The standards used were chlorogenic acid, p-coumaric acid, caffeic acid, rutin, apigenin, quercetin, isoquercitrin, hyperoside, kaempferol, quercetol, myricetol, fisetin, gallic acid, aucubin, catalpol, harpagoside, β-sitosterol, brassicasterol, stigmasterol, campesterol and ergosterol from Sigma–Aldrich (Germany), ferulic acid, sinapic acid, gentisic acid, patuletin, luteolin from Roth (Germany), caftaric acid from Dalton (United States), harpagide, 8-O-acetyl-harpagide from PhytoLab GmbH & Co. (Germany). Methanol of HPLC analytical-grade, acetonitrile of HPLC analytical-grade, ammonium acetate of HPLC analytical-grade, silver nitrate of HPLC analytical-grade, chloroform, petroleum ether, n-hexane, potassium hydroxide of analytical-grade and hydrochloric acid of analytical-grade, acetic acid of analytical-grade, Folin–Ciocâlteu reagent were purchased from Merck (Germany). Sodium carbonate, Copper (II) sulfate pentahydrate, sodium acetate trihydrate and anhydrous aluminum chloride were acquired from Sigma–Aldrich (Germany). The DPPH (2,2-diphenyl-1-picrylhydrazyl), Trolox (6-hydroxy-2,5,7,8-tetramethylchroman-2-carboxylic acid) were obtained from Alfa-Aesar (Karlsruhe, Germany), HRP (horseradish peroxidase), Fremy’s salt were purchased from Sigma–Aldrich (Germany).

Methanolic stock solutions (100 mg/mL) of the flavonoid standards were prepared and stored at 4°C, protected from daylight. They were appropriately diluted with double distilled water before being used as working solutions. Methanolic stock solutions of iridoids (1 mg/mL) were prepared and stored at 4°C, protected from daylight. They were appropriately diluted with double distilled water before being used as working solutions. Chloroform stock solutions (1 mg/mL) of the phytosterol standards were prepared and stored at 4°C, protected from daylight. Before being used as working solutions, they were appropriately diluted with acetonitrile. Distilled, deionised water was produced by a Direct Q-5 Millipore (Millipore SA, Molsheim, France) water system.

Ajuga laxmannii aerial parts were collected from Cluj County (Romania) spontaneous flora during flowering stage in June 2015. The air-dried powder of herbal material was extracted with different solvents. The methanol extract was obtained from 5 g herbal material and 50 mL 70% methanol for 30 min on a water bath at 60°C (Methanol Extract, ME). The 10% tincture was prepared at room temperature from 100 g of herbal material and 1000 mL 70% ethanol by maceration at room temperature for 7 days (Ethanol Extract, EE) as previously described by Toiu et al. (2017). In order to evaluate the anti-inflammatory activity of A. laxmannii aerial parts, three extracts were used: A. laxmannii ethanol extract 100% (100 mg dry weight herbal material/mL), A. laxmannii ethanol extract 50% (50 mg dw herbal material/mL), and A. laxmannii ethanol extract 25% (25 mg dw herbal material/mL).

For identification and quantification of phytosterols, and for determination of antifungal properties, chloroform (CE) and petroleum ether extracts (PEE) were also prepared. Thus, 2.5 g of herbal material were extracted with 25 mL chloroform and 25 mL petroleum ether, respectively, for 30 min in a sonication bath at 60°C. The extracts were cooled down, and then centrifuged at 4500 rpm for 15 min, and the supernatant was recovered (Mocan et al., 2014).

For testing the antioxidant capacity, the A. laxmannii extracts were further tested using three different assays.

Targeted A. laxmannii iridoids (aucubin, catalpol, harpagide, harpagoside, and 8-O-acetylharpagide) were analyzed by HPLC-MS on a Agilent 1100 liquid chromatography system equipped with a binary pump, autosampler, thermostat and detector (all 1100 Series from Agilent Inc., United States). The system was controlled with Data Analysis software (version B01.03, Agilent Inc., United States). The separation was carried out on an Atlantis HILIC 3.5 μm (100 mm × 3.0 mm i.d.) (Waters Inc., United States) column equipped with an online 0.2 μm filter (Agilent Inc.), at a working temperature of 40°C, a flow rate of 0.75 mL/min and an injection volume of 8 μL. A binary gradient system with eluent (A) 0.1% acetic acid (v/v) and 20 μM sodium acetate in water, and eluent (B) 0.1% acetic acid (v/v) and 20 μM sodium acetate in acetonitrile was used for the analyzed samples with the following gradient: 95–80% B (0–5 min). The HPLC system was coupled with an Agilent Ion Trap 1100 SL mass spectrometer equipped with an electrospray ionisation (ESI) source and operated in the positive mode with a scan range between 360 and 680 m/z. The newly developed LC-ESI-MS/MS method was used to identify the targeted compounds based on their sodium adducts (M+23 m/z): aucubin (369 m/z), catalpol (385 m/z), harpagide (387.2 m/z), harpagoside (517.4 m/z) and 8-O-acetylharpagide (429.3 m/z), and by comparison with standards in the same chromatographic conditions. The capillary voltage was set to 4 kV and the capillary temperature to 300°C. Nitrogen (N₂) was used as dry gas with a dry flow of 12 L/min and a pressure of 60 psi for the nebulizer. For quantification of the iridoids, stock solutions of the five commercially available standards substances were prepared in acetonitrile, and different concentrations of each standard were used. All calibration curves yielded a coefficient of determination of R² ≥ 0.990. The results are expressed as μg per mL of extract (μg/mL). All phytochemical assays were performed in triplicate.

To investigate the antifungal activities of A. laxmannii extracts, the following fungi were used: Aspergillus flavus (ATCC 9643), Aspergillus niger (ATCC 6275), Candida albicans (ATCC 10231), Candida parapsilosis (ATCC 22019) and Penicillium funiculosum (ATCC 56755). These fungi were obtained from the Food Biotechnology Laboratory, Life Sciences Institute, University of Agricultural Sciences and Veterinary Medicine Cluj-Napoca, Romania. Cultures were maintained on malt agar at 4°C and subcultured every month. Spore suspension (1.0 × 10⁵ CFU/mL) was obtained by washing agar plates with sterile solution containing [0.85% saline, 0.10% Tween 80 (v/v)], then added to each well to a final volume of 100 μL. Inocula were screened for contamination by culturing on a solid medium. The minimum inhibitory (MIC) and minimum fungicidal (MFC) concentrations assays were determined using the microdilution method by preparing a serial of dilutions in 96-well microtiter plates. The extracts (EE, PEE, CE) were diluted in 0.85% saline (10 mg/mL), then added to microplates containing Broth Malt medium with inoculum and incubated for 72 h at 28°C on a rotary shaker. The lowest concentrations without visible growth (at the binocular microscope) were defined as MICs. The MFCs were determined by serial sub-cultivation of 2 μL of tested extracts dissolved in medium and inoculated for 72 h, into microtiter plates containing 100 μL of broth per well and further incubation 72 h at 28°C. The lowest concentration with no visible growth was defined as MFC indicating 99.5% killing of the original inoculum. The fungicide fluconazole was used as positive control (1–3500 μg/mL). All the experiments were performed in duplicate and repeated three times (Stana et al., 2017).

All results were expressed as the mean ± SD. Otherwise, the median and first quartile (Q1) and third quartile (Q3) were reported. Statistical comparisons between two independent groups were performed using the Student’s t-test (with equal and unequal variances, depending upon to the results of the F-test) for normally distributed data. Mann–Whitney’s test was used for non-parametric data. Pearson and Spearman’s correlation analyses were used to calculate statistical relationships between parameters. A p-value < 0.05 was considered as statistically significant. Analyses were performed using SPSS 16.0 for Windows (SPSS Inc., United States).

Various studies showed that phenolic compounds are widely distributed in the Ajuga species and these compounds could contribute to their antioxidant activity. In this part, a preliminary comparative overview of the total phenolic, flavonoid and iridoid contents of the different extracts of the A. laxmannii is presented. The TPC is presented in Table 1 and was 67.68 ± 1.57 mg GAE/g dw for ethanol extract, and 56.76 ± 0.92 mg GAE/g dw for methanol extract. The TPC values of analyzed A. laxmannii aerial parts extracts were higher than those obtained previously for A. reptans flower extracts (20.86 ± 0.53 and 24.11 ± 0.57 mg GAE/g dw, for methanol and ethanol extracts, respectively) by Toiu et al. (2017). Another study performed by Movahhedin et al. (2016) revealed that ethanol extract of Ajuga chamaecistus subsp. scoparia (Boiss.) Rech.f. aerial parts (6.5 g extract obtained from 50 g plant material) had a TPC value of 20.32 ± 0.39 mg GAE/g extract (representing 2.64 mg GAE/g dw), and the water extract had TPC values of 18.94 ± 0.13 mg GAEs/g extract, which is lower than both previously considered Ajuga species.

The TFC for ethanol extract of A. laxmannii (36.14 ± 0.53 mg RE/g dw), was lower than the one reported for the ethyl acetate, methanol and acetone extract of A. chamaepitys (L.) Schreb (91.76 ± 0.81, 63.87 ± 0.66, and 61.77 ± 0.51 mg RE/g, respectively), and considerably higher than the water extract from same species (9.32 ± 0.33 mg RE/g) (Jakovljević, 2015). However, a clear comparison between the results of the present study is rather impossible, due to different extraction protocols and ways of expressing results.

In previous studies, Toiu et al. (2017) found a TFC value of 12.38 ± 0.22 mg RE/g dw for a methanol extract of A. reptans flowers.

Concerning the TIC of different species of Ajuga, the available data is limited. In a former research on A. reptans flowers, Toiu et al. (2017) revealed that the methanol extract content in iridoids is lower than ethanol extract from the same species (22.17 ± 0.89 vs. 27.49 ± 0.94 mg AE/g dw). The same trend was observed in this study for the A. laxmannii, the TIC being 15.37 ± 0.77 and 16.28 ± 0.85 mg AE/g dw for methanol and ethanol extract, respectively.

In order to determine the polyphenolic compounds from A. laxmannii extracts, an optimized HPLC/MS method for the identification and quantification of 18 polyphenols was employed. The A. laxmannii extracts contain one caffeic acid derivative (chlorogenic acid), corresponding to peak 1, with m/z 353, three flavonoid glycosides (isoquercitrin, rutin, and quercitrin), corresponding to peaks 2, 3, and 4, with m/z 463, 609, and 447, respectively. Additionally, two free aglycones (luteolin and apigenin), with m/z 285 and 279, corresponding to peaks 5 and 6 were identified.

The HPLC chromatogram of A. laxmannii ethanol extract (Figure 1), and the amounts of polyphenols identified in the analyzed extracts expressed as μg/g dw are presented (Table 2).

Rutin, an important flavonoid glycoside, was the major compound found in a significant quantity, both in ethanol and methanol extract (6883.48 ± 9.12 and 6721.49 ± 8.92 μg/g dw, respectively). Various studies showed the effectiveness of rutin in various diseases such as inflammatory bowel disease and Alzheimer’s disease (Kim et al., 2005; Xu et al., 2014). Another flavonoid glycoside compound which was found and quantified in ethanol and methanol A. laxmannii extracts was isoquercitrin, which is known to have good anti-inflammatory effects (Rogerio et al., 2007). The quantities obtained are significant lower than those obtained for rutin, but still important (685.35 ± 5.72 and 636.1 ± 5.44 μg/g dw), for ethanol and methanol extracts, respectively.

Considering the correlation between the type of the extract and the quantity of a particular compound, with one exception, all extracts showed similar values. Only in case of luteolin, the methanol extract showed a lower value than the ethanol extract (88.24 ± 1.09 vs. 122.27 ± 1.14 μg/g dw).

Under the proposed chromatographic conditions, retention times of the five analyzed sterols were: 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 3. In the ionization conditions all sterols have lost a water molecule, therefore the ions detected by the mass spectrometer are always in the form [M-H₂O+H]⁺.

The pseudo-molecular ions of 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 determination because the intensity of ions in the mass spectrum is proportional to the concentration of the substance in the sample.

In order to quantify the five sterols from A. laxmannii extracts (EE, PEE, CE), we have constructed the extracted chromatograms for each compound, taking into account the intensity of major ions in the mass spectrum (Table 3).

Calibration curves were obtained 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. Concentrations of phytosterols in A. laxmannii extracts are presented in Table 4. Significant differences between the three A. laxmannii extracts were observed: all five sterols were identified in CE, whereas the EE contains β-sitosterol, stigmasterol, ergosterol and brassicasterol and PEE contains campesterol, stigmasterol, ergosterol and brassicasterol. The A. laxmannii CE was the richest in phytosterols, with β-sitosterol as major compound in very high concentration (11589.96 ± 8.66 μg/mL), while in EE it was found in smaller quantities (367.24 ± 2.97 μg/mL), and in PEE campesterol was the main sterol (598.04 ± 4.22 μg/mL). The concentrations of stigmasterol, ergosterol, and brassicasterol were comparable in all three extracts. To the best of our knowledge, this is the first report on phytosterols from A. laxmannii aerial parts extracts. Previous studies showed the presence of stigmasterol and β-sitosterol in other Ajuga species, such as A. bracteosa, A. relicta, A. taiwanensis (Israili and Lyoussi, 2009).

Iridoids are important compounds for the genus Ajuga, and many Ajuga species contain the iridoid glycoside harpagide (Manguro et al., 2011; Mamadalieva et al., 2013). The main known ethnopharmacological indications for Ajuga species are oedema, hypertension, fever, intestinal and biliary disorders, ulcer, they are used as antipyretic, diuretic, and astringent (Toiu et al., 2017), and several studies have shown that iridoid glycosides in Ajuga species are linked to this therapeutic effects (Makni et al., 2013; Hailu and Engidawork, 2014). The HPLC-MS results from the present study show the characterization of Ajuga laxmannii aerial parts in five commercially available iridoid glycosides, namely aucubin, catalpol, harpagide, harpagoside, and 8-O-acetylharpagide. From a pharmaceutical point of view, the concentrations of the compounds determined in plant extract cannot be neglected as they are directly linked to their pharmaceutical efficacy and effectiveness. 8-O-acetylharpagide was the major compound found in ethanol extract (266.3 ± 3.92 μg/mL extract), followed by harpagide (87.4 ± 2.39 μg/mL extract). The concentrations of aucubin and catalpol (7.2 ± 0.41 and 3.1 ± 0.23 μg/mL ethanol extract, respectively) were significantly lower than the other iridoids. We observed that A. laxmannii aerial parts ethanol extract contains higher amounts of iridoids than methanol extract (Table 5). As far as one can tell, this is the first report of a rapid, simple and highly accurate HPLC-MS/MS method for the identification and quantification of iridoids from A. laxmannii extracts.

The obtained results for the antibacterial activity of A. laxmannii extracts and gentamicin against Gram+ and Gram- bacteria are presented in Table 7. The antimicrobial effect was measured by microdilution assay, and the determination of MIC (mg/mL) and MBC (mg/mL) was assessed.

The MIC values obtained for the ethanol extract ranged from 0.78 to 6.25 mg/mL, and from 1.56 to 6.25 mg/mL for the methanol extract of A. laxmannii. Against some bacterial strains, such as Pseudomonas aeruginosa, Listeria monocytogenes, Escherichia coli and Salmonella typhimurium, both extracts showed comparable activities. The best antimicrobial activity against S. aureus is associated with A. laxmannii ethanol extract (MIC value = 0.78 mg/mL and MBC value = 1.56 mg/mL). The less susceptible strains were: Listeria monocytogenes, Escherichia coli and Salmonella typhimurium, for both methanol and ethanol extracts. Previous studies showed a similar trend in terms of MIC and MBC for A. reptans (Toiu et al., 2017). According to Salvat et al. (2004), herbal extracts with MIC values less than/around 0.50 mg/mL indicate good antimicrobial effect. Consequently, the results presented herein showed moderate antibacterial activity.

Generally, the bacterial strains were more sensitive to ethanol extract of A. laxmannii. Considering HPLC–MS results presented in this study, we can derive some assumptions regarding antibacterial activity of A. laxmannii aerial parts. The content of polyphenolic compounds in ethanol extract of A. laxmannii was higher than in methanol extract. Many recent investigations confirmed antibacterial and antifungal properties of phenolic compounds from plant origin, among which are the main constituents of examined extracts (rutin and isoquercitrin) (Alves et al., 2013; Stojković et al., 2013). The exerted antibacterial potential of A. laxmannii could be associated with higher level of mentioned phenolic compounds in ethanol extract.

The antifungal activity of the A. laxmannii extracts (EE, PEE, and CE) was tested against a panel of five fungi, selected on the basis of their relevance for public health. The results obtained for the antifungal efficacy of A. laxmannii extracts and fluconazole against tested strains are presented in Table 8. Candida parapsilosis possessed the highest sensitivity to the ethanolic extract of A. laxmannii, with MIC = 0.012 mg/mL and MFC = 0.025 mg/mL. Moreover, Candida albicans and Penicillium funiculosum were similarly susceptible to the inhibitory (MICs = 0.012 mg/mL) and fungicidal effects (MFCs = 0.025 mg/mL) of the chloroform extract. Nonetheless, the most resistant fungal strains were Candida parapsilosis and Candida albicans, toward petroleum ether extract with MFCs 0.5 and 0.2 mg/mL, respectively. According to Kawamura and Ohara (2005), the antifungal activity of plant extracts might be ascribed to the high level of iridoids. Both methanol and ethanol extracts from A. laxmannii aerial parts showed high values for iridoid glycosides, especially for 8-O-acetylharpagide. These results are in accordance to previous studies performed by Makni et al. (2013), who similarly demonstrated the antifungal effect of A. iva extracts.

The anti-inflammatory effects of three A. laxmannii ethanol extract concentrations (25 mg dw/mL, 50 mg dw/mL, and 100 mg dw/mL) were evaluated in vivo on a model turpentine oil-induced inflammation in rats by determining WBC count, differential WBC count, serum total nitrites and nitrates, TOS, TAR and OSI. These three extract dilutions were also evaluated in vitro for the ability to inhibit phagocytosis. The 50 mg dw/mL diluted extract had the best inhibitory activity on phagocytosis and oxidative stress. In conclusion, these results support the hypothesis that extracts from A. laxmannii aerial parts exert anti-inflammatory activities by inhibiting phagocytosis through the reduction of oxidative stress (Table 9).

Compared to the inflammation group, A. laxmannii ethanol extracts significantly reduced (p < 0.001) total WBC count (Figure 2) by lowering PMN% (Figures 3, 4). That was associated with an important decrease of the phagocytosis indices PA (Figure 5) and PI (Figure 6) (p < 0.001). Extracts 50 mg dw/mL and 25 mg dw/mL had the best inhibitory effects (p < 0.001) and this was comparable to diclofenac activity (p > 0.05).

Turpentine-induced inflammation significantly increased (p < 0.001) and treatment with diclofenac significantly reduced (p < 0.001) the TOS (Figure 7). Importantly, the TOS was also reduced by the treatment with all dilutions of the A. laxmannii extract. The inhibitory effects were strongest for the 50 mg dw/mL (p < 0.001) and 25 mg dw/mL (p < 0.01) plant extracts. Diclofenac treatment had a similar effect on TOS inhibition (p < 0.01) compared to treatment with either the 25 mg dw/mL (p < 0.01) or the 50 mg dw/mL (p < 0.01) extract. The A. laxmannii extract had no important effect on TAR (Figure 8) (p > 0.05).

In the inflammation group, the OSI was significantly elevated (p < 0.001), and diclofenac treatment decreased the OSI (p < 0.001) (Figure 9). The 25 mg dw/mL and 50 mg dw/mL extracts of A. laxmannii aerial parts induced a significant decline in OSI (p < 0.001). The 50 mg dw/mL extract was the best OSI inhibitor (p < 0.001). The 50 mg dw/mL (p < 0.001) and 25 mg dw/mL (p < 0.01) A. laxmannii extract dilutions significantly reduced NOx (Figure 10). The OSI correlated with the TOS (r = 0.92) and NOx (r = 0.81).

Compared to diclofenac treatment, A. laxmannii extract had a lower anti-inflammatory and anti-nitro-oxidative stress effect upon all measured parameters (p < 0.001). Among the three extracts, the 50 mg dw/mL A. laxmannii one had the best effect in comparison with diclofenac.