Báo cáo Y học: Production and chemiluminescent free radical reactions of glyoxal in lipid peroxidation of linoleic acid by the ligninolytic enzyme, manganese peroxidase pot

Production and chemiluminescent free radical reactions of glyoxal in lipid peroxidation of linoleic acid by the ligninolytic enzyme, manganese peroxidase Takashi Watanabe1, Nobuaki Shira

Production and chemiluminescent free radical reactions of glyoxal in lipid peroxidation of linoleic acid by the ligninolytic enzyme,

manganese peroxidase

Takashi Watanabe1, Nobuaki Shirai2, Hitomi Okada1, Yoichi Honda1and Masaaki Kuwahara1

1 Laboratory of Biomass Conversion, Wood Research Institute, Kyoto University, Gokasho, Uji, Japan;2Industrial Research Center of Shiga Prefecture, Ritto, Kamitoyama, Japan

Glyoxal is a key compound involved in glyoxal oxidase

(GLOX)-dependent production of glyoxylate, oxalate and

H2O2by lignin-degrading basidiomycetes In this paper, we

report that glyoxal was produced from a metabolite of

ligninolytic fungi, linoleic acid, by manganese peroxidase

(MnP)-dependent lipid peroxidation In the absence of the

parent substrate of linoleic acid, the dialdehyde was

oxidized by MnP and Mn(III) chelate to start free radical

reactions with emission of chemiluminescence at 700 –

710 nm The spectroscopic profile of the light emission is

distinguishable from (a) singlet oxygen, (b) triplet carbonyls

from dioxetane and a-hydroxyperoxyl radicals, and (c) biacyl triplet formed by the coupling of two acyl radicals The photon emission of glyoxal by MnP was activated by co-oxidation of tartrate The MnP-dependent oxidation of glyoxal in tartrate buffers continued for 10 days without addition of exogenous H2O2 The importance of these results is discussed in relation to the free radical chemistry

of lignin biodegradation by wood rot fungi

Keywords: Manganese peroxidase; lipid peroxidation; Ceriporiopsis subvermispora; acyl radical

Lignin biodegradation by white rot fungi is an extracellular

chemical event generating free radicals Lignin-degrading

enzymes, lignin peroxidase (LiP), manganese peroxidase

(MnP) and laccase (Lac), play a key role in generating free

radicals from lignin and oxidizable fungal metabolites such

as oxalate, glyoxylate, malonate, hydroquinones and aryl

alcohols Due to the participation of peroxidases in the

lignin breakdown, a supply of hydrogen peroxide is essential

to drive the extracellular enzymatic process So far, several

oxidases have been proposed as the enzymes which carry

out this task The finding that glyoxal and glyoxal oxidase (GLOX) are secreted by white rot fungi strongly suggests that the GLOX system plays a key role in the extracellular

H2O2 production [1 – 6] As GLOX is activated by peroxidases, the peroxidase-dependent lignin-degradation can be controlled by the combination of GLOX and its substrate, glyoxal [2,7] Thus, the importance of glyoxal oxidation in wood decay has been recognized However, little is known about the biosynthetic route for the extra-cellular production of glyoxal by wood rot fungi In this paper, we first report that a ligninolytic enzyme, MnP, is able

to catalyze formation of glyoxal from a metabolite of wood rot fungi, linoleic acid [8], by lipid peroxidation The glyoxal produced by MnP can be converted to glyoxylate and oxalate by GLOX [6] and these carboxylic acids are further oxidized by MnP or LiP/VA to yield O2†– and

CO2†–, which in turn reduce free radicals and transition metals like Fe(III) [9 – 12] Thus, the present result highlights the new roles of MnP-dependent lipid peroxi-dation in free radical chemistry of wood rot fungi

In lipid peroxidation of USFAs, it has been reported that Mn(II) reacts with a chain-carrying radical, peroxyl radical (LOO†), to terminate the chain reactions [13,14] This raises the question of how the MnP-lipid system generates free radicals in the presence of antioxidant, Mn(II) Recently, we reported that the chain-braking antioxidative activity of Mn(II) is suppressed by regeneration of free radicals by breaking down of LOOH with MnP [15] In this process, we found that acyl radicals were predominantly formed This suggests that hydrogen abstraction from aldehydes is involved in the major chain propagation reactions of the MnP-dependent lipid peroxidation The observation of acyl radicals in the MnP/lipid system prompted us to analyze whether MnP can directly oxidize the aldehyde intermediate in order to carry chain-reactions

Correspondence to T Watanabe, Laboratory of Biomass Conversion,

Wood Research Institute, Kyoto University, Gokasho, Uji, Kyoto

611-0011, Japan, Fax: 181 744 38 3600,

E-mail: twatanab@kuwri.kyoto-u.ac.jp

Enzymes: manganese peroxidase (EC 1.11.1.13); lipoxygenase

[linoleate:oxygenoxidoreductase (EC 1.11.13)]; glyoxal oxidase

(EC 1.2.3.-).

(Received 8 May 2001, revised 24 September 2001, accepted

27 September 2001)

Abbreviations: O 2 † – , superoxide anion; CO 2 † – , formate anion

radical; MnP, manganese peroxidase; LiP, lignin peroxidase;

HRP, horseradish peroxidase; 13(S)-HPODE,

13(S)-hydroperoxy-9Z,11E-octadecadienoic acid; SFA, saturated fatty

acid; USFA, unsaturated fatty acid; 2,6-DMP, 2,6-dimethoxyphenol;

ESR, electron spin resonance; MDA, malondialdehyde; MSTFA,

N-methyl-N-trimethylsilyltrifluroacetamide; DFB, decafluorobenzene;

GLOX, glyoxal oxidase, TBARS, thiobarbituric acid reactive

substances; PFBHA, O-(2,3,4,5,6-pentafluorobenzyl)hydroxylamine

hydrochloride; PFBO, pentafluorobenzyl oxime; CH 3 CN, acetonitrile;

MeOH, methyl alcohol; EtOH, ethyl alcohol; DM, n-dodecyl

b-maltoside; DHMA, dihydroxymaleic acid; EI/GC/MS, electron

ionization-gas chromatography-mass spectrometer; PAH, polycyclic

aromatic hydrocarbon.

without the aid of the other oxidizable substrates We now

report the formation and chemiluminescent chain reactions

of glyoxal in MnP-dependent lipid peroxidation of linoleic

acid

M A T E R I A L S A N D M E T H O D S

General methods

Manganese (II) sulfate and 1,2,3-trimethoxybenzene,

decafluorobenzene, 1-dodecanal, 1-decanal, 2,4-nonadienal,

1-hexanal, 1-nonanal, 1-pentanal, 1-octanal, 1-butanal,

glyoxlic acid, glycol aldehyde, glyoxal were obtained

from Wako Pure Chemical Industries (Tokyo, Japan)

trans,trans-2,4-Decadienal, cis-4-decenal was obtained from

Aldrich Chemical Company (Milwaukee, USA)

trans-2-Hexenal, 1-undecanal, 1-heptanal, trans-2-nonenal,

1-tride-canal, 2-butanone, 3-buten-2-one, 3-pentanone, 2-pentanone,

2-heptanone, 2-hexanone, 2-octanone was obtained from

Tokyo Kasei Kogyo (Tokyo, Japan) Linoleic acid was

purchased from Nacalai Tescque (Kyoto, Japan) The linoleic

acid was purified by passing through a Sep-PakTMCN Light

cartridge (Waters, Milford, MA, USA) After dissolving in

n-hexane, the eluent from the cartridge was evaporated with a

gentle stream of N2 gas Milli-QTM water was used

throughout the experiments All of the chemicals used were

of analytical reagent grade

13(S)-Hydroperoxy-9Z,11E-oc-tadecadienoic acid [13(S)-HPODE] was prepared as

described previously [15] Malondialdehyde (MDA) was

synthesized as described previously [16]

Enzyme preparation

Crude MnP from Ceriporiopsis subvermispora FP-90031

was collected from 7-day-old cultures grown on a wood

medium composed of beech wood (5 g), glucose (0.7 g) and

peptone (0.7 g) at 28 8C The culture filtrate was dialyzed

against 20 mM sodium succinate buffer (pH 4.5) The

dialyzate was concentrated by ultrafiltration, precipitated

with (NH4)2SO4 and then purified by gel filtration on

Superdex 75 PG (1.6  60 cm, Amersham Pharmacia

Biotech, Sweden) using 20 mM sodium succinate buffer

containing 0.1MNaCl as an eluent Fractions showing MnP

activities were collected, and desalted with Centriprep

YM-30 (cut off, 30,000, Millipore, USA) MnP was further

purified by preparative IEF as described previously [15]

[pI 3.40, Reinheitzahl (RZ, A at lmax/A 280) value: 3.0,

1.0 U ¼ 8.75  10211mol] Low molecular mass

com-pounds were removed by successive washings with

Milli-QTMwater with a Centricut N-10 ultrafiltration concentrator

(cut off, 10 000, Kurabo, Japan) before use For the time

course experiments of aldehyde production, the enzyme

purified on Superdex 75 PG was desalted with distilled

water in Centricut N-10 and used without further

purification (15 U:mL21) Laccase activity in the partially

purified fraction was below 0.02 U:mL21 Glyoxal oxidase

activity was not found in all the enzyme preparations

Enzyme assay

MnP activity was measured with 2,6-DMP The reaction

mixture contained 0 2 mM 2,6-DMP, 0 5 mM MnSO4,

0 1 mMH O, 25 mMsodium tartrate buffer (pH 3 0) and

the enzyme solution Reactions were started by adding H2O2 and were quantified by monitoring the initial rate of increase in absorbance at 470 nm in the presence and absence of manganese One unit of enzyme activity is defined as the amount of enzyme that oxidizes 1 mmol of 2,6-DMP in 1 min Laccase activity was measured with 2,6-DMP under the same conditions but without

H2O2 Lipoxygenase activity was measured by O2uptake in

a reaction system containing 1 5 mM linoleic acid, 1 mM n-dodecyl b-maltoside (DM) and 20 mM Tris/HCl buffer (pH 9 0) One unit of lipoxygenase activity is defined as the amount of enzyme that absorbs 1 mmol of O2in 1 min GLOX activity was measured by O2 uptake in a reaction system containing 3 mMglyoxal in 20 mMsodium tartrate (pH 3 0), acetate (pH 4 5) or phosphate (pH 6 0) buffers

Electron ionization/gas chromatography/mass spectrometetry (EI/GC/MS) analysis of oxidation products by MnP

Linoleic acid and aldehydes were reacted with 250 mU of the purified MnP, 0.5 mMof Mn(II) and 50 mM of H2O2at

20 8C for 1 – 24 h in 10 mM acetate, formate, lactate and tartrate buffers (pH 4.5) After the reaction, 0.5 mL of aqueous PFBHA (0.05M, 200 mL) was added and reacted at

35 8C for 0.5 h [17] To this solution, 10 mL of a 10-mM methanol solution of decafluorobenzene (DFB) and a drop of 18-N-sulfuric acid were added and the mixture was partitioned between n-hexane and H2O twice The hexane layer was dried over Na2SO4, evaporated with a gentle stream of N2gas and directly injected into an EI/GC/

MS system The EI/GC/MS analysis was done with a Shimadzu QP-5050 A GC/MS with ionization energy of

70 eV on CP-Sil-8 (50 m  0.25 mm internal diemeter, Chrompack, Netherlands) using helium as a carrier gas The column oven temperature was raised from 80 8C to 250 8C

at 5 8C:min21, and maintained at 250 8C for 20 min The time course of glyoxal production by MnP was analyzed as described above after the reaction with and without linoleic acid in formate and tartrate buffers EI/GC/MS analyses of authentic aldehydes and ketones were carried out using a 0.6-mMmethanol solution after derivatization with PFBHA under the conditions described above Tetramethylsilation

by N-methyl-N-trimethylsilyltrifluroacetamide (MSTFA) was carried out as described previously [18]

Chemiluminescence measurements Chemiluminescence was measured by an ultra-high sensi-tive photon counter (ARGUS-50/VIM, Hamamatsu Photo-nics, Hamamatsu, Japan) equipped with a charge-coupled device (CCD) camera connected with an image intensifier and ARGUS-50 image processor The wavelength range of the detector was 350 – 650 nm, 512  483 pixels, and the noise count was 0.15 c.p.s The reactions were carried out in

a cuvette for a 96-well microplate reader The conditions for each experiment are described in the figure legends Inactivation of MnP was carried out by heating the MnP

in a boiling water bath for 10 min The chemiluminescence spectra were measured by a simultaneous multiwavelength analyzer CLA-SP2 (Tohoku Electronic Industries Co Ltd, Sendai, Japan) with an

incident slit width of 1.0 mm The wavelength range of the

spectrometer was 370 – 820 nm Experimental conditions

are described in the legend of each figure

R E S U L T S

Formation of glyoxal in the reaction of linoleic acid

with MnP

Lipid peroxidation by MnP is a free radical process capable

of decomposing recalcitrant PAH and nonphenolic lignin

model compounds [19 – 21] We previously reported that the

oxidation of linoleic acid by MnP produced acyl radicals in

both tartrate and acetate buffers [15] The formation of acyl

radicals strongly suggests that hydrogen abstraction from

aldehyde [22,23] is involved in the oxidative process To

analyze the aldehydes formed by this reaction, linoleic acid

was reacted with MnP for 19 h at 20 8C in sodium acetate,

formate, lactate and tartrate buffers and the oxidation

products were analyzed by EI/GC/MS after derivatization

to pentafluorobenzyloxims (PFBO) with PFBHA [17] EI/

GC/MS analysis of the reaction products and authentic 19

aldehydes and seven ketones demonstrated that glyoxal,

1-hexanal and 1-pentanal were formed from linoleic acid

by MnP in any of the buffer systems (Fig 1) Syn and

anti-isomers of these PFBO derivatives were separated on the GC/MS column The mass spectrum of PFBO derivatives of glyoxal formed from linoleic acid is shown

in Fig 2, together with that of authentic standard MDA, a major peroxidation product derived from polyunsaturated fatty acids was not detected in the reaction products of MnP

in contrast to the oxidation of linoleic acid by xantine/ xanthinoxidase/Fe(II) [24] The mass fragments of PFBO derivatives characteristic to saturated aldehyde (m/z 239), 2-enal (m/z 250), 2,4-dienal (m/z 276) and saturated 2-ketones (m/z 72) [25], were not observed in the spectra

of unidentified carbonyl compounds, indicating that the MnP/Mn(II)/lipid system proceeds by complex radical reactions involving the formation of unusual carbonyl species Tetramethylsilation with MSTFA did not change the mass chromatogram at m/z 181 that originates from C – O bond cleavage products of pentafluorobenzyl oxime [26] (data not shown)

The reactions of MnP in four different buffers clearly demonstrate that the formation of glyoxal was significantly stimulated by the presence of tartrate Therefore, the reaction was carried out with and without linoleic acid in sodium formate and tartrate buffers (Figs 1 and 3) GC/MS analysis demonstrated that glyoxal was explosively produced after 6 h in tartrate buffer containing linoleic

Fig 1 Mass chromatograms of PFBO derivatives of products of lipid peroxidation by C subvermipora MnP and soybean lipoxygenase at m/z 181 (A) Products of the oxidation of linoleic acid by MnP in sodium acetate buffer for 19 h The reaction system (500 mL) contained 3 m M

linoleic acid, 500 m M MnSO 4 , 50 m M H 2 O 2 , 0.02% of Tween 20, 250 mU of purified MnP and 10 m M sodium acetate buffer (pH 4.5) (B) As (A) but

10 m M sodium formate buffer (pH 4.5) was used instead of acetate buffer (C), As (A) but 10 m M sodium lactate buffer (pH 4.5) was used instead of acetate buffer (D) As (A) but 10 m M sodium tartrate buffer (pH 4.5) was used instead of acetate buffer (E) As (B) but the reaction was carried out without addition of linoleic acid (F) As (D) but the reaction was carried out without addition of linoleic acid (G) Products of the oxidation of linoleic acid with soybean lipoxygenase Linoleic acid (3 m M ) was reacted with soybean lipoxygenase (10 U) in 40 m M Tris/HCl buffer (pH 9.0) containing 0.02% of Tween 20 for 24 h at 20 8C (H) Products of the oxidation of 13(S )HPODE by MnP in sodium lactate buffer (pH 4.5) for 3 h The reaction system contained 3 m M 13(S )HPODE, 500 m M MnSO 4 , 50 m M H 2 O 2 , 0.02% of Tween 20, MnP (250 mU) and 10 m M sodium lactate buffer (pH 4.5).

acid However, direct formation of glyoxal from tartrate was

also observed In formate buffer, the production of glyoxal

was dependent on the presence of linoleic acid The same

results were obtained with lactate and acetate buffers (data

not shown) In contrast to the oxidation of linoleic acid,

oxidation of 13(S )HPODE with MnP selectively produced

1-hexanal for 1 – 3 h (Fig 1H) No PFBO-derivatives were

detected after the prolonged reaction of 13(S )HPODE Thus

it was found that the formation of glyoxal was not catalyzed

by the direct oxidation of 13(S )HPODE with MnP

Oxidation of linoleic acid with soybean lipoxyegnase

produced 1-hexanal and 1-pentanal (Fig 1G)

Emission of chemiluminescence in lipid peroxidation

The chemiluminescence detector is a powerful tool for

analyzing the oxidation of aldehydes due to its high

sensitivity and emission spectra characteristic to chemically excited species Therefore, oxidation of aldehydes and linoleic acid by MnP was analyzed by a chemiluminescence detector, in comparison with light emission by lipoxygenase and the Fenton reaction (Fig 4) Lipoxygenase is an enzyme that abstracts hydrogen from the bis-allylic position of unsaturated fatty acids containing cis,cis-1,4-pentadienyl moiety In the reaction with linoleic acid, the fatty acid is oxidized to yield a pentyl radical [27] and 12-oxododecyl-cis-9-enoic acid [28] via b-scission of hydroperoxide intermediates, leading to production of 1-hexanal [29] and 1-pentanal as shown in Fig 1G When linoleic acid was oxidized by soybean lipoxygenase, emission of chemilumi-nescence was close to the background level, both in the presence and absence of Fe(II) In the Fenton system, chemiluminescence was also below the background level, except for a weak emission of light from linoleic acid after 2 days (Fig 4)

In contrast to these oxidation systems, reactions of glyoxal with MnP in tartrate buffer emitted strong chemilumines-cence As shown in Figs 5 and 6, intensive light emission was observed immediately after the reaction started The photon emission reached a maximum (35 000 counts:h21) within 30 min, and then decreased, but chemiluminescence

of < 9000 counts:h21 was observed even after 1 h In lactate, formate and acetate buffers, the photon emission was also observed within 30 min but the intensity was much lower than that of the tartrate system In the tartrate system, the photon emission continued for 10 days, both in the presence and absence of exogenous H2O2 added initially (Fig 6) The photon emission from glyoxal was dependent

on the presence of Mn(II) and active enzyme However, it was found that the emission of chemiluminescence continued for around 10 days when the reaction was started without addition of glyoxal This can be explained by the in situ formation of glyoxal from tartrate with MnP (Fig 1,3)

In the MnP-catalyzed oxidation of linoleic acid and the other aldehydes, the light emission was not observed when Mn(II) was omitted from the reaction system (data not shown) When linoleic acid and seven different aldehydes were reacted with Mn(III)–tartrate complex, strong light emission was observed in the reaction system with glyoxal (Fig 7) The maximum photon emission intensity from glyoxal reached 12 000 counts:h21 The photon emission was also

Fig 2 Mass spectra of PFBO derivatives of glyoxal formed by the

oxidation of linoleic acid with MnP (A) and authentic standard (B).

(A) Glyoxal formed by the oxidation of linoleic acid with MnP for 19 h.

The reaction system (500 mL) contained 3 m M linoleic acid, 500 m M

MnSO 4 , 50 m M H 2 O 2 , 0.02% of Tween 20, MnP (250 mU) and 10 m M

sodium acetate buffer (pH 4.5) (B) Authentic standard of glyoxal.

* 1/10 of the original signal intensity.

Fig 3 Time course of glyoxal formation by MnP (A) Glyoxal formed by the reaction of linoleic acid with MnP in sodium tartrate buffer The reaction system (500 mL) contained 3 m M linoleic acid, 500 m M MnSO 4 , 50 m M H 2 O 2 , 0.02% of Tween 20, MnP (250 mU) and 10 m M sodium tartrate buffer (pH 4.5) (B) As (A) but linoleic acid was omitted (C) As (A) but 10 m M sodium formate buffer (pH 4.5) was used instead of sodium tartrate bufer (D) As (C) but linoleic acid was omitted.

Fig 4 Time course of light emission during oxidation of linoleic acid by soybean lipoxygenase (I) and the Fenton reaction (II) (I): (A) The reaction system (200 mL) contained

4 m M linoleic acid, 10 U of lipoxygenase, 0.05%

of Tween 20, 10 m M Tris/HCl buffer (pH 9.0) (B)

As (A) but lipoxygenase was omitted (C) As (A) but 0.5 m M FeSO 4 was added II: (A) The reaction system (200 mL) contained 4 m M linoleic acid, 0.1 m M FeSO 4 , 0.2 m M H 2 O 2 , 0.05% of Tween 20 (B) As (A) but glyoxal was added instead of linoleic acid (C) As (A) but trans-2-nonenal was added instead of linoleic acid (D) As (A) but 1-dodecanal was added instead of linoleic acid (E)

As (A) but 1-hexanal was added instead of linoleic acid (F) As (A) but 2,4-nonadienal was added instead of linoleic acid (G) As (A) but MDA was added instead of linoleic acid (H) As (A) but linoleic acid was omitted.

Fig 5 Chemiluminescence emitted by the oxidation of aldehydes and linoleic acid with MnP in sodium tartrate buffer (A) The reaction system (200 mL) contained 4 m M linoleic acid,

250 mU of MnP, 500 m M MnSO 4 , 0.2 m M H 2 O 2 , 0.05% of Tween 20 and 10 m M sodium tartrate buffer (pH 4.5) (B) As (A) but glyoxal was added instead of linoleic acid (C) As (A) but

trans-2-nonenal was added instead of linoleic acid (D) As (A) but 1-dodecanal was added instead of linoleic acid (E) As (A) but 1-hexanal was added instead of linoleic acid (F) As (A) but

2,4-nonadienal was added instead of linoleic acid (G) As (A) but MDA was added instead of linoleic acid (H) As (A) but linoleic acid was omitted Inset shows the time course of the reactions (A – H) during 2.5 h.

Fig 6 Chemiluminescence emitted by the oxidation of glyoxal with MnP (I): (A) The reaction system (200 mL) contained 4 m M glyoxal,

250 mU of MnP, 500 m M MnSO 4 , 0.2 m M H 2 O 2 , 0.05% of Tween 20 and 10 m M sodium acetate buffer (pH 4.5); (B) As in (A) but 10 m M sodium formate buffer (pH 4.5) was used instead of sodium acetate bufer (C) As (A) but 10 m M

sodium tartrate buffer (pH 4.5) was used instead

of sodium acetate bufer (D) As (A) but 10 m M

sodium lactate buffer (pH 4.5) was used instead

of sodium acetate buffer.

(II): (A) The reaction system (200 mL) contained

4 m M glyoxal, 250 mU of MnP, 500 m M MnSO 4 , 0.2 m M H 2 O 2 , 0.05% of Tween 20 and 10 m M

sodium tartrate buffer (pH 4.5) (B) As (A) but MnSO 4 was omitted (C) As (A) but H 2 O 2 was omitted (D) As (A) but glyoxal was omitted (E)

As (A) but inactivated MnP was used instead of native MnP.

observed with MDA, trans-2-nonenal and linoleic acid, but

the intenisity was less than 1/10 of that observed in the

oxidation of glyoxal Light emissions from 1-dedecanal,

1-hexanal, 2,4-nonadienal were almost at the same level as

that observed without addition of linoleic acid/aldehyde No

photon emission was observed in the reactions of these

oxidizable substrates with Mn(II) – tartrate complex (data

not shown) These results demonstrate that MnP catalyzes

oxidation of Mn(II) to Mn(III), which in turn reacts with

glyoxal to generate electronically excited species

Co-oxida-tion of tartrate is essential to carry the chemiluminescent

chain reactions over several days

Figure 8 shows emission spectra obtained by glyoxal

oxidation with (A) Mn(III) – lactate complex, and (B) MnP/

Mn(II)/H2O2in tartrate buffer The spectra showed a broad

single peak with emission maxima at 700 and 710 nm,

respectively Figure 2C is the chemiluminescence spectrum

of singlet oxygen formed by the reaction of HClO– with

H2O2 The spectrum showed two sharp emission maxima at

634 and 704 nm as reported [30] In the spectra obtained by

the glyoxal oxidation by MnP and Mn(III) – lactate, no

shoulder peaks of the dimol emission of singlet oxygen was

observed

D I S C U S S I O N

Formation and oxidation of glyoxal in lipid peroxidation

of linoleic acid by MnP

It has been widely recognized that selective white rot fungi

such as Ceriporiopsis subvermispora can delignify wood

without penetration of their extracellular enzymes into wood

cell walls Therefore, there is increasing interest in the roles

of low molecular mass compounds that generate free

radicals capable of decomposing lignin at a site far from

enzymes Lipid peroxidation by manganese peroxidase

(MnP) is one candidate for this system because diffusible

Mn(III) chelate can react with lipid and lipid hydroperoxides

to generate free radicals [15] When C subvermispora was cultivated on wood meal medium, the fungus produced saturated fatty acids (SFAs) and unsaturated fatty acids (USFAs) including linoleic acid at an incipient stage of cultivation and consume them with concomitant formation

of lipid hydroperoxide and TBARS during prolonged cultivation [8] In the lipid peroxidation process, titres of MnP reached a maximum around day 4 and then gradually decreased, coincident with the peroxidation of the fatty acids Thus, accumulated data supports the involvement of MnP-dependent lipid peroxidation in wood decay by white rot fungi

With regard to the radicals produced in the lipid peroxidation by MnP, we reported that MnP oxidized linoleic acid to generate acyl radicals in acetate and tartrate buffers in the presence of Mn(II) [15] The formation of acyl radicals strongly suggests that hydrogen abstraction from aldehydes is involved in the chain propagation cycle of the MnP-dependent lipid peroxidation Therefore, aldehydes formed by the MnP/linoleic acid/Mn(II)/H2O2 reactions were analyzed by EI/GC/MS after derivatization to PFBO (Figs 1 – 3) The GC/MS analysis demonstrated that oxidation of linoleic acid with MnP produced glyoxal, 1-hexanal and 1-pentanal Time course experiments of the MnP reactions showed that glyoxal was not formed on initiation of the lipid peroxidation but after 6 h (Fig 3) In contrast to the oxidation of linoleic acid, the reaction of MnP with 13(S)-HPODE selectively produced 1-hexanal, indicating that the glyoxal formation is not catalyzed by the direct breakdown of lipid hydroperoxide with MnP and Mn(III) chelates

In wood decay, a supply of extracellular hydrogen peroxide is essential to initiate peroxidase-dependent free radical processes An extracellular oxidase, GLOX, has been identified from wood decay fungi and is considered as an enzyme that catalyzes extracelular H2O2 production However, little is reported about the biosynthetic pathway

of glyoxal in wood rot fungi In 1994, Hammel et al

Fig 7 Chemiluminescence emitted by the

oxidation of aldehydes and linoleic acid with

Mn(III) – tartrate complex (A) The reaction

system (200 mL) contained 4 m M linoeic acid,

0.05% of Tween 20, and 2.5 m M Mn(III) – tartrate.

A Mn(III) – tartrate solution (10 m M ) was prepared

by dissolving 0.1 m mol of Mn(III) – acetate in

10 mL of 0.1 M sodium tartrate buffer (pH 4.5).

The reaction was initiated by adding 50 mL of this

solution Therefore, the final concentration of

tartrate in the reaction system was 25 m M (B) As

(A) but glyoxal was added instead of linoleic acid.

(C) As (A) but trans-2-nonenal was added instead

of linoleic acid (D) As (A) but 1-dodecanal was

added instead of linoleic acid (E) As (A) but

1-hexanal was added instead of linoleic acid (F)

As (A) but 2,4-nonadienal was added instead of

linoleic acid (G) As (A) but MDA was added

instead of linoleic acid (H) As (A) but linoleic acid

was omitted.Time course of the photon emission

from glyoxal is shown separately from that of the

other oxidizable compounds due to the difference

of emission intensity.

reported that lignin peroxidase deomposed a b-O-4 lignin

model compound with production of glycol aldehyde, a

substrate of GLOX [6] The glycol aldehyde formed by this

process was converted to oxalate with the production of 2.8

equivalent of H2O2 Therefore, they proposed a pathway

producing oxalate from the b-O-4 lignin model compound

via glyoxal and glyoxylate However, there has been no

direct evidence for the glyoxal formation from lignin by the

LiP/GLOX system The finding of glyoxal formation by MnP-dependent lipid peroxidation indicates that MnP and Mn(III) chelate part in the formation of glyoxal, leading to the enzymatic production of glyoxylate, oxalate and H2O2

by GLOX Mn(III) stabilized by the former two carboxylic acids can diffuse into the wood cell wall region At the same time, glyoxylate and oxalate are oxidized by Mn(III) to produce CO2†–

and O2†–

[11,12] The same reaction was also catalyzed by LiP/VA [9,10] Due to the high reduction potential of CO2†–, the radical catalyzes reduction of Fe(III) [12] and reductive dehalogenation of recalcitrant aromatic halides [31] O2†– catalyzes oxidation of Mn(II) and reduction of Fe(III) in addition to disproportionation yielding H2O2 A combination of the iron reduction and

H2O2 formation generates hydroxyl radicals Thus, MnP-dependent lipid peroxidation provides the substrate of GLOX to produce active oxygen species in combination with redox cycle of transition metals

Oxidation of glyoxal by MnP

In lipid peroxidation involving aldehyde oxidation, it has been postulated that acyl radicals are formed from aldehydes

by hydrogen abstraction with radicals (X†) [22] or transition metals [23] according to:

M31ðM21Þ 1 RCHO ! M21ðM1Þ 1 RCO† 1 H1 ð2Þ With regard to the light emission from acyl radicals, four different pathways can be discussed (Fig 9) As shown in Fig 9 (pathway 2) two acyl radicals can recombine to produce a biacyl triplet [32] The light emission reported in excited biacyl compounds like biacetyl (l max at 515 and

560 nm) [32] is different from the emission spectra observed

in the MnP reactions a-Oxidation of aldehydes via a dioxetane intermediate also produces excited triplet carbonyls (Fig 9, pathway 1) but the absorption maximum

of the light emission is in the range of l max 450 – 550 nm [28,32] Singlet oxygen can be formed by disproportionation

of two a-hydroxyperoxyl radicals (Fig 9, reaction 4) However, there are no shoulder peaks of the dimol emission from singlet oxygen (l max 634 and 703 nm) [30] in the spectrum of glyoxal oxidation by MnP (Fig 8), indicating that 1O2 is not the major excited species formed by the MnP/glyoxal system The other possible route for

Fig 8 Chemiluminescence spectra of (A) oxidation of glyoxal by MnP in tartrate buffer (B) oxidation of glyoxal by Mn(III) – lactate complex and (C) singlet oxygen formed by the reaction of ClO –

with H 2 O 2 (A) The reaction system (500 mL) contained 3 m M glyoxal,

250 mU of MnP, 500 m M MnSO 4 , 50 m M H 2 O 2 , 0.02% of Tween 20 and 10 m M sodium tartrate buffer (pH 4.5) (B) The reaction system (500 mL) contained 3 m M glyoxal, 0.02% of Tween 20, and 2 m M

Mn(III) – lactate A Mn(III) – lactate solution (10 m M ) was prepared by dissolving 0.1 m mol of Mn(III) – acetate in 10 mL of 0.1 M sodium lactate buffer (pH 4.5) The reaction was initiated by adding 100 mL of this solution Therefore, the final concentration of lactate in the reaction system was 20 m M (C) The reaction was started by adding 1 mL of 30% H 2 O 2 and 3 mL of 10% NaClO solution Scanning time for (A) (B) (C) were 20, 15, and 5 min, respectively.

chemiluminescence emission from acyl radical is a

forma-tion of triplet carbonyls from a-hydroxyperoxyl radicals

(Fig 9- [3]) that has been reported in the oxidation of

aetaldehyde with xantine oxidase [33] However, the

emission maximum of the chemiluminescence by this

mechanism was lower than 500 nm [33] (Fig 9) Thus, the

MnP-dependent light emission from glyoxal at 700 nm is a

new chemical event difficult to explain by the excited

species from acyl radicals reported before

As shown in Fig 8, the reaction of Mn(III) – lactate with

glyoxal emitted the chemiluminescence similar to that

observed in the reactions of MnP Therefore, it can be

concluded that Mn(III) chelate is capable of abstracting

hydrogen from glyoxal to form the electronically excited

species, which spontaneously decay to emit the

chemilumi-nescence As shown in Fig 1, peroxidation of linoleic acid

with MnP produced glyoxal However, the

chemiclumines-cence from linoleic acid was much less intensive than that of

the direct oxidation of glyoxal with MnP This suggests that

the excited species from glyoxal react with peroxidation

intermediates from linoleic acid, leading to quenching of the

excited compound [34]

Oxidation of tartrate by MnP

In this study, we also found that tartrate is oxidized by MnP

and Mn(III) chelates in aqueous solutions to produce glyoxal

with emission of chemiluminescence Although tartrate is

not a metabolite of ligninolytic fungi, this carboxylic acid is

widely used in studies on MnP For tartrate, unlike oxalate

and malonate, there has been no report of MnP-catalyzed

degradation For instance, the ratio of H2O2consumption vs

oxidation of Mn(II) by MnP in tartrate buffer is reported to

be nonstoichiometric due to reduction of H2O2 to O2 by

Mn(III) – tartrate complex [35,36] However, no special

attention was paid to the oxidation of tartrate itself in these

studies This may be due to the understanding that the

reactivity of tartrate is too low to be involved in the free

radical reactions by Mn(III) For instance, Perez reported

that veratryl alcohol oxidation by LiP is not affected by the

presence of tartrate in the presence or absence of Mn(II) and

Mn(III) [37] More recently, Collins reported that the rate

of 2,20-azinobiz(3-ethylbenzo-6-thiazolinesulfonic acide)

(ABTS†1) reduction is enhanced by the presence of

malonate, glyoxylate and oxalate but no stimulating effects

of tartrate on the ABTS†1reduction was observed [38] In contrast, the results obtained in the present study clearly indicate that tartrate itself was oxidized by MnP to produce glyoxal (Figs 1 – 3), thereby assisting chain reactions of the aldehyde accompanied by photon emission (Fig 7,8) In lipid peroxidation of linoleic acid by MnP, the consecutive formation of aldehydes and acyl radicals was observed in acetate and formate buffers as well as in tartrate buffer Therefore, we propose that the enzymatic process produces counterpart compounds like tartrate to assist the chain propagation reactions of acyl radicals in combination with redox cycle of Mn(II)/Mn(III)

In conclusion, the first evidence for the production of glyoxal from linoleic acid in MnP-dependent lipid peroxi-dation has been presented Glyoxal formed by this process can be used as a substrate of GLOX and MnP to participate

in the extracellular free radical reactions of wood rot fungi

In addition to the interest on lignin biodegradation, the analysis of manganese-dependent glyoxal oxidation associ-ated with tartrate oxidation will lead to the understanding of cellular injury caused by the carcinogenic aldehyde in the presence of catalytic amount of manganese

A C K N O W L E D G E M E N T S

This work was supported by a Grant-in-Aid for Scientific Research (B) from the Ministry of Education, Science, Sports and Culture, Japan We are grateful to Ms M Nakagawa for technical assistance in the analysis

of aldehydes We also thank Dr Rie Yamada, Tohoku Electoric Co Ltd, for the measurement of chemiluminescence spectra.

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