Phytochemical Characterization of Veronica officinalis L., V. teucrium L. and V. orchidea Crantz from Romania and Their Antioxidant and Antimicrobial Properties

Aerial parts of Veronica species are used in Romanian traditional medicine for the treatment of various conditions like kidney diseases, cough, and catarrh, and are known for their wound-healing properties. In the present study, the phenolic and sterolic content and the antioxidant and antimicrobial activities of three Veronica species (Plantaginaceae), V. officinalis L., V. teucrium L. and V. orchidea Crantz, were studied. The identification and quantification of several phenolic compounds and phytosterols were performed using LC/MS techniques and the main components were p-coumaric acid, ferulic acid, luteoline, hispidulin and β-sitosterol. More than that, hispidulin, eupatorin and eupatilin were detected for the first time in the Veronica genus. Nevertheless, representatives of the Veronica genus were never investigated in terms of their phytosterol content. The antioxidant potential investigated by Trolox equivelents antioxidant capacity (TEAC) and EPR spectroscopy revealed that V. officinalis and V. orchidea extracts presented similar antioxidant capacities, whilst the values registered for V. teucrium extract are lower. Regarding the antimicrobial activity of the investigated species, Staphylococcus aureus, Listeria monocytogenes and Listeria ivanovii were the most sensitive strains with MIC values between 3.9 and 15.62 mg/mL. The results obtained by this study may serve to promote better use of representatives from the genus Veronica as antioxidant and antimicrobial agents.


Introduction
Natural products have been and continue to be a source of inspiration for a substantial portion of human therapeutics. In medicinal plants, secondary metabolites are considered bioactive natural compounds and may ultimately be developed as drugs. In food, they would be defined as phytonutrients without having therapeutic claims but with significant health benefits that can be useful in disease prevention [1]. Interest in developing natural nutritional antioxidants is increasing due to their well documented impact on human health [2], but also due to the fact that synthetic antioxidants have been incriminated as endocrine disrupters or even carcinogenic agents [3]. Medicinal plants rich in polyphenols can retard the oxidative degradation of lipids and improve the quality and nutritional value of food [2]. Considered to be the most frequent antioxidant compounds in human diets, polyphenols possess multiple biological properties [4], making it vital to learn about their amounts and varieties in medicinal plants and natural foods [5,6].
Sterolic compounds occur in a wide range of plant species; both yellow and green vegetables contain appreciable quantities. Phytosterols have demonstrated the ability to block the uptake of cholesterol (to which they are structurally related) and also facilitate its excretion from the body [7]. The most common phytosterols in natural products are β-sitosterol, stigmasterol, and campesterol. They can reduce the atherosclerotic risk and offer protection against cardiovascular diseases, and decrease the risks of breast, prostate and colon cancer [8,9]. Furthermore, phytosterols have anti-inflammatory and immunomodulatory properties [10]. However, all phytosterol intake comes exclusively from the diet, as they cannot be synthesized by humans. It is known that more than 95% of total phytosterol dietary intake is represented by β-sitosterol, stigmasterol and campesterol [8].
The genus Veronica L. is the largest genus of the Plantaginaceae family, with about 500 species widespread over most of the Northern Hemisphere and in many parts of the Southern Hemisphere; it presents high ecologically diversity, with species growing in aquatic to dry steppe habitats from sea level to high alpine regions. This diversity and the fact that many species have beautiful blue flowers may explain the interest Veronica has attracted for a long time [11]. Aerial parts of Veronica species are used as traditional medicine for treatment of various inflammatory conditions, including rheumatism [12]. Some of the Veronica species, like Veronica officinalis L. have a long history of medicinal use as diuretic and diaphoretic agents. In Romanian folk medicine, it has been used for kidney diseases, cough, and catarrh, and was known for its wound-healing properties and its indication in lung diseases and hypercholesterolemia [13][14][15]. The chemical composition of Veronica has been previously investigated regarding its iridoid profile [16,17], but no other data was found regarding the phenolic or sterolic profile of Romanian harvested V. officinalis, V. teucrium and V. orchidea. However, recently, a few studies have confirmed that certain Veronica species showed noticeable bioactivity such as antibacterial [18], antioxidant [19,20], anti-inflammatory [21] and citotoxic [21,22] activity.
Within this frame, this study aimed to investigate the phenolic and sterolic composition of aerial parts of relevant Veronica species (V. officinalis, V. teucrium and V. orchidea) harvested from the Romanian spontaneous flora (Figure 1a-c). The quantitative content of the phenolic or sterolic compounds was estimated using HPLC-MS (high performance liquid chromatography coupled with mass spectrometry) techniques. This study was also intended to explore the antioxidant capacities of the three species by means of spectrophotometry and EPR (electron paramagnetic resonance) spectroscopy. Additionally, the evaluation of the antimicrobial effect was carried out using a microdilution technique.

HPLC-MS Analysis of Phenolic Compounds
In this study the presence and content of different phenolic compounds in 70% ethanolic extracts was studied using an HPLC-MS method which allows the simultaneous detection of several phenolic compounds with a single column pass [23][24][25]. In order to obtain more accurate data on flavonoid glycoside and aglycone concentrations, and to estimate the nature of the hydrolyzed compounds, each sample was analyzed before and after acid hydrolysis [26]. According to the obtained results, the phenolic content varies greatly among tested Veronica species, as seen in Table 1. Regarding the phenolic acids, p-coumaric acid was the most abundant in V. teucrium extract (24.27 ± 0.23 μg/g d.w. plant material) and ferulic acid (31.35 ± 0.25 μg/g d.w. plant material) in the V. officinalis extract. However, gentisic and chlorogenic acids were identified in all extracts but their amounts were too low to be quantified. The presence of phenolic acids in several Veronica species was previously reported by several authors. Thus, Beara et al. [12] reported lower amounts of ferulic and p-coumaric acids in Serbian harvested V. teucrium. The same authors reported the presence of these compounds also in aerial parts of V. jaquinii and V. urticifolia [12]. Higher amounts of caffeic acid were reported by Barreira et al. [27] in V. montana and V. spuria and by Živković et al. [28] in V. urticifolia. The increased quantities of phenolic acids after acid hydrolysis suggest the presence of several glycosylated structures in these compounds.
Quercitrin was identified only in V. officinalis (87.78 ± 0.51 μg/g d.w. plant material) and in traces in V. orchidea. Regarding the flavonoid aglycones, apigenin was identified in both V. officinalis and V. orchidea unhydrolyzed samples and just in the hydrolyzed extract of V. teucrium. The richest species in luteolin was V. officinalis (36.48 ± 0.18 μg/g d.w. plant material), the aglycone being present in both hydrolyzed (36.48 ± 0.18 μg/g d.w. plant material) and unhydrolyzed (89.72 ± 3.08 μg/g d.w. plant material) samples, whilst in V. teucrium and V. orchidea it was only present in glycosylated forms. Different flavone aglycones luteolin, apigenin, chrysoeriol, scutellarein and isoscutellarein have been previously detected in Veronica species [29]. Our results are also in line with previous findings by Beara et al. [12], who reported the presence of several glycosylated forms of apigenin and luteolin in aerial parts of Veronica species, but regarding V. teucrium the presence of apigenin was not detected in the unhydrolyzed extract.

HPLC-MS Analysis of Methoxylated Flavones
The importance of methoxylated flavones has increased nowadays due to their superior cancer chemopreventive role. Some of the methoxylated citrus flavonoids have also, in preliminary studies, demonstrated antiproliferative properties [29]. Other compounds like hispidulin have been proven as potent antiepileptic [30] and antifungal agents [31]. Within this frame, another aim of this study was to quantitatively characterize the aerial parts of V. officialis, V. teucrium and V. orchidea related to their jaceosidin, hispidulin, eupalitin, eupatorin, casticin and acacetin content by using a newly developed LC-MS/MS method. Because of the lack of authentic standards, flavonol glycosides are in most cases hydrolysed to their respective aglycons prior to analysis. In this case the samples were subjected to analysis before and after acid hydrolysis.
Under the described chromatographic conditions, the compounds eluted in less than 10 min: jaceosidin (RT = 2.9 min), hispidulin (RT = 4.2 min), eupalitin (RT = 7.05 min), eupatorin (RT = 7.6 min), casticin (RT = 8.05 min) and acacetin (RT = 9.8 min), as seen in Figure 2. The ions monitorized in the MS method are presented in Table 2 (Table 2) the extracted chromatograms of each compound were constructed for quantification, taking into account the intensity of major ions in the mass spectrum.  Hispidulin was found in all samples of V. officinalis and V. orchidea and only in the hydrolyzed extract of V. teucrium. The richest source of hispidulin was V. orchidea (4.115 ± 0.09 μg/g d.w. plant material) followed by V. officinalis (0.747 ± 0.01 μg/g d.w. plant material). The increased yields of these compounds after acid hydrolysis suggest that they are present also in glycosylated forms. Eupatorin was quantified in both samples of V. officinalis, while it was present just in the hydrolyzed sample of V. teucrium (0.68 ± 0.04 μg/g d.w. plant material) as seen in Table 3. As a peculiarity, eupatilin was found only in V. orchidea extracts (0.491 ± 0.04 μg/g d.w. plant material and 0.252 ± 0.02 μg/g d.w. plant material, respectively). More than that, hispidulin, eupatilin and eupatorin were detected for the first time in Veronica genus and the analyzed plant species, respectively.

HPLC-MS Analysis of Phytosterolic Compounds
In the proposed chromatographic conditions, the compounds eluted with the following retention times: 3.2 min for ergosterol, 3.9 min for brassicasterol, 4.9 min for stigmasterol and campesterol (co-elution) and 5.7 min for β-sitosterol. The ions monitorized in the MS method are presented in Table 4. Because, in the ionization conditions, all sterols have lost a water molecule, the ions detected are always in the form [M − H2O + H] + [32]. The derived ions of the sterols (379 for ergosterol, 381 for brassicasterol, 395 for stigmasterol, 383 for campesterol and 397 for β-sitosterol) have been fragmented, and based on their daughter ions from the MS spectrum the extracted chromatograms of each compound were constructed. The method can also be applied for quantitative analysis because the intensity of ions in the mass spectrum is proportional to the concentration of the substance in the sample.
For quantitative analysis of the five sterols from Veronica species, the extracted chromatograms for each compound were constructed, taking into account the intensity of major ions in the mass spectrum (Table 4) as seen in Table 5. β-Sitosterol, campesterol and stigmasterol were quantified in all the analyzed species. The major sterolic compound was β-sitosterol in all samples, the richest source being V. officinalis (729.43 ± 9.21 μg/g d.w. plant material). V. orchidea and V. officinalis presented similar amounts of campesterol (32.75 ± 1.05 and 30.32 ± 0.31 μg/g d.w. plant material, respectively). The highest amount of stigmasterol was found in V. officinalis (42.09 ± 1.01 μg/g d.w. plant material) followed by V. teucrium (29.16 ± 1.06 μg/g d.w. plant material). As a peculiarity, ergosterol was found only in V. officinalis and in a small amount (1.91 ± 0.01 μg/g d.w. plant material). This is the first report that deals with the quantification of several phytosterols from the Veronica genus, respectively from V. officinalis, V. teucrium and V. orchidea aerial parts.

Determination of Phenolic Compound Content
Besides the identified compounds, many other polyphenolic compounds are widely distributed in aerial parts of Veronica and contribute to their antioxidant activity. In this part a preliminary comparative view of the total phenolic and flavonoid content of V. officinalis, V. teucrium and V. orchidea is presented. The total phenolic content (TPC; Figure 3a) varied from 17.71 ± 0.44 for V. teucrium to 34.40 ± 2.08 mg Gallic acid (GAE) equivalents/g d.w. vegetal material for V. orchidea, V. officinalis presenting a similar value in terms of TPC to that of V. orchidea (32.37 ± 1.27 mg GAE/g d.w.).
The highest total flavonoid content (TFC; Figure 3b) was registered for V. teucrium (6.60 ± 0.26 mg Quercetin (QE) equivalents/g d.w. vegetal material). Lower amounts were obtained for V. orchidea (2.95 ± 0.02 mg QE/g d.w.) and V. offcinalis (2.52 ± 0.16 mg QE/g d.w.). Available literature on Veronica species illustrates a high variation of total phenolic contents. While some reported that aerial parts of Serbian V. teucrium provides phenolic contents of approx. 157 mg GAE/g of dry methanol extract and 172 mg GAE/g of dry 70% aqueous acetone extract, respectively [33], others reported higher levels in V. officinalis with values of approx. 200.20 mg GAE/g of dry methanolic extract [34]. In the present study, the phenolic contents of Veronica species were expressed as mg/g of d.w. herbal products. Taking all this into account, the present results are hard to compare with previous results obtained by other authors due to the fact that the authors expressed their values in a different manner.

Antioxidant Features
Antioxidant activity of natural products, resulting from many compounds such as phenolic compounds (e.g., flavonols) and pigments, offers preventive potential against oxidative stress in the human body. Thus, the trend is towards herbal supplements or foods with more phytochemicals and natural antioxidants. In this part of the investigation, the goal was to evaluate the antioxidant activity of V. officinalis, V. teucrium and V. orchidea. As several authors suggest, the antioxidant capacity V. officinalis V. teucrium V. orchidea cannot be evaluated by using a single test [35,36]. Thus, the widely used TEAC assay was applied for characterizing the free radical scavenging effects of the three Veronica species (Figure 4a). Additionally, the antioxidants in speedwell 70% ethanolic extracts were assessed using electron spin resonance (ESR) spectrometry to evaluate their efficiency to reduce a synthetic free radical species, i.e., the semi-stable nitroxide radical Fremy's salt (potassium nitrosodisulfonate) (Figures 4b and 5).   antioxidant activity of Veronica species is scarce. However, in a report by Harput et al. [34], a comparison study between fourteen Veronica species indicated V. officinalis had the highest antioxidant activity.
To support the results from the TEAC and Folin-Ciocalteu assays, the three Veronica species were additionally analyzed using EPR with Fremy's salt as stable radical. An important advantage of this assay is the matrix-independent measurement of the reaction between potential antioxidants and radicals in an electromagnetic field instead of the absorbance of light.
The degraded amount of Fremy's salt after 30 min of incubation time ranged between 730.88 ± 1.82 mg FSE/g d.w. for V. officinalis and 398.90 ± 0.99 mg FSE/g d.w. indicating a 68.17% of degradation for the first and just a 37.21% for the latter. Information about the antioxidant activity of Veronica species using the electron paramagnetic resonance (EPR) spectrometry assay is not available, so far. Therefore, a comparison with data from other researchers is lacking.
The antioxidant activity of all analyzed Veronica species evaluated by TEAC assay and EPR assay was also in line with their corresponding total phenolic content, indicating V. officinalis and V. orchidea were superior sources of antioxidant compounds (p < 0.001).

Antimicrobial Activity
The results of antibacterial activity from V. officinalis, V. teucrium and V. orchidea ethanolic extracts and standard antibiotic streptomycin, tested by microdilution assay, are presented in Tables 6 and 7.
In the case of V. officinalis, the most sensitive bacterial strains were Listeria monocytogenes and Listeria ivanovii, with equal values of MIC and MBC of 7.81 mg/mL. Regarding V. teucrium antibacterial activity, the strains of Staphylococcus aureus, Bacillus cereus, Enterococcus faecalis showed the same values for MIC and MBC (7.81 mg/mL), being the most sensitive. Referring to the V. orchidea extract, the most sensitive strains were Listeria monocytogenes and Listeria ivanovii with equal MICs of 3.9 mg/mL and MBCs of 7.81 mg/mL.  The antibacterial activity of sterolic compounds like β-Sitosterol and campesterol has already been demonstrated by Sharma and Mahmood et al. [37,38], and these compounds exhibited a strong antibacterial activity on gram-positive bacteria i.e., S. aureus and S. viridians and a moderate response against gram-negative bacteria like Escherichia coli. As a result of these findings, the activity of Veronica ethanolic extracts against gram-positive bacteria like L. monocytogenes, L. ivanovii and S. aureus could be attributed at least in part to their high β-Sitosterol content but also to the presence of campesterol and stigmasterol. Nevertheless, other constituents of the extract should also be taken into consideration for the global activity, e.g., the high amounts of apigenin, luteolin and their glycosides [28]. The antibacterial activity of Veronica extracts might be influenced also by the presence of hispidulin, as already suggested by Exarchou et al. [31]. The most resistant species to the V. officinalis extract were Bacillus cereus, Pseudomonas aeruginosa and Escherichia coli with equal values of MIC = 15.62 mg/mL and a MBC = 15.62 mg/mL for B. cereus and MBC = 31.25 mg/mL for P. aeruginosa and E. coli. The same bacterial strains were more sensitive to the V. teucrium extract, presenting lower values for their MIC and MBC than V. officinalis extract. As shown in Tables 6 and 7, streptomycin has greater activity than the tested extract.
The obtained results for antibacterial activity are comparable to those previously published for V. montana water extract [39], and also with the ones obtained for V. urticifolia methanolic extract [28], the most sensitive strains in all these cases being S. aureus and L. monocytogenes whilst the most resistant were by B. cereus and P. aeruginosa.

Plant Collection and Sample Preparation
The plant material (Voucher No. 3592, 3593 and 3594) was collected from Romanian spontaneous flora, in the summer of 2014. Voucher specimens were deposited in the Department of Pharmaceutical Botany Herbarium of the Faculty of Pharmacy, "Iuliu Hațieganu" University of Medicine and Pharmacy, Cluj-Napoca, Romania. The vegetal material was dried in a shaded place and stored properly, until the moment of analysis. Two grams were weighed, ground and extracted with 20 mL of 70% ethanol, twice for 30 min in an ultrasonic bath at room temperature. The samples were then centrifuged at 4000 rpm for 30 min, and the supernatant was recovered, filtered through a 0.45 μm micropore membrane (PTFE, Waters, Milford, MA, USA) and subjected to further analysis.
In order to obtain more accurate data on flavonoid glycosides and aglycones concentration, each sample was analyzed before and after acid hydrolysis. Two milliliters of extractive solution were treated with 2 M hydrochloric acid (2 mL) and ascorbic acid solution (0.2 mL, 100 mg·mL −1 ), and the mixtures were heated at 80 °C on a water bath for 30 min, ultrasonicated for 15 min, and heated for another 30 min at 80 °C. During the heating, 70% ethanol (1 mL) was added to the extraction mixture every 10 min, in order to ensure the permanent presence of solvent. The mixtures were centrifuged at 4000 rpm and the solutions were diluted with distilled water in a 10 mL volumetric flask and filtered through a 0.45 μm filter before injection [26,32].
For the antimicrobial activity evaluation, the obtained extract was evaporated to dryness under reduced pressure at <30 °C and re-suspended in 1 mL of bi-distilled water.

HPLC-MS Analysis of Phenolic Compounds
The identification and quantification of polyphenolic compounds was carried out using an Agilent Technologies 1100 HPLC Series system (Agilent, Santa Clara, CA, USA) equipped with G1322A degasser, G13311A binary gradient pump, column thermostat, G1313A autosampler and G1316A UV detector. The HPLC system was coupled with an Agilent 1100 mass spectrometer (LC/MSD Ion Trap SL). For the separation, a reverse-phase analytical column was employed (Zorbax SB-C18 100 × 3.0 mm i.d., 3.5 μm particle) and the work temperature was set at 48 °C. The detection of the compounds was performed in both UV and MS mode. The UV detector was set at 330 nm until 17.5 min, then at 370 nm. The MS system operated using an electrospray ion source in the negative mode. ChemStation and DataAnalysis software from Agilent were used for processing the chromatographic data. The mobile phase was a binary gradient: methanol and acetic acid 0.1% (v/v). The elution started with a linear gradient, beginning with 5% methanol and ending at 42% methanol, for 35 min; then 42% methanol for the next 3 min. The flow rate was 1 mL·min −1 and the injection volume was 5 μL.
The MS signal was used only for qualitative analysis based on the specific mass spectra of each polyphenol. Later, the MS traces/spectra of the analyzed samples were compared to spectra from library, which allows positive identification of compounds, based on spectral match. The UV trace was used for quantification of identified compounds from MS detection. For all compounds, the limit of quantification was 0.5 μg/mL, and the limit of detection was 0.1 μg/mL. Calibration curves in the 0.5-50 μg/mL range with good linearity (R 2 > 0.999) for a five point plot were used to determine the concentration of polyphenols in the analyzed samples. In all analyzed samples the compounds were identified by comparison of their retention times and recorded electro-spray mass spectra with those of standards in the same chromatographic conditions [23][24][25][26]32].

HPLC-MS Analysis of Methoxylated Flavones
The separation of the methoxylated flavones was achieved using a Zorbax SB-C18 reversed-phase analytical column (100 × 3.0 mm i.d., 3.5 μm particle) operated at 48 °C. The mobile phase consisted in 0.1% (v/v) acetic acid and methanol with the following gradient: beginning with 45% methanol and ending at 50% methanol, in 8 min, with a flow rate of 0.9 mL/min and an injection volume of 5 μL. Mass spectrometry analysis was performed on an Agilent Ion Trap 1100 VL mass spectrometer with an electrospray ionization (ESI) source, in the negative mode. For the MS analysis the following optimized conditions were used: gas (nitrogen) temperature 325 °C at a flow rate of 12 L/min, nebulizer pressure 60 psi and capillary voltage +2500 V. The ions monitorized in the MS method are presented in Table 2 The full identification of compounds was performed by comparing the retention times and mass spectra with those of standards in the same chromatographic conditions. To avoid or limit the background interference, the multiple reactions monitoring analysis mode was used instead of single ion monitoring (e.g., MS/MS instead of MS). ChemStation (vA09.03) and DataAnalysis (v5.3) from Agilent, USA were used for the acquisition and analysis of chromatographic data.

HPLC-MS Analysis of the Phytosterols
Compounds were separated using a Zorbax SB-C18 reversed-phase analytical column (100 × 3.0 mm i.d., 5 μm particle) fitted with a guard column Zorbax SB-C18, both operated at 40 °C. Sterols were separated under isocratic conditions using a mobile phase consisting of 10:90 (v/v) methanol and acetonitrile. The flow rate was 1 mL/min and the injection volume was 5 μL. Mass spectrometry analysis was performed on an Agilent Ion Trap 1100 VL mass spectrometer with atmospheric pressure chemical ionization (APCI) interface. The instrument was operated in positive ion mode. Operating conditions were optimized in order to achieve maximum sensitivity values: gas temperature (nitrogen) 325 °C at a flow rate of 7 L/min, nebulizer pressure 60 psi and capillary voltage −4000 V. The full identification of compounds was performed by comparing the retention times and mass spectra with those of standards in the same chromatographic conditions. To avoid or limit the background interference, the multiple reactions monitoring analysis mode was used instead of single ion monitoring (e.g., MS/MS instead of MS). Calibration curves were obtain from standard solutions at different concentration levels, selected as representative of the range of concentration in the sample. Regression analysis of various concentrations of standard solutions (0.08-8 μg/mL) gave good correlation coefficients for the calibration curves of sterols. The software ChemStation (vA09.03) and DataAnalysis (v5.3) from Agilent, USA were used for the acquisition and analysis of chromatographic data [32].

Determination of Total Phenolic Content
The total phenolic content (TPC) of the extracts was measured using the Folin-Ciocâlteu method with some modifications. Two milliliters from each ethanolic extract were diluted 25 times and then mixed with Folin-Ciocâlteu reagent (1 mL) and distilled water (10 mL) and diluted to 25 mL with a 290 g/Lsolution of sodium carbonate. The samples were incubated in the dark for 30 min. The absorbance was measured at 760 nm, using a Jasco UV-VIS spectrophotometer. A standard curve was prepared by using different concentrations of gallic acid and the absorbances were measured at 760 nm. TPC values were determined using an equation obtained from the calibration curve of gallic acid (R 2 = 0.999). Total polyphenolic content was expressed as mg gallic acid equivalents/g dry material plant (mg GAE/g plant material) [26,40].

Determination of Total Flavonoid Content
The total flavonoid content was calculated and expressed as quercetin equivalents after the method described in the Romanian Pharmacopoeia (10th Edition) for Cynarae folium. Each extract (5 mL) was mixed with sodium acetate (5 mL, 100 g/L), aluminum chloride (3 mL, 25 g/L), and made up to 25 mL in a calibrated flask with methanol. Each solution was compared with the same mixture without reagent. The absorbance was measured at 430 nm. The total flavonoid content values were determined using an equation obtained from calibration curve of the quercetin graph (R 2 = 0.999) (Tămaș et al., 2009) [41].

Trolox Equivalent Antioxidant Capacity (TEAC)
The effects of extract on the synthetic ABTS radical were estimated by the method previously described by Toma et al. [26]2015 with some modifications. In the Trolox equivalent antioxidant capacity (TEAC) assay, the antioxidant capacity is reflected in the ability of the natural extracts to decrease the color, reacting directly with the ABTS cation radical. The latter was obtained by oxidation of 2,2′-azinobis(3-ethylbenzothiazoline-6-sulfonic acid (ABTS) with potassium persulfate. Original extracts were diluted appropriately, and 3 μL from the diluted extract were added to 997 μL ABTS solution. The amount of ABTS radical consumed by the tested compound was measured at 734 nm, after 30 min of reaction time, with 70% ethanol (vehicle) as negative control. The evaluation of the antioxidant capacity was obtained using the total change in absorbance at this wavelength.

EPR Measurements
EPR measurements were carried out by the method previously described by Mocan et al. [24] with some modifications. Appropriate extract dilutions (1:400) were prepared and 25 μL aliquots were allowed to react for 30 min with an equal volume of a solution of Fremy's salt (1 mM in phosphate buffer, pH 7.4). EPR spectra of Fremy's radical were obtained with a Bruker Elexsys E500 spectrometer (Bruker, Billerica, MA, USA). The antioxidant activity expressed as mg Fremy's salt equivalents reduced by 25 μL diluted extract was calculated by comparison with a control reaction with 25 μL Fremy's salt and 25 μL of extraction solvent.

Microdilution Method
The modified microdilution technique was used to evaluate antimicrobial activity. Bacterial species were cultured overnight at 37 °C in Tryptic Soy Broth (TSB) medium. The bacterial cell suspensions were adjusted with sterile saline to a concentration of approximately 3 × 10 5 CFU/mL in a final volume of 100 μL per well. The inoculum was stored at +4 °C for further use. Dilutions of the inoculum were cultured on solid Muller-Hinton (MH) for bacteria to verify the absence of contamination and to check the validity of the inoculum. Determinations of minimum inhibitory concentrations (MICs) were made using a serial dilution technique using 96-well microtitre plates. Different dilutions of ethanolic extract were carried out over the wells containing 100 μL of Tryptic Soy Broth (TSB) and afterwards, 10 μL of inoculum was added to all the wells. The microplates were incubated for 24 h at 37 °C. The MIC of the samples was detected following the addition of 20 μL (0.2 mg/mL) of resazurin solution to each well, and the plates were incubated 2 h at 37 °C. A change from blue to pink indicates reduction of resazurin and therefore bacterial growth. The MIC was defined as the lowest extract concentration that prevented this color change. The minimum bactericidal concentrations (MBCs) were determined by serial subcultivation of a 2 μL into microtitre plates containing 100 μL of broth per well and further incubation for 48 h at 37 °C. The lowest concentration with no visible growth was defined as MBC, indicating a 99.5% kill rate for the original inoculum. Streptomycin (Sigma P 7794, Santa Clara, CA, USA) (0.05-3 mg/mL) was used as positive control for bacterial growth. A 10% solution of ethanol in water was used as negative control.

Statistical Analysis
A statistical approach was designed and the experimental data were evaluated using one-way analysis of variance (ANOVA), with p < 0.05 as threshold for statistical significance. The statistical results confirm the hypothesis that the differences between the results are either not significant (p > 0.05), significant (0.001 < p < 0.05) or highly significant (p < 0.001). The average of multiple measurements (triplicates) was listed in the tables together with the standard deviations. Statistical analysis was performed using the Excel software package.

Conclusions
In the present study, V. officinalis, V. teucrium and V. orchidea were investigated for their chemical composition, antioxidant and antimicrobial effects. These species showed marked phenolic and sterolic content, and among the determined compounds, p-coumaric acid, ferulic acid, luteoline, hispidulin and β-sitosterol were dominant. More than that, hispidulin, eupatorin and eupatilin were detected for the first time in the Veronica genus. Nevertheless, representatives of Veronica genus were never investigated related to their content in phytosterols. V. officinalis and V. orchidea extracts presented similar antioxidant capacities related to their phenolic content whilst the values registered for V. teucrium extract were lower. Concerning the antimicrobial potential of the investigated species, Staphylococcus aureus, Listeria monocytogenes and Listeria ivanovii were the most sensitive strains with MIC values between 3.9 and 15.62 mg/mL. The results of this study bring new perspectives for further pharmaceutical and nutraceutical development of Veronica species as natural sources of bioactive compounds with antioxidant and antimicrobial potential. However, further studies are necessary in order to elucidate the mechanisms of in vivo antioxidant action, bioavailability and the involved metabolic pathways.