Electrochemical Evaluation of Laccase Activity in Must

: As laccase (produced by Botrytis cinerea ) can significantly alter the properties of wine, winemakers frequently use commercially available colorimetric kits and spectrophotometers to measure the activity of this enzyme in grapes, must and wine. Although the used kits are based on electrochemically active substrates (such as syringaldazine and 2,2 (cid:48) -azino-bis(3-ethylbenzothiazoline-6-sulfonic acid), ABTS), the electrochemical determination of laccase activity as an alternative to the colorimetric determination was not thoroughly investigated up to now. Therefore, in the present work, we explored the electrochemical determination of laccase activity. Laccase activity measurements were carried out using either carbon fiber microelectrodes or screen-printed electrodes as working electrodes, either syringaldazine or ABTS as the electrochemically active laccase substrate, and either cyclic voltammetry or constant potential amperometry as the electrochemical method. The best performing approach, which combines ABTS, screen-printed gold electrodes, and constant potential amperometry, allowedidentifying laccasepositive mustsample (i.e., must sampleswith ›3U / mL laccase) in about 5 min.


Introduction
Laccases (E.C 1.10.3.2) are copper oxidase enzymes produced by fungi, plants, and bacteria that catalyze the oxidation of a variety of phenolic and nonphenolic substrates in the presence of molecular oxygen. Laccase is also one of the metabolites produced in grapes by Botrytis cinerea, a necrotrophic fungus producing significant economic damages in vineyards worldwide. Wines produced from infected grapes suffer enzymatic oxidative processes, irreversibly affecting their organoleptic properties. Detection of Botrytis cinerea in grapes using DNA-or antibody-based methods [1,2] is direct and accurate, but it is also complex, time-consuming, and costly, despite recent progress [3,4]. Alternative indirect methods of detecting Botrytis report on indicators such as laccase, gluconic acid, and glycerol, whose production is triggered in infected grapes [2]. While diagnostic methods based on infrared [2] and Raman spectroscopy [5] are emerging, fast, specific, and cost-effective methods for determining the degree of contamination by Botrytis cinerea are not yet available. In this context, even though it is not a direct and specific indicator, laccase activity is used to detect batches of Botrytis-affected grapes and musts in order to take corrective actions.
The spectrophotometric method developed by Dubourdieu and Grassin is among the widely used methods for determining laccase activity. It is based on syringaldazine (a reagent specific to laccase [6,7] that is not converted by the tyrosinase present in grapes) and is suitable for automated Buffer solutions used in this work were 0.1 M acetate (pH 4, 4.5, 5 and 5.5) and a phosphate buffer 0.1 M pH 6. All solutions were prepared using water from a Direct-Q 3 UV water purification system from Millipore SAS (Molsheim, France).

Measurements of Laccase Activity Using Electrochemistry
Both screen-printed electrodes and CFMEs were used to measure laccase activity through electrochemistry. The screen-printed Au electrodes (DRP 220 AT) were from Metrohm Dropsens (Oviedo, Spain). These are three-electrode systems printed on a ceramic support, including a 4 mm diameter Au working electrode, Au counter electrode and Ag reference electrode. The CFMEs were built using carbon microfibers with a diameter of 37 µm as previously described by us [28].
Electrochemistry experiments were performed using a VSP potentiostat and a computer equipped with the EC Lab software (BioLogic SAS, Grenoble, France). CFMEs were completed with a Pt wire counter electrode and a Ag/AgCl wire pseudoreference electrode when used in cyclic voltammetry. For laccase activity measurements, this three-electrode system was immersed into a 4 mL electrochemical cell containing 2.3 mL ABTS solution in 0.1 M acetate buffer at pH 4.5. Cyclic voltammograms were next recorded until the oxidation and reduction of ABTS produced stable currents. Then, either laccase standard solution (68.6 U/mL) or 150 µL of must sample was injected into the electrochemical cell and additional voltammograms were recorded to observe the evolution of the oxidation and reduction currents given by ABTS. The evolution of these currents was found to be laccase-activity-dependent for both standard solutions and must samples.
Chronoamperometry experiments using the screen-printed electrodes were performed, with the electrodes fixed horizontally, by applying onto the electrode surface a total volume of 100 µL solution (25 µL sample and 75 µL ABTS solution, 0.4 mM in 0.1 M acetate buffer pH 4.5) and polarizing the working electrode at 0 V versus the screen-printed reference electrode. The current intensity was recorded for 300 s and the difference between the current intensity at 30 s and at 300 s was taken as the analytical signal to be correlated with laccase activity in the sample.

Measurement of Laccase Activity Using Spectrophotometry
Measurements of laccase activity were performed using an Evolution 600 spectrophotometer (from Thermo Scientific, Gloucester, UK), at the fixed wavelength of 530 nm.
The method of Grassin and Dubourdieu [6] was followed, using syringaldazine as enzyme substrate and monitoring the enzymatic reaction at 530 nm, where the extinction coefficient of oxidized syringaldazine is 65,000 M −1 cm −1 . According to the method, one unit of enzymatic activity is defined as the amount of enzyme catalyzing the oxidation of a nanomole of syringaldazine per minute in the reaction conditions.

Preparation of Grape Musts
Musts were either provided by the Research and Development Institute for Vine and Wine Valea Calugareasca, Romania (from Sauvignon grapes contaminated with Botrytis cinerea) or were prepared in the laboratory from white or black grapes purchased from a local supermarket. Spiking with laccase was performed by adding an appropriate volume of stock laccase solution into Eppendorf tubes containing white or red must. The unspiked or spiked must samples were filtered through a PVPP cartridge, according to the method of Grassin and Dubourdieu [6] with some modifications: a 1 mL syringe filter was filled with 0.15 g of PVPP and a volume of 1 mL of must was passed through this filter. In some cases, as described in the text, a second filtration was performed by passing the PVPP filtered must through a centrifuge filter with a 10 kDa cutoff.

Electrochemical Evaluation of Laccase Activity Using CFMEs
Electrodes are relatively easy to miniaturize; this fact is considered an important advantage of electrochemical analytical methods as compared to optical analytical methods. Electrodes have already been miniaturized, even to sizes facilitating experiments in the tiny intracellular space of a single living cell (see, for example, [29]). Therefore, with laccase activity measurements in a single grape berry in mind, we investigated if CFMEs are suitable for the electrochemical evaluation of laccase activity.
Both syringaldazine and ABTS were initially considered to carry out the present study. However, syringaldazine was observed to show an increased tendency to irreversibly adsorb onto CFMEs. Therefore, in our first experiments, we combined CFMEs with ABTS.
In cyclic voltammetry experiments performed with carbon electrodes in acetate buffer pH 5, ABTS displayed two redox couples with formal potentials at 0.469 V and 0.870 V [30], corresponding to the following one electron, quasireversible transformations: Enzymatic oxidation of ABTS by laccase produces only ABTS .+ [30]; hence, in our cyclic voltammetry experiments, we concentrated on the first redox couple of ABTS, corresponding to the transformation (1), and investigated potential ranges up to 0.7 V. Figure 1A,B show typical cyclic voltammograms recorded with CFMEs in the presence of 0.5 mM of ABTS and two different concentrations of laccase (0.12 U/mL and 0.47 U/mL). As one can observe, the electrochemical oxidation of ABTS gives S-shaped voltammograms due to the enhanced, hemispherical diffusion of ABTS to the surface of the microelectrodes. Notably, in the absence of laccase, these voltammograms are stable for extended periods of time (>30 min) presenting no signs of ABTS adsorption to the surface of the microelectrode (see red signals in Figure 1A,B). However, in the presence of laccase, the currents resulting from the oxidation of reduced ABTS (e.g., at +0.4 V) start decreasing over time (see Figure 1C), whereas the currents resulting from the reduction of oxidized ABTS (e.g., at 0 V) start increasing over time (see Figure 1D). This time evolution of the voltammograms is due to the laccase consuming reduced ABTS and producing oxidized ABTS, and thus interfering with the electrochemistry of ABTS. Moreover, the decrease of the oxidation currents and the increase of the reduction currents are both faster when the laccase concentration is larger ( Figure 1C,D). Cyclic voltammograms similar to those shown in Figure 1A,B were recorded in the presence of several other concentrations of laccase (from 1.5 µg/mL to 24 µg/mL, i.e., from 0.12 U/mL to 1.89 U/mL). The way the oxidation current decreases at +0.4 V and the reduction current increases at 0 V in these voltammograms was then quantified and used to build calibration curves for the determination of laccase activity. The procedure was carried out both at pH 6 (in phosphate buffer) and at pH 4.5 (in acetate buffer). The obtained average calibration curves (see Figure 2) show that laccase converts ABTS about seven times faster at pH 4.5 than at pH 6.
After we obtained the calibration curves shown in Figure 2, we proceeded to analyze must samples spiked with different concentrations of laccase. These must samples (white and red) were obtained from healthy grapes and were tested by the spectrophotometric method with syringaldazine. As expected, no laccase activity was detected. The musts were then spiked with laccase from Trametes versicolor and pretreated with PVPP cartridges as described in the Materials and Methods section. The results obtained from analyzing the must samples are summarized in Table 1.   It is important to note that currents at +0.4 V decrease when laccase is present, whereas currents at 0 V increase when laccase is present. As one can observe, the CFME-based electrochemical approach has a significant tendency to underestimate the laccase content of must (somewhat more when the must is red as compared to when the must is white). Phenolic compounds that were not removed during sample pretreatment and that are converted by laccase but not detected electrochemically could be the cause of this underestimation. Nevertheless, we consider the possibility offered by the electrochemical method to determine laccase activity at two different potentials interesting and promising as it can provide robustness and reliability. At this point of time, laccase activity determination at positive potentials (e.g., +0.4 V) seems to function in a manner similar to that of laccase activity determination at negative potentials (e.g., 0 V). It was also investigated if replacing cyclic voltammetry with constant potential amperometry improves the CFME-based laccase activity assay. Typical current signals recorded in the presence of different laccase concentrations and the average calibration curve for laccase activity determination using amperometry are shown in the Supplementary Material. Unfortunately, when tested with must samples spiked with laccase, the amperometry-based approach showed the same tendency to underestimate the laccase content of must as the cyclic-voltammetry-based approach.

Evaluation of Laccase Activity Using SPAuEs
While the approach based on cyclic voltammetry and CFMEs can sensitively detect laccase and is amenable to further miniaturization, it requires additional development to convert it into a fast, simple and reliable assessment of laccase activity outside the laboratory. Screen-printed systems are commercially available as ready-to-use three-electrode systems, appropriate for analyzing small volume samples. A variety of electrode materials and modifiers are currently available. Constant potential amperometry is an electrochemical method that is available even on the simplest electrochemical equipment. Moreover, it is minimally affected by capacitive currents, has excellent temporal resolution and allows an easier calculation of the laccase activity than potentiodynamic methods. With this in mind, we examined the performances of screen-printed electrodes for the assessment of laccase activity by chronoamperometry.
Initial screening of carbon and gold electrodes emphasized unwanted adsorption of must components on the carbon surface for low sample dilution factors. Consequently, the studies reported below were conducted exclusively using SPAuEs. The measurement principle for laccase activity using SPAuEs, ABTS as substrate and chronoamperometric detection is illustrated in Figure 3.
methods. With this in mind, we examined the performances of screen-printed electrodes for the assessment of laccase activity by chronoamperometry.
Initial screening of carbon and gold electrodes emphasized unwanted adsorption of must components on the carbon surface for low sample dilution factors. Consequently, the studies reported below were conducted exclusively using SPAuEs. The measurement principle for laccase activity using SPAuEs, ABTS as substrate and chronoamperometric detection is illustrated in Figure  3. Principle of measuring the activity of laccase in must with SPAuEs: laccase-containing must obtained from Botrytis cinerea-infected grapes is filtered through a PVPP cartridge to eliminate phenolic compounds; then, it is mixed with ABTS on the surface of a SPAuE. The oxidized ABTS formed in the laccase-catalyzed reaction (i.e., ABTS .+ ) is reduced on the electrode at 0 V vs. Ag/AgCl and the difference in the cathodic current recorded at 300 s and 30 s (ΔI) is proportional to laccase activity in the must.

Optimization of The Experimental Conditions and Calibration
First, the feasibility of exploiting the electrochemistry of ABTS at the surface of SPAuE for measuring laccase activity was confirmed by cyclic voltammetry (reported in the Supplementary Material, Figure S2). Next, the main experimental parameters, i.e., the pH of the buffer solution, the concentration of ABTS and the value of the applied potential were optimized ( Figure 4A-C). The influence of the applied potential in the chronoamperometric determination of laccase activity was studied in the range from −0.2 to +0.5 V, using a solution of 7.89 U/mL laccase from Trametes versicolor and a concentration of ABTS of 0.2 mM in 0.1 M acetate buffer pH 5. These studies indicated that the largest increase in the cathodic current due to the reduction of the enzymatically generated ABTS .+ was recorded at potentials from 0.050 to −0.1 V (see Figure 4A). Additional studies were performed with PVPP-filtered must to identify any potential interferences due to electrochemically active compounds from the grapes. Based on the combined results of these studies, an applied potential of 0 V was found as optimum. Tests performed with laccase from Trametes versicolor and with a must from Botrytis cinerea-contaminated grapes in acetate buffer with pH in the range 4.5-6 let us identify an optimum pH of 4.5 (see Figure 4B). By repeated testing using ABTS concentrations of 0.2, 0.4, 0.97 and 1.94 mM, the optimum concentration of enzyme substrate was found to be 0.4 mM (see Figure 4C).

Optimization of The Experimental Conditions and Calibration
First, the feasibility of exploiting the electrochemistry of ABTS at the surface of SPAuE for measuring laccase activity was confirmed by cyclic voltammetry (reported in the Supplementary Material, Figure S2). Next, the main experimental parameters, i.e., the pH of the buffer solution, the concentration of ABTS and the value of the applied potential were optimized ( Figure 4A-C). The influence of the applied potential in the chronoamperometric determination of laccase activity was studied in the range from −0.2 to +0.5 V, using a solution of 7.89 U/mL laccase from Trametes versicolor and a concentration of ABTS of 0.2 mM in 0.1 M acetate buffer pH 5. These studies indicated that the largest increase in the cathodic current due to the reduction of the enzymatically generated ABTS .+ was recorded at potentials from 0.050 to −0.1 V (see Figure 4A). Additional studies were performed with PVPP-filtered must to identify any potential interferences due to electrochemically active compounds from the grapes. Based on the combined results of these studies, an applied potential of 0 V was found as optimum. Tests performed with laccase from Trametes versicolor and with a must from Botrytis cinerea-contaminated grapes in acetate buffer with pH in the range 4.5-6 let us identify an optimum pH of 4.5 (see Figure 4B). By repeated testing using ABTS concentrations of 0.2, 0.4, 0.97 and 1.94 mM, the optimum concentration of enzyme substrate was found to be 0.4 mM (see Figure 4C).
Calibration experiments with the SPAuE in optimized conditions (i.e., 0.1 M acetate buffer pH 4.5, 0 V applied potential, 0.4 mM ABTS) led to determining the linear range as 0.79-15.8 U/mL and the detection limit as 0.5 U/mL, calculated as three times the standard deviation of the blank, divided by the slope of the linear range of the calibration curve. An average sensitivity of 9.23 ± 1.06 nA.mL/U was also calculated, based on n = 6 calibration curves obtained with different sensors, on different days. A typical calibration curve is shown in Figure 4D.

Investigation of The Grape Must Matrix Effects
Phenolic antioxidants in grapes/must/wine can affect the determination of laccase activity in different ways: (i) by reacting with ABTS .+ , i.e., by scavenging the stable radical cation ABTS .+ ; (ii) by acting as substrates for laccases; (iii) by presenting electrochemical activity in the potential range used with the proposed sensor. Therefore, an accurate determination of laccase activity requires elimination of possibly interfering phenolic compounds prior to analysis. This was achieved by filtering the grape must through a PVPP cartridge according to the procedure proposed by Dubourdieu [7] adapted for small sample volumes. The electrochemical activity and potential interferences of the PVPP-filtered  Figure 5A). With PVPP-filtered red must, a small anodic current was observed (red colored signal in Figure 5A), as compared to the stable signal in buffer (black colored signal in Figure 5A) and to the cathodic current, growing with time in laccase-containing solutions (blue colored signal in Figure 5A). Consequently, there are no electrochemical reduction processes in PVPP-filtered must that interfere with the reduction of the enzymatically formed ABTS .+ .  Calibration experiments with the SPAuE in optimized conditions (i.e., 0.1 M acetate buffer pH 4.5, 0 V applied potential, 0.4 mM ABTS) led to determining the linear range as 0.79-15.8 U/mL and the detection limit as 0.5 U/mL, calculated as three times the standard deviation of the blank, divided by the slope of the linear range of the calibration curve. An average sensitivity of 9.23 ± 1.06 nA.mL/U was also calculated, based on n = 6 calibration curves obtained with different sensors, on different days. A typical calibration curve is shown in Figure 4 D.

Investigation of The Grape Must Matrix Effects
Phenolic antioxidants in grapes/must/wine can affect the determination of laccase activity in different ways: (i) by reacting with ABTS .+ , i.e., by scavenging the stable radical cation ABTS .+ ; (ii) by acting as substrates for laccases; (iii) by presenting electrochemical activity in the potential range used with the proposed sensor. Therefore, an accurate determination of laccase activity requires elimination of possibly interfering phenolic compounds prior to analysis. This was achieved by filtering the grape must through a PVPP cartridge according to the procedure proposed by Dubourdieu [7] adapted for small sample volumes. The electrochemical activity and potential interferences of the PVPP-filtered must were checked by chronoamperometry at 0 V ( Figure 5A). With PVPP-filtered red must, a small anodic current was observed (red colored signal in Figure  5A), as compared to the stable signal in buffer (black colored signal in Figure 5A) and to the cathodic current, growing with time in laccase-containing solutions (blue colored signal in Figure  5A). Consequently, there are no electrochemical reduction processes in PVPP-filtered must that interfere with the reduction of the enzymatically formed ABTS .+ .
These promising initial results were reconfirmed by performing calibration experiments with the same sensor, for (i) a series of five laccase standard solutions made in buffer with laccase concentrations in the range from 0.79 to 15.8 U/mL and for (ii) white and (iii) red must spiked with These promising initial results were reconfirmed by performing calibration experiments with the same sensor, for (i) a series of five laccase standard solutions made in buffer with laccase concentrations in the range from 0.79 to 15.8 U/mL and for (ii) white and (iii) red must spiked with laccase in the same concentrations. A total of n = 3 replicate assays were performed at each concentration.
As illustrated in Figure 5B, the sensitivity of the electrochemical detection of laccase activity is significantly lower in must than in buffer, and the matrix effect is more evident for red musts compared to the white musts. Most probably, the consistently lower laccase activity in red musts is due to the phenolic compounds (more abundant in red musts compared to white musts), which are either outcompeting ABTS for oxidation by laccase or quenching the ABTS .+ formed in the enzymatic reaction. The outcome of both processes is a smaller amount of oxidized ABTS available for electrochemical reduction on the electrode.
Further investigation of possible interferences focused on comparing the results of the electrochemical assay using SPAuE and ABTS with the spectrophotometric method using syringaldazine as enzyme substrate. In these experiments, a series of grape must samples with activities in the range 2.4-15.8 U/mL was analyzed, including both Botrytis cinerea-contaminated samples and must from healthy grapes intentionally spiked with laccase from Trametes versicolor. The results in Figure 5C emphasize a relatively good agreement between the results obtained by the two methods, better for white musts than for the red ones, i.e., the correlation coefficient R 2 decreases from 0.9072 to 0.8475 when red wines are included in the comparison. From the results in Figure 5C, it is obvious that the laccase activity of red musts (shown in red) is underestimated by the electrochemical method compared to the spectrophotometric method with syringaldazine. In contrast, in some white musts, we observed significantly higher activities measured electrochemically with ABTS than by the spectrophotometric method. Both syringaldazine and ABTS are used as enzyme substrates for measuring the laccase activity of musts by optical methods, as detailed in the Introduction. While syringaldazine is considered specific for laccase, it has some disadvantages related to the low solubility in aqueous solutions, low stability, adsorption on carbon surface and color similar to that of wine. Instead, ABTS is considered by some reports a better alternative for optical detection [11]. More relevant for this work, the experimental conditions for the spectrophotometric test with syringaldazine (pH 5.5, presence of ethanol in the reaction medium) and for the proposed electrochemical assay using ABTS (pH 4.5, no organic solvent) are quite different. To verify if the differences reported in Figure 5 are due to the electrochemical method or are mainly associated with the different substrate and experimental conditions, we performed parallel measurements using the proposed electrochemical method and using a colorimetric test with ABTS for a set of 14 samples including both white and red musts. The tests were performed in the same experimental conditions (pH, concentration of ABTS). The results reported in Supplementary Material, Figure S3A,B show good agreement between activities measured via chronoamperometry and values determined spectrophotometrically for all wines.  As illustrated in Figure 5B, the sensitivity of the electrochemical detection of laccase activity is significantly lower in must than in buffer, and the matrix effect is more evident for red musts compared to the white musts. Most probably, the consistently lower laccase activity in red musts is due to the phenolic compounds (more abundant in red musts compared to white musts), which are either outcompeting ABTS for oxidation by laccase or quenching the ABTS .+ formed in the enzymatic reaction. The outcome of both processes is a smaller amount of oxidized ABTS available for electrochemical reduction on the electrode.
Further investigation of possible interferences focused on comparing the results of the electrochemical assay using SPAuE and ABTS with the spectrophotometric method using (B) Sensitivity of the electrochemical assay (slope of the calibration curve) in buffer, white and red must, respectively. (C) Comparison between the laccase activity measurements performed by the spectrophotometric method based on syringaldazine and by the proposed electrochemical method based on ABTS and SPAuEs. Black: white musts from Botrytis cinerea-contaminated grapes and from white grapes spiked with laccase. Red: red musts spiked with laccase. The linear fit between the two methods for all samples (white and red musts included) is shown in red; the fit for white-only musts is shown in black.
Consequently, the differences observed between the reference spectrophotometric method with syringaldazine and the proposed electrochemical assay are mostly due to the differences in catalytic oxidation of the two substrates, syringaldazine and ABTS by laccase [23], and to the different ways in which these catalytic processes are affected by grape phenolics. Electroactive phenolic compounds or phenols reacting with ABTS in a laccase-mediated reaction are possible sources of interference in the proposed electrochemical assay. However, analysis of laccase-free musts in the presence of ABTS by chronoamperometry at 0 V did not show any interference by a direct contribution to the cathodic current ( Figure 5A).
Optimization of sample preparation is anticipated to eliminate the inaccuracies due to interfering compounds in musts. As a preliminary solution, we investigated the introduction of a second filtration step through a centrifuge filter with a cutoff of 10 KDa, after the filtration through the PVPP cartridge. This procedure should eliminate all small molecular weight compounds such as phenolic compounds. A first test was conducted using a white must for which the difference between the result given by the spectrophotometric method and the result given by the electrochemical assay was large, i.e., no laccase was detected in the PVPP-filtered must using spectrophotometry, while 2.41 ± 0.23 U/mL laccase was measured using the electrochemical method. When the additional filtration through the 10 kDa filter was performed, the activity determined using spectrophotometry was 2.71 ± 0.15 U/mL, in good agreement with the results from the electrochemical method, 2.56 ± 0.42 U/mL. While the results remain to be confirmed for more must samples, they suggest that additional filtration would improve the accuracy of measurements using both spectrophotometric and electrochemical methods.

Accuracy of The Assay
The accuracy of the electrochemical assay was checked with a series of spiked white and red musts samples with laccase activities covering the linear range of the assay ( Table 2). The samples (1.5 mL) were filtered through the PVPP cartridge, recovering the first 1 mL. While the recovery factors were 88.2%-113.4% in white musts, in red musts the recoveries averaged 73.5%, confirming the matrix effect (observed also with CFMEs, see Table 1). Literature data suggest that removing color from red musts through treatment with PVPP also removes some laccase [31]. However, this does not appear to fully explain our results, since the recovery was quantitative when checked using spectrophotometry.
Optimization of sample preparation is anticipated to eliminate the inaccuracies due to interfering compounds in musts. The matrix effect can be overcome using the standard additions method instead of external calibration or by introducing a second filtration step through a suitable filter to eliminate small molecular weight interfering compounds (as shown above). As these two solutions imply a longer analysis time and incompatibility with in-field measurements, we will explore in future studies another alternative: optimizing the sample pretreatment by adapting the composition of the filter cartridge so that sample pretreatment will consist of a single fast filtration step.
Compared to colorimetric kits and optical detection methods developed for laccase activity measurements, the proposed electrochemical assay has the advantages of delivering quantitative results in short time. With further improvements, as discussed above, it can be adapted for in-field measurements to provide winemakers with the needed support to take timely corrective actions and maximize the quality of their wine. Other electrochemical methods for the detection of Botrytis cinerea infection in grapes either provide another indirect evaluation of fungal infection by measuring the levels of glycerol and gluconic acid produced [25] or use an antibody that binds to several Botrytis species in addition to Botrytis cinerea. Antibody-based assays use the monoclonal antibody (BC-12.CA4) [32,33] raised against a mycelium antigen. These assays were developed in various formats, from lateral flow devices to ELISA kits and biosensors [2]. Electrochemical immunosensors developed by Fernández-Baldo et al., which used screen-printed carbon electrodes modified with carbon nanotubes [34] or magnetic beads [35] detected Botrytis antigen down to 0.008 µg/mL [35]. Another electrochemical biosensor reported by Binder et al. [3], based on the same antibody and a SPAuE, detected the pathogen responsible for the neck rot infection of onions. While the antibody differentiates Botrytis from potentially co-infecting Aspergillus and Penicillium microorganisms in grapes, it is not specific for Botrytis cinerea, e.g., the biosensor developed by Binder et al. responded to four Botrytis species [3]. Moreover, a standard of Botrytis cinerea antigen is not commercially available; this poses some limitations to the development of biosensors for detecting this fungal pathogen. While the above-reported electrochemical sensors for glycerol, gluconic acid and Botrytis cinerea have good analytical characteristics, laccase detection is preferable, considering the oxidative processes catalyzed by this enzyme, leading to irreversible alterations of organoleptic properties of wine, if the enzyme activity is not inhibited. To summarize, fast, simple and accurate assays for measuring laccase activity such as the electrochemical procedures proposed in this work have clear advantages and usefulness for winemakers over other existing analytical tools to check the sanitary status of the grapes and evaluate the potential for irreversible oxidative damage.

Conclusions
Collectively, the information presented above shows that the simple electrochemical assay based on commercially available SPAuEs can be used for the fast determination of laccase activity at levels relevant for the wine industry. The assay is able to differentiate between healthy grapes with low (under 1 U/mL) laccase activities and grapes seriously affected by fungi (showing laccase levels higher than 3 U/mL), which will pose problems for wine production. The proposed procedure for measuring laccase activity, including a fast (<1 min) filtration of the must through a PVPP cartridge, dilution with buffer containing ABTS and a 3-min-long electrochemical analysis with a disposable electrode, is adequate for implementation in wineries, at the point of grape processing (to determine preventive actions) or in the vineyard (to establish the spread of fungal diseases and help with taking corrective actions such as spraying with fungicides).
However, for measuring low activities of laccase, e.g., to study the mechanism of fungi attack on grapes or to sensitively measure the amounts of extracellular enzyme generated in culture media of laccase-producing fungi, analytical tools with higher sensitivity are required. The investigated approach based on CFMEs delivered better sensitivity and is amenable to further miniaturization, whereas the analysis by cyclic voltammetry offered reliability as both oxidation and reduction of ABTS were explored. An underestimation of the laccase activity with the CFMEs was observed, despite using a higher dilution factor compared to the SPAuEs; this was attributed to adsorption of must components onto the CFMEs and the presence of phenolic compounds, which consume oxidized ABTS and/or inhibit its enzymatic generation. In perspective, we plan to change the material of our microelectrodes to gold and further miniaturize the three-electrode setup to perform studies in single berries.
Differences observed between the proposed electrochemical assays with ABTS and the spectrophotometric method with syringaldazine, much higher in the case of red musts than for white musts, are attributed to the differences in the kinetics and affinity of the two substrates for laccase and their different susceptibility to competition with remaining phenolic compounds. Future studies will include comparison with a spectrophotometric method based on ABTS to eliminate any differences due to the different substrates and enable a clearer assessment of possible interferences in laccase determination by the proposed approach. Sample preparation will be also a focus of our future studies to address the matrix effects.
Supplementary Materials: The following are available online at http://www.mdpi.com/2227-9040/8/4/126/s1, Figure S1, Chronoamperometric signals recorded with a CFME in the presence of increasing concentrations of laccase and average calibration curve for laccase activity determination obtained with CFMEs and chronoamperometry, Figure S2: Cyclic voltammograms recorded with a SPAuE in ABTS solutions with and without laccase, Figure S3: Calibration curve for laccase activity determination using the spectrophotometric method with ABTS and comparison between the proposed electrochemical assay with ABTS and the spectrophotometric method with ABTS.

Conflicts of Interest:
The authors declare no conflict of interest.