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Some Biochemical properties of polyphenoloxidase from spearmint (Mentha arvensis)

Abstracts

Polyphenoloxidase (PPO; EC 1.14.18.1) extracted from Mentha arvensis leaves was isolated by (NH4)2SO4 precipitation and extensive dialysis. Its optimum pH and temperature varied with the substrate. The PPO showed activity with various diphenols. Km values were found 0.825, 0.928 and 7.41mM for caffeic acid, 4-methylcatechol and catechol, respectively. On heat-inactivation, half of the activity was lost after 60 and 15 sec at 70 and 75ºC, respectively. Measuring of residual activity showed a stabilizing effect of sucrose at various temperatures with activation energy (Ea) for inactivation increasing with sucrose concentration from 0 to 40% (w/w). Ea values of 78.13; 80.37; 82.79 and 81.00 kJ/Mol were found for 0, 15; 30 and 40% sucrose, respectively. PPO was inhibited by ascorbic, benzoic, cinnamic, ferulic, p-coumaric, protocatechuich acids, sodium metabisulfite, pyrogallol and resorcinol. The Ki values showed that ascorbic acid was the most effective inhibitor. The type inhibition was determined for each inhibitor.

polyphenoloxidase; Mentha arvensis; characterization; heat inactivation; inhibitors


Polifenoloxidase (PPO, EC 1.14.18.1) extraída de folhas de Mentha arvensis foi isolada por precipitação com (NH4)2SO4 e diálise extensiva. Seu pH e temperatura ótimos variaram com o substrato. A PPO apresentou atividade com vários difenóis. Valores de Km foram 0,825; 0,928 e 7,41 mM para ácido caféico, 4-metilcatecol e catecol, respectivamente. Na inativação térmica, 50% da enzima foi inativada após 60 e 15 segundos a 70 e 75ºC, respectivamente. A medida de atividade residual mostrou um efeito estabilizante de sacarose a várias temperaturas e uma energia de ativação (Ea) para inativação aumentando com a concentração de sacarose de 0 a 40% (p/p). Valores de energias de ativação de 78,13; 80,37; 82,79 and 81,00 kJ/Mol foram encontradas para 0, 15, 30 e 40% de sacarose, respectivamente. A PPO foi inibida pelos ácidos ascórbico, benzóico, cinamico, ferulico, p-cumárico, protocatéquico, além de metabisulfito de sódio, resorcinol e pirogalol. Os valores de Ki mostram que o ácido ascórbico foi o mais efetivo inibidor. O tipo de inibição foi determinado para cada inibidor.


FOOD/FEED SCIENCE AND TECHNOLOGY

Some Biochemical properties of polyphenoloxidase from spearmint (Mentha arvensis)

Valdir Augusto Neves** Author for correspondence: nevesva@fcfar.unesp.br; Douglas Gatte Picchi; Maraiza Aparecida da Silva

Departamento de Alimentos e Nutrição; Faculdade de Ciências Farmacêuticas; Universidade Estadual Paulista; Rodovia Araraquara Jaú Km 1; São Paulo - SP - Brasil

ABSTRACT

Polyphenoloxidase (PPO; EC 1.14.18.1) extracted from Mentha arvensis leaves was isolated by (NH4)2SO4 precipitation and extensive dialysis. Its optimum pH and temperature varied with the substrate. The PPO showed activity with various diphenols. Km values were found 0.825, 0.928 and 7.41mM for caffeic acid, 4-methylcatechol and catechol, respectively. On heat-inactivation, half of the activity was lost after 60 and 15 sec at 70 and 75ºC, respectively. Measuring of residual activity showed a stabilizing effect of sucrose at various temperatures with activation energy (Ea) for inactivation increasing with sucrose concentration from 0 to 40% (w/w). Ea values of 78.13; 80.37; 82.79 and 81.00 kJ/Mol were found for 0, 15; 30 and 40% sucrose, respectively. PPO was inhibited by ascorbic, benzoic, cinnamic, ferulic, p-coumaric, protocatechuich acids, sodium metabisulfite, pyrogallol and resorcinol. The Ki values showed that ascorbic acid was the most effective inhibitor. The type inhibition was determined for each inhibitor.

Key words: polyphenoloxidase; Mentha arvensis; characterization; heat inactivation; inhibitors

RESUMO

Polifenoloxidase (PPO, EC 1.14.18.1) extraída de folhas de Mentha arvensis foi isolada por precipitação com (NH4)2SO4 e diálise extensiva. Seu pH e temperatura ótimos variaram com o substrato. A PPO apresentou atividade com vários difenóis. Valores de Km foram 0,825; 0,928 e 7,41 mM para ácido caféico, 4-metilcatecol e catecol, respectivamente. Na inativação térmica, 50% da enzima foi inativada após 60 e 15 segundos a 70 e 75ºC, respectivamente. A medida de atividade residual mostrou um efeito estabilizante de sacarose a várias temperaturas e uma energia de ativação (Ea) para inativação aumentando com a concentração de sacarose de 0 a 40% (p/p). Valores de energias de ativação de 78,13; 80,37; 82,79 and 81,00 kJ/Mol foram encontradas para 0, 15, 30 e 40% de sacarose, respectivamente. A PPO foi inibida pelos ácidos ascórbico, benzóico, cinamico, ferulico, p-cumárico, protocatéquico, além de metabisulfito de sódio, resorcinol e pirogalol. Os valores de Ki mostram que o ácido ascórbico foi o mais efetivo inibidor. O tipo de inibição foi determinado para cada inibidor.

INTRODUCTION

Polyphenoloxidase (PPO, monophenol, dydhydroxy-L-phenylalanine oxygen oxidoreductase, E.C. 1.14.18.1) is an enzyme that catalyzes the oxidation of mono-, di-and polyhydric phenols to o-quinones. Different names have been associated with this enzyme including tyrosinase, cresolase, catecholase, diphenolase and phenolase. The enzyme is widely distributed on the phylogenic scale and responsible for the deleterious effect of enzymatic browning reactions in foods and other materials. It is well known that browning reactions, initiated by the enzyme, occur generally post-harvest when the tissues are exposed either to stress conditions, to deterioration or during handling, storage and processing (Tomás-Barberán and Espín, 2001). PPO has been extensively studied and characterized in a variety of tissues, as sweet potato (Lourenço et al., 1992) potato and taro (Duangmal and Owusu Apenten, 1999); egg plant (Concellón et al., 2004); palmito (Lourenço et al., 1990); apple (Nicolas et al., 1994); pears (Gauillard and Richard-Forget, 1997); grapes (Rapeanu et al., 2006); herbs (Arslan et al., 1997); tea leaves (Halder et al., 1998); peppermint (Kavrayan and Aydemir, 2001); oregano (Dogan et al., 2005) and artichoke (Aydemir, 2004). Mentha arvensis is the Mentha specie extensively cultivated in Brazil for the industrial and home uses as tea infusion. It has a great number of uses as medicinal crop, refreshing flavouring agent for foods, candy, gum and dental products. To date, there are no studies reported on the isolation and characterization on PPO from M. arvensis leaves. The present study was conducted to obtain information on PPO from this source and describes some properties of the enzyme and the inhibitory effect of various substances.

MATERIALS AND METHODS

Plant material and chemicals

The Mentha leaves were harvested fresh from the botanic garden of Faculty of Pharmaceutical Sciences-UNESP. The leaves were washed with distilled water, dried on filter paper and stored at 4ºC before use. The fresh leaves were weighted and used for the preparation of the enzyme extracts.

Catechol, 4-methylcatechol, ascorbic acid, sodium metabisulfite, mercaptoethanol, DL-DOPA, dethioerythritol, L-tyrosine, Triton X-100, cinnamic, p-coumaric, ferulic, caffeic, protocathechuic, benzoic acid, resorcinol, pyrogallol were obtained from Sigma Chemical Co. (St. Louis, USA). All other chemicals used were analytical reagent grade.

Enzymes extraction and partial purification

Fresh leaves (5g) were grinding in a mortar followed by Ultra-turrax homogenization in 15 ml 0.05 M of phosphate buffer (pH 6.0) containing 0.030 M ascorbic acid, 0.35 M KCl, 0.5% TRITON X-100 and policlar aT (0.1g/g) as phenolic scavengers. The homogenates were filtered through two layers of cheese-cloth and centrifuged at 10.000g for 40 min at 4ºC. (NH4)2SO4 was added to the supernatant to obtain 20-90% saturation with gentle stirring and centrifuged at 10.000g for 40 min at 4ºC. The protein fraction that precipitated was dissolved in 0.05 M of phosphate buffer (pH 7.0), containing 0.030 M ascorbic acid and dialyzed at 4ºC for 22 h against the same buffer containing 0.010 M ascorbic acid. The dialyzed sample was used as the PPO enzyme source in the experiments.

Enzyme assay

PPO activity was determined by measuring the initial rate of quinone formation as indicated by an increase in absorbance at 420 nm at 30ºC for 4methylcatechol (4-methyl-1,2-benzenediol) as substrate (Lourenco et al., 1990). An Ultrospec 2000 (Pharmacia Biotech) spectrophotometer was employed throughout the experiment. The reaction mixture contained 0.002 M 4-methylcathecol, 0.05 M phosphate buffer (pH 6.0), and enzyme solution in a total volume of 3mL in the cuvette. The initial rate of the enzyme-catalysed reaction was a linear function of time for 3 min. In all determinations, PPO activity was assayed in triplicate measurements and one unit was defined as a change of 0.001 absorbance unit per min.

Protein determination

Protein concentration of the various extracts and solutions was determined by the dye-binding method of Bradford (1976) using bovine serum albumin as standard.

Effect of temperature/thermal stability

PPO activity as a function of temperature was determined from 5 to 60ºC. The heat inactivation studies were performed over the range of 50-80ºC. After heating for a given period, the enzyme aliquot was cooled and immediately assayed as described above. To study the effect of additives on heat stability, PPO was incubated in the presence of sugar followed by the determination of the remaining activity. The constant rates (k) for inactivation were determined from the slopes of the time course denaturation according to: log (A/Ao .100) = -(k/2.303)t or ln (A/Ao) = -kt, where Ao is the initial enzyme activity and A is the activity at the time measured. The slopes of these plots were determined by linear regression and the constant rates were calculated by replotting. The apparent activation energies (Ea) were calculated from the slopes of the Arrhenius plots: ln k x 1/T according to the equation ln K = -Ea/RT, where R is the gas constant (8.314 J Mol-1 K-1), T is the temperature in Kelvin. Slopes were calculated by linear regression. The apparent activation energy (Ea) for inactivation was also performed by measuring the reaction rate constant for inactivation at different temperatures in the presence and absence of sucrose as additive. All of the assays were performed in triplicate.

pH optimum and stability

PPO activity as a function of pH was determined using 4-methylcatechol, catechol and caffeic acid as substrates. Phosphate and phosphate-citrate buffer, ranging from pH 3.0 to 8.0 was used at the assays. The pH stability was determined by incubating the enzyme in the above buffer (pH 3.0 to 8.0) for 30 min and at the end of the incubation period, samples were taken and assayed under standard conditions as described above. All of the assays were performed in triplicate.

Substrate specificity and kinetic studies

Michaelis-Menten constant (Km) and maximum reaction velocity (Vmax) of Mentha PPO were determined using various substrates (catechol, 4methylcatechol, caffeic, protocatechuic, cinnamic acids, tyrosine, pyrogallol and resorcinol, in each own wavelength). Data were plotted as 1/V x 1/S concentration according to the method of Lineweaver and Burk (1934). All of the assays were performed in triplicate.

Effect of various inhibitors in the activity

The effect of inhibitors (ascorbic, caffeic, pcoumaric, ferulic, protocatechuic, benzoic acids, resorcinol, pyrogallol, sodium metabisulfite) on PPO activity was measured in the standard reaction medium in the presence and absence of different concentrations of the substances. Using two different concentrations of substrates, PPO activity was assayed at various concentrations of the substances. Values of 1/V x [i] concentration were plotted and the Ki determined according to the method of Dixon (1953). All of the assays were performed in triplicate.

SDS activation

Enzyme extract was incubated with sodium dodecyl-sulphate (SDS) at various concentrations for 5 min, followed by the determination of the enzyme activity as described above. SDS concentrations in the incubation medium were varied from 0.01 to 0.1%.

RESULTS AND DISCUSSION

The extraction of PPO from the leaves of M. arvensis needed the addition of browning inhibitors because the tanning reactions caused partial inactivation of the enzymes and/or also rendered the extract browned. Various compounds were tested in the extraction medium as 2-mercaptoethanol, PEG 6000, dithioeritrithol, metabisulfite. However, some of them inactivated the enzyme or did not interact with phenolics and produced various degree of browning. The higher yields of PPO activity associated with a lower browning was obtained in the pH range of 5.5-7.0, with phosphate buffer 0.05 M containing 0.030 M ascorbic acid, 0.35 M KCl, addition of Policlar aT (0.1g/g) and 0,5% Triton X-100. Since PPO precipitated in a broad ammonium sulfate saturation range (20-90%), followed by extensive dialysis (22 h). This preparation was used as the source of enzyme for the studies. The PPO activity can be assayed in the presence or absence of SDS (Moore and Flurkey, 1990; Nunez-Delicado et al., 2003; Concellón et al., 2004). The effect of SDS in the activation process results from a conformational change due to the binding of a small quantity of SDS to the active site (Moore and Flurkey, 1990, Gauillard and Richard-Forget, 1997). Nunez-Delicado et al. (2003) related a latent form of PPO in persimmon fruit that was optimally activated by the presence of 1 mM SDS; the latent enzyme presented monophenolase and diphenolase activities and in the absence of SDS the enzyme activity increased at acidic pH. Sodium dodecyl sulphate from 0.01 to 0.1% concentration was tested in the assay of mentha PPO, but it did not affect the activity (data not shown). This indicated that the mentha PPO was fully active without the presence of a latent form of the enzyme.

pH optima

Optimum pH for PPO activity with caffeic acid, 4-methylcatechol and catechol as substrates were pH 4.5, 5.0 and 6.5, respectively (Fig 1). However, when using 4-methylcatechol at pH 3.5 and 8.0, the enzyme still retained 15 and 30% of the optima activity. Differences in optimum pH for PPO with distinct substrates have been reported for the enzyme from various sources (Lourenço et al., 1990; Gonzalez et al., 2000; Kavrayan and Aydemir, 2001; Nunez-Delicado et al., 2003; Dogan et al., 2005; Rapeanu et al., 2006). However, for 4-methylcatechol, pH optima of 4.0; 5.7 and 6.5 were found for sweet potato (Lourenco et al., 1992), egg plant (Concellón et al., 2004) and longan fruit (Jiang, Yue-Ming, 1999), respectively.


The effect of temperature on PPO activity

Optimum temperature for PPO activity with caffeic acid and catechol was 30ºC; however, when using 4-methylcathecol as substrate, it was 15ºC (Fig 2). This surprising behavior of the PPO enzyme with the last substrate was confirmed after several repetitions. Heating for 30 min at 30ºC caused no changes in the activity; however, at the higher temperatures, the enzyme was rapidly inactivated. Optimum temperatures for PPO activity in others sources were reported to be between 20 and 40ºC.


The enzyme was reasonably stable at 60ºC and, as expected, the rate of inactivation was higher with increasing temperature (Fig. 3). When exposed to 65ºC, a 65% residual activity was registered for 60 sec, in contrast to 30 and 15 sec at 70 and 75ºC, respectively. The times required for 50% inactivation of PPO activity at 70ºC and 75ºC were 60 and 15 sec, respectively (Fig. 3). The mentha PPO showed a biphasic thermal inactivation behavior to 60, 65 and 70ºC. However, several workers imputed this character non-linear to the formation during the heating of denaturated protein forms and groups of PPO molecule that remained active (Neves and Lourenço, 1998, Hemeda and Klein, 1991, Vamos-Vigyázo, 1981).


Contrary to peroxidases, PPO is not a heat-stable enzyme (Vamos-Vigyázo, 1981). The half-life of the mentha PPO at 70ºC was similar to PPO from other sources such as taro and potato (Duangmal and Owusu Apenten, 1999) grape (Rapeanu et al., 2006) and less resistant to heating than PPO from peppermint (Kavrayan and Aydemir, 2001) sweet potato (Lourenço et al., 1992) and palmito (Lourenço et al., 1990).

The effect of sugars on heat stability and activation energy

The enzyme was heated at 70, 75, 80, 85 and 90ºC in the presence and absence of sucrose at 0, 15, 30 and 40% concentration (w/w) in the incubation mixture. A rise in sucrose concentration corresponded to an increase in enzyme stability regardless of the heating temperature, when compared to control without sugar (Figs 4 to 6). The temperature-dependence of k was evaluated using Arrhenius equation as shown by the graph in Fig. 7. The apparent activation energy (Ea) for enzyme inactivation in the absence of sucrose was 78.13 kJ Mol-1 , a value higher than PPO from potato (Duangmal and Owusu Apenten, 1999) and lower than taro, Victoria grape and DeChaunac grape (Duangmal and Owusu Apenten, 1999, Rapeanu et al., 2006, Lee et al., 1983). The calculated values of the apparent activation energy (Ea) for enzyme inactivation in the absence and presence of sucrose at the temperature range studied showed an increase with sugar concentration. Ea values of 78.13, 80.37, 82.79 and 81.0 kJ Mol-1 were found at 0, 15, 30 and 40% sucrose, respectively. These results were contrary to that observed for peppermint PPO (Kavrayan and Aydemir, 2001) where the sucrose solutions at 20 and 40% (w/w) did not protect the enzyme against heat-inactivation. Lourenço et al (1992) observed a higher stability for sweet potato PPO in the presence of 20 and 40% (w/w) of sucrose. However, there are only few data related to activation energy in the presence of sugars for PPO from other materials. According to the present results and those of other authors the enzymes from different sources appeared to behave differently in the presence of sugars on heating. Various oxidative enzymes such as peroxidases were less susceptible to thermal inactivation when heated in different sucrose solution concentration (Chang et al, 1988, Neves and Lourenço, 1998; Neves, 2002). The protective effect of polyols on thermal denaturation of proteins is a fact; however, the mechanisms are still in discussion (Arakawa and Timashef, 1982, Neucere and St Angelo, 1985). Lee and Timashef (1981) and Arakawa and Timashef (1982) showed evidences of the protein-solvent relationship as a stabilizing factor of the authors observed an increase in the activation energy (Ea) for denaturation with an increase in sucrose concentration for different enzymes and they suggested that some physicochemical properties alterations of the system could be due to the water structure (Arakawa and Timashef, 1982, Back et al., 1979, Lee and Timashef, 1981).


 





Substrate specificity and enzyme kinetics

The extracted PPO from various sources have been shown varying substrate specificity as reported in the literature (Dogan et al., 2005; Dogan et al., 2005a, Aydemir, 2004, Lourenço et al., 1990; Concellón et al., 2004). The PPO from M. arvensis showed activity with various o-diphenols tested. The apparent Km and Vmax for the three substrates tested are present in the Table 1. Maximum activity was observed with caffeic acid, followed by 4-methylcathecol and catechol. L-tyrosine was not oxidized by the enzyme, suggesting a possible absence of cresolase activity. Resorcinol, DL-Dopa, pyrogallol, protocatechuic, p-coumaric, ferulic and cinnamic acids; catechin and quercetin were not oxidized by M. arvensis PPO (data not shown). The enzyme had a relatively high affinity towards caffeic acid, which was the the best substrate of those tested (lowest Km value). The Km for caffeic acid was 0.825 mM a value lower than 2.3 mM and 5mM related for potato (Duangmal et al., 1999) and sweet potato enzymes (Lourenço et al., 1992), respectively. However, it compared with the value of 0.590 mM for palmito PPO (Lourenço et al., 1990). The Km obtained for 4-methylcatechol was lower than reported for egg plant (Concellón et al., 2004), palmito stem (Robert et al., 1996), blackberry fruits (Gonzalez et al., 2000) and pear (Gauillard and Richard-Forget, 1997).

Lee et al. (1983) found Km values of 15.9 and 24.6 mM, respectively, for DeChaumac grape with caffeic and 4-methylcatechol as substrate. Duangmal and Owusu Apenten (1999) reported that 4-methylcatechol was the preferred substrate for PPO from taro and potato with a Km value of 9.0 and 1.1 mM, respectively.

When catechol was used as substrate the Km for M. arvensis PPO was close to the value of 7.51 mM, 5.0 mM, 6.25 mM, and 6.8 mM reported for PPO from Victoria grape (Rapeanu et al., 2006), litchi (Yue-Ming et al., 1997), peppermint (Kavrayan and Aydemir, 2001) and potato (Duangmal and Owusu Apenten, 1999). The apparent Vm/Km values for caffeic acid and 4-methylcatechol (Table 1) indicated a more enzymatic browning capability for the first substrate; however, the substrate catechol showed a lower affinity for PPO than the others. Victoria grape PPO (Rapeanu et al., 2006) showed higher values of specificity coefficient for chlorogenic, catechin and 4-methyl catechol, in the sequence. The M. arvensis PPO maintained activity when stored at -15 ºC for a period up to 30 days; it lost only 14% enzyme activity for five days and after 30 days, about 52% loss was observed. Thus, the M. arvensis PPO presented more stable than others like peppermint (Kavrayan and Aydemir, 2001) and artichoke (Dogan et al., 2005) for the same temperature and storage period. The Victoria grape PPO was very stable when stored at -80 and -35ºC (Rapeanu et al., 2006).

Effect of inhibitors on PPO activity

The potential of inhibition of PPO activity was verified with phenolic compounds analogue to the substrate, reducing agents and others. Table 2 shows the effect of various compounds on the activity of M. arvensis PPO. The most potent inhibitors were ascorbic acid and sodium metabisulfite since these compounds induced a high degree of inhibition, even at the lowest concentration used. Both inhibitors presented an initial lag phase when measuring the PPO activity. With regard to substrate analogues, cinnamic acid was the most effective inhibitor followed by pyrogallol, a trihydroxyphenol; p-coumaric and benzoic acid. EDTA did not inhibit the enzyme at concentrations up to 8 mM while ferulic acid acted as an activator of the mentha PPO at concentrations as low as 1.5 mM (data not shown). The inhibition was determined by a Dixon (1953) plot of 1/V versus [i] at two substrate concentrations (50 and 100 mM). The Ki and type of inhibition calculated are present in Table 2.

A competitive-type inhibition was obtained with ascorbic, cinnamic, protocatechuich, benzoic acid and metabisulfite. However, pyrogallol, pcoumaric acid and resorcinol showed to be non competitive-type inhibitors. Robert et al. (1997) observed a competitive-type inhibition with cinnamic and benzoic acid using 4-methylcatechol as substrate, while p-coumaric was shown to be non-competitive inhibitor for palmito PPO. The same was observed by Gunata et al. (1987) for grape polyphenoloxidase. Lourenço et al. (1992) reported that cinnamic and p-coumaric acids were competitive-type inhibitors of sweet potato PPO when 4-methylcatechol was used as substrate.

ACKNOWLEDGEMENTS

This study was supported by the Faculty of Pharmaceutical Sciences-UNESP Research Commission Program (PADC-FCF-UNESP).

Received: September 24, 2006; Revised: April 30, 2007; Accepted: July 30, 2008.

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  • *
    Author for correspondence:
  • Publication Dates

    • Publication in this collection
      10 Sept 2009
    • Date of issue
      Aug 2009

    History

    • Accepted
      30 July 2008
    • Reviewed
      30 Apr 2007
    • Received
      24 Sept 2006
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