uptake is essential for life. Further study of this relationship can be expected. A schematic diagram of the EfeUOB operon from the above three organisms is shown in Figure 5. the life-cycle of the organism [8]. Collectively, these studies suggest that the relationship between iron uptake and the role of DyP-type peroxidases must be critical to bacterial viability because iron uptake is essential for life. Further study of this relationship can be expected. A schematic diagram of the EfeUOB operon from the above three organisms is shown in Figure 5.

Oxidase
Peroxidase reactions absolutely depend on peroxides such as H2O2. Surprisingly, MscDyP from Marasmius scorodonius, a typical class V DyP, appears to oxidize β-carotene without H2O2 [39]. If this proves to be the case, it means that MscDyP not only shows peroxidase activity but also possesses oxidase activity, suggesting a bifunctional enzyme. Additionally, catalases, which are similar to heme peroxidases, are also suggested to show phenol oxidase activity in the absence of H2O2 [71]. However, it has been reported that PsaPOX (class V) from Pleurotus sapidus oxidizes β-carotene in the presence of H2O2, suggesting peroxidase activity [57]. Strikingly, β-carotene was found to be transformed by recombinant PsaDyP in both the presence and absence of H2O2, although enzymatic activity was increased by the addition of H2O2 [56]. This suggests that rPsaDyP has an oxidase function in addition to peroxidase activity. PsaPOX was also shown to oxidize several alkenes, such as anethol to anisaldehyde, but the details of the reaction mechanism are still obscure [57].

Physiological Role of DyP-Type Peroxidases
One of the accepted physiological role of a plant peroxidase is to form lignin of cell wall consuming H2O2 generated inside of cells. In contrast, it is noteworthy that many DyP-type peroxidases function in the extracellular environment. This suggests that the main physiological role of these peroxidases is not removal of intracellular H2O2, leading to speculation about other cryptic roles. An additional noteworthy characteristic of DyPtype peroxidases is that they are distributed across a broad range of organisms, suggesting possible divergent physiological roles. Probable physiological roles are considered below.

Anthraquinone Degradation
The DyP (class V) from Bjerkandera adusta Dec 1 is a classic member of this family.

Oxidase
Peroxidase reactions absolutely depend on peroxides such as H 2 O 2 . Surprisingly, MscDyP from Marasmius scorodonius, a typical class V DyP, appears to oxidize β-carotene without H 2 O 2 [39]. If this proves to be the case, it means that MscDyP not only shows peroxidase activity but also possesses oxidase activity, suggesting a bifunctional enzyme. Additionally, catalases, which are similar to heme peroxidases, are also suggested to show phenol oxidase activity in the absence of H 2 O 2 [71]. However, it has been reported that PsaPOX (class V) from Pleurotus sapidus oxidizes β-carotene in the presence of H 2 O 2 , suggesting peroxidase activity [57]. Strikingly, β-carotene was found to be transformed by recombinant PsaDyP in both the presence and absence of H 2 O 2 , although enzymatic activity was increased by the addition of H 2 O 2 [56]. This suggests that rPsaDyP has an oxidase function in addition to peroxidase activity. PsaPOX was also shown to oxidize several alkenes, such as anethol to anisaldehyde, but the details of the reaction mechanism are still obscure [57].

Physiological Role of DyP-Type Peroxidases
One of the accepted physiological role of a plant peroxidase is to form lignin of cell wall consuming H 2 O 2 generated inside of cells. In contrast, it is noteworthy that many DyP-type peroxidases function in the extracellular environment. This suggests that the main physiological role of these peroxidases is not removal of intracellular H 2 O 2 , leading to speculation about other cryptic roles. An additional noteworthy characteristic of DyP-type peroxidases is that they are distributed across a broad range of organisms, suggesting possible divergent physiological roles. Probable physiological roles are considered below.

Anthraquinone Degradation
The DyP (class V) from Bjerkandera adusta Dec 1 is a classic member of this family. This strain was isolated from soil in Japan and exhibits broad decolorizing effects on various synthetic dyes [72]. Notably, DyP showed stronger decolorizing actions against anthraquinone dyes than azo dyes, a unique characteristic compared with other decolorizing enzymes known to date, which have been reported to be effective toward azo dyes [73][74][75][76]. One of the most distinctive characteristics of DyP from B. adusta is its unique ability to degrade the anthraquinone skeleton. Reactive blue 5 is actually completely decolorized through concerted reactions with versatile peroxidases and DyP [46], making these enzymes suitable for treating wastewater containing synthetic dyes. However, such synthetic dyes are not true substrates because they are never generated in nature, suggesting that natural anthraquinone compounds must be true substrates. For example, plants, including trees, synthesize multiple anthraquinone compounds that serve antifungal functions. In this context, DyP from B. adusta degrades alizarin, which is a natural antifungal anthraquinone compound produced by plants [47]. B. adusta is a white rot fungus that parasitizes living trees, which in response generate phytoalexin to protect against infection. Therefore, one probable physiological role is to degrade antifungal anthraquinone compounds and accelerate tree parasitism. This is the only study of its kind to date, but future work on this issue is expected.

Lignin Degradation
A relationship between lignin degradation and some DyP-type peroxidases has been reported. In particular, there are many reports of this function for class V DyPs, as shown in Table 1. To date, lignin peroxidase (LiP), versatile peroxidase (VP), manganese peroxidase (MnP), and laccase (Lac) from basidiomycetes and ascomycetes have been well studied, as have lignin-degrading enzymes from basidiomycetes, such as white rot fungi [67,[76][77][78]. In recent years, several DyP-type peroxidases have been found to degrade lignin or its model compounds [30,[79][80][81]. Interestingly, lignin degradation by DyP-type peroxidases has been reported for bacteria as well as basidiomycetes, whereas general lignin-degrading enzymes are mainly isolated from basidiomycetes. DyPA from Pseudomonas fluorescens pf-5 [17], TfuDyP from Thermobifida fusca [5], and SviDyP from Saccharomonospora viridis DSM43017 [33] are class I, whereas DyP1B from Pseudomonas fluorescens pf-5 [17], DyP2B, and DyPB from Rhodococcus jostii are class P. DypB from Rhodococcus jostii, which is an actinomycete, has been reported to degrade lignin in the presence of Mn 2+ and H 2 O 2 , but its activity is low compared with that of fungal lignin-degrading enzymes [24,35,66]. DypB might be a manganese peroxidase whose primary role is to oxidize Mn 2+ to Mn 3+ [24]. However, the k cat /K m ratio of DypB for Mn 2+ was reported to be 1/31,250th of that of a typical MnP, indicating that Mn 2+ is unlikely an essential substrate for DypB [82]. In contrast, DypA (class I) from the same strain shows no lignin-degrading activity, suggesting a difference in physiological roles, despite the fact that both are DyP-type peroxidases [24]. More puzzlingly, TfuDyP (class I) from T. fusca, which is also an actinomycete, was shown to degrade kraft lignin and oxidize a β-aryl ether lignin model compound [32]. Specifically, this latter study demonstrated that Streptomyces sp. S6 grew in medium containing kraft lignin as a sole carbon source and showed apparent LiP activity. However, in the case of DyP, S6 showed low activity-at most 1% compared with LiP [81]. SviDyP from Saccharomonospora viridis showed optimum pH and temperatures of pH 7.0 and 70 • C, respectively. These characteristics seem to offer advantages compared with other DyP-type peroxidases for practical biobleaching of kraft pulp [33]. Furthermore, two lignin-degrading bacteria, Ochrobacterium sp. and Paenibacillus sp., which contain no class P DyP-type peroxidases that have been implicated in lignin degradation in other bacteria, alternatively possess a multi-copper oxidase gene, which shows oxidation activity for β-aryl ether and biphenyl lignin dimer model compounds [83]. Thus, the importance of DyP-type peroxidases in lignin degradation, at least in bacteria, is open to interpretation.
The situation is different in basidiomycetes, for which considerable research supports lignin degradation. White rot fungi, such as Phanerochaete chrysosporium and Pleurotus ostreatus, in particular have demonstrated prominent lignin degradation activity. Their main enzymes are LiP, MnP and VP. Notably, P. chrysosporium does not have a DyP-type peroxidase. Since DyP-type peroxidases were first identified, their potential for lignin degradation has been a focus of research attention [39,40,[49][50][51][52]84]. Such studies have confirmed the widespread transcript-level expression of DyP-type peroxidases in almost all samples of fungi from forest floor habitats [85]. The class V DyP-type peroxidases, AjP I, AjP II, EglDyP and MepDyP, from basidiomycetes are secreted outside the cell and degrade non-phenolic lignin model compounds through their peroxidase activity [40,50]. However, the lignin-degrading activity of DyP-type peroxidases from basidiomycetes is at most 4% that of LiP from P. chrysosporium [40,66]. IlDyP (class V) from Irpex lacteus has been characterized and suggested to hydrolyze wheat straw [86]. Because wheat straw contains lignocellulose, IlDyP might function in lignin degradation. Consistent with this, IlDyP-1 and IlDyP-2 were reported to degrade the lignin model compound, DMP [87], although this study reported no data on degradation of lignin itself by IlDyP.
Taken together, these observations indicate that most lignin-degrading organisms that possess DyP also have general lignin-degrading enzymes, such as LiP, MnP, VP and multi-copper oxidase; thus, whether lignin-degrading activity is an essential function of DyP-type peroxidases remains obscure.

Life Cycle of an Actinomycete
DtpA (class I) from the actinomycete S. lividans appears to have a specific role in the life cycle of the organism. In S. lividans, copper is important for stimulating the developmental switch between vegetative mycelium and aerial hyphae. DtpA uses H 2 O 2 to oxidize Cu + to Cu 2+ , which causes maturation of GlxA; thus, DtPA is required for maturation of GlxA. GlxA, in turn, generates H 2 O 2 from O 2 , thereby providing the H 2 O 2 necessary for DtPAmediated oxidation of Cu + to Cu 2+ . GlxA is a key protein in the shift from vegetative mycelium to aerial hyphae [88]. Mature GlxA acts in concert with the cellulose synthaselike protein, CslA, to form an extracellular glycan specific for aerial hyphae. This role for DtpA in oxidizing metal ions would thus be similar to the function of EfeB, which oxidizes Fe 2+ to Fe 3+ [8]. Notable in this context, S. lividans also appears to have an efeB homologue, which is located in a gene cluster harboring an iron transporter. Streptomyces avermitilis also has an efeB homologue (SAV_5925), strongly suggesting its specific role.

Cargo Protein of Encapsulin
An additional unique characteristic of several DyPs is their function as a cargo protein for encapsulin, a bacterial nanocompartment protein. One of the best-studied of these DyPs is MtDyP (class P) from Mycobacterium tuberculosis [13,26], a bacterium that slips through defenses generated by the host immune response and induces tuberculosis. MtDyP, which is shielded from oxidative stress in the nanocompartment through association with encapsulin, appears to play an important role in defending against the immune assault by virtue of its peroxidase activity. DypB (class P) from R. jostii was shown to assemble with encapsulin in vitro [12], suggesting the potential of class P DyPs to act as cargo proteins of encapsulin. A recent high-resolution cryogenic electron microscopy study revealed that a DyP-type peroxidase from Mycobacterium smegmatis is a primary cargo protein of mycobacterial encapsulins [89]. Notably, this latter study noted that the encapsulin shell plays a role in stabilizing DyP in a dodecameric form, which is larger than any previously reported DyP oligomer. Considering this packaging of M. smegmatis encapsulin as a model system for M. tuberculosis would suggest a similar role for DyP from M. smegmatis in protecting cells against oxidative stress. By extension, if DyPs from pathogens indeed serve to defend against immune assault from the host, VC2145 VcDyP (class P) from Vibrio cholerae [67] might be speculated to have a similar role. One more noteworthy characteristic is that encapsulated DyP has a specified target peptide toward encapsulin. If this is the case, screening for the presence of the target peptide is effective to find unknown encapsulated DyP-type peroxidase [90].

Perspectives
In this review, we have highlighted the prominent themes in the progression of DyPtype peroxidase research over the past decade. The feature of DyP-type peroxidase that has received the greatest emphasis is the diversity of this family, which displays a widespread expansion of three different classes: P, I and V. Tertiary structural analyses have clearly identified both common and distinct features among the three classes. Substrate specificities and catalytic efficiencies have also been shown to vary among the three classes. Therefore, researchers should continue to apply the current structure-function approach to clarify the catalytic mechanism, which remains unclear. In the end, the catalytic mechanism will likely turn out to be more complicated than that of ubiquitous heme peroxidases, reflecting additional functions such as hydrolase or oxidase activity. One issue in particular that will require further careful study as part of efforts to elucidate the multifunctional feature of DyP-type peroxidase is the wet and dry states of compound I. Surprisingly, the true physiological roles of DyP-type peroxidases remain unclear; thus, establishing these roles is an important area for future research. As noted above, DyPtype peroxidases have been clearly shown to function in various environments, including extracellular, periplasmic as well as intracellular environments, including within encapsulin. These observations suggest that the physiological role of DyP-type peroxidases is not limited to removal of H 2 O 2 inside of cells, hinting at other critical physiological functions. In particular, MtDyP and DyP from B. adusta seem to have a similar physiological role: defending against counterattacks from the host. Moreover, EfeB and DtpA play important roles in oxidizing Fe 2+ and Cu + , respectively, taking part in the life cycle of their organisms. Compared with other peroxidases reported to date, DyP-type peroxidase have unique features that put them in a class of their own, arguably one that is more advanced than that of ubiquitous peroxidases. With future studies, the universe of DyP-type peroxidase will be unveiled, revealing itself to be widespread and deep like the cosmos.
Author Contributions: Conceptualization and organization, writing-original draft preparation, review and editing, supervision Y.S.; data curation and validation T.Y. All authors have read and agreed to the published version of the manuscript.