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Article

Application of Deep Eutectic Solvents for the Extraction of Carnosic Acid and Carnosol from Sage (Salvia officinalis L.) with Response Surface Methodology Optimization

by
Martina Jakovljević
1,
Stela Jokić
1,
Maja Molnar
1 and
Igor Jerković
2,*
1
Faculty of Food Technology Osijek, Josip Juraj Strossmayer University of Osijek, Franje Kuhača 18, 31000 Osijek, Croatia
2
Faculty of Chemistry and Technology, University of Split, Ruđera Boškovića 35, 21000 Split, Croatia
*
Author to whom correspondence should be addressed.
Plants 2021, 10(1), 80; https://doi.org/10.3390/plants10010080
Submission received: 4 November 2020 / Revised: 24 December 2020 / Accepted: 24 December 2020 / Published: 2 January 2021
(This article belongs to the Special Issue Structural and Functional Analysis of Extracts in Plants)
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Abstract

:
Salvia officinalis L. is a good source of antioxidant compounds such as phenolic diterpenes carnosic acid and carnosol. From 17 deep eutectic solvents (DESs) used, choline chloride: lactic acid (1:2 molar ratio) was found to be the most suitable for the extraction of targeted compounds. The influence of H2O content, extraction time, and temperature (for stirring and heating and for ultrasound-assisted extraction (UAE)), H2O content, extraction time, and vibration speed for mechanochemical extraction on the content of targeted compounds were investigated. Carnosic acid content obtained by the extraction assisted by stirring and heating was from 2.55 ± 0.04 to 14.43 ± 0.28 µg mg−1, for UAE it was from 1.62 ± 0.29 to 14.00 ± 0.02 µg mg−1, and for mechanochemical extraction the yield was from 1.80 ± 0.02 to 8.26 ± 0.45 µg mg−1. Determined carnosol content was in the range 0.81 ± 0.01 to 4.83 ± 0.09 µg mg−1 for the extraction with stirring and for UAE it was from 0.56 ± 0.02 to 4.18 ± 0.05 µg mg−1, and for mechanochemical extraction the yield was from 0.57 ± 0.11 to 2.01 ± 0.16 µg mg−1. Optimal extraction conditions determined by response surface methodology (RSM) were in accordance with experimentally demonstrated values. In comparison with previously published or own results using conventional solvents or supercritical CO2, used DES provided more efficient extraction of both targeted compounds.

1. Introduction

The growth of the pharmaceutical industry and increased need for bioactive components has led to the increased development of new extraction and isolation methods [1]. The most important differences between these methods are better efficiency and shorter extraction time for modern techniques compared to the conventional ones. Furthermore, conventional solvents are very often flammable and toxic with their manufacture depending on fossil resources [2]. However, there are also certain issues associated with the modern techniques, such as poor selectivity and solubility of targeted components in the solvents used, such as H2O, ethanol, or CO2, as well as recovery of bioactive components and their chemical changes during the extraction period due to the reactions such as ionization, hydrolysis, and oxidation [3,4]. Over the past few years, deep eutectic solvents (DESs), first proposed by Abbott et al. [5,6], have been developed as analogues of ionic liquids (ILs), although they differ from them in the starting material and the method of preparation. DESs are mixtures of hydrogen bond acceptor (HBA) and hydrogen bond donor (HBD) with a lower melting point relative to the starting components. Their green character is also attributed to their low price, easy preparation, biodegradability, and low toxicity [7]. In addition to these properties, different studies reported that DES could dissolve several components better than organic solvents, due to dissolving lignocellulose which causes damage of plant cell wall and strengthens the mass transfer process [8]. DESs can be prepared from different combinations of the starting compounds, thus being tunable solvents with different functionality and solubility for various compounds. Therefore, a suitable combination of the starting solvents and their molar ratio can increase the solubility and the extraction efficiency of DESs for desired compounds [9]. However, their shortcomings should also be taken into account with an emphasis on viscosity and low vapor pressure which makes it difficult to isolate and purify desired components. In addition, high viscosity complicates industrial application due to the high energy consumption needed to ensure their liquid state [10].
One of the most commonly used HBA is choline chloride (ChCl), since it is an inexpensive, biodegradable, and non-toxic quaternary ammonium salt. ChCl can form DES with different nontoxic components as carboxylic acids, sugars, sugar alcohols, or amines which act as HBDs [5,6]. In the last few years, deep eutectic solvents are increasingly used for the extraction of phenolic compounds including phenolic acids, flavonoids, stilbenes, anthocyanins, and furanocoumarins [1,2,11,12,13]. In the research performed by Bi et al. [11] DESs were used to extract flavonoids such as myricetin and amentoflavone from Chamaecyparis obtusa (Siebold and Zucc.) Endl. leaves by alcohol-based DESs. Wang et al. [13] extracted polyphenols and furanocoumarins from fig (Ficus carica L.) with tailor-made DESs and showed that DESs were effective for the extraction of these components. Anthocyanins in the flower petals of Catharanthus roseus L. were extracted with natural deep eutectic solvents (NADESs) such as lactic acid—glucose and propane-1,2-diol—choline chloride, which provided higher stability for anthocyanins [12]. The extraction with DES can be improved by combination with ultrasound (UAE), microwaves and heating as well as by mechanochemical extraction (MCE). Therefore, Bosiljkov et al. [14] successfully extracted anthocyanins with UAE combined with DESs. Wang et al. [4] developed fast, efficient, and ecofriendly MCE for tanshinones as well as bioactive compounds from tea leaves [15]. Due to the desirability of DESs in the extraction of phenolic components, we decided to extract phenolic diterpenes, carnosic acid, and carnosol from sage (Salvia officinalis L.) applying DESs. These compounds have been suggested to account for over 90% of the sage antioxidant properties [16]. In addition to antioxidant activity, carnosic acid, and carnosol showed proapoptotic [17], antiproliferative [18], anti-angiogenic [19] and antitumor activity. So far, there are no available data on DESs extraction and optimization of the parameters for carnosic acid and carnosol from sage. There are few reports dealing with DESs extraction of sage by Bakirtzi et al. [2] and Georgantzi et al. [20] who investigated the influence of different DESs on the extraction of polyphenols from medicinal plants including sage. In paper by Bakirtzi et al. [2] lactic acid-based natural deep eutectic solvents in combination with ultrasound were used for the extraction of total polyphenols and flavonoids from sage, while Georgantzi et al. [20] investigated combination of lactic acid-based DES with cyclodextrin for UAE of total polyphenols and flavonoids.
Taking into account all the above mentioned, the objectives of this study were focused on (1) investigation on finding appropriate choline chloride based deep eutectic solvent for the extraction of carnosic acid and carnosol as well as (2) suitable extraction techniques (stirring with heating, UAE or MCE). Afterwards, the influence of various DES extraction parameters (H2O content, time, and temperature for stirring and heating and UAE; H2O content, extraction time and vibration speed for mechanochemical extraction) on the (3) content of carnosic acid and carnosol in sage extract analyzed by HPLC was investigated. In addition, (4) the optimal extraction conditions by RSM for desired antioxidant components (carnosic acid and carnosol) were determined.

2. Results and Discussion

2.1. Influence of DESs on the Obtained Amount of Carnosic Acid and Carnosol in the Extracts

Due to the different effects of viscosity, surface tension, polarity, and HBD interaction it is hard to estimate the suitability of a DES for the extraction of targeted compounds. Therefore, in order to select the best DES for the extraction of carnosic acid and carnosol from sage, the extraction was performed with different solvents and different H2O addition at 30 °C (Figure A1). According to Dai et al. [12] and Bosiljkov et al. [14], H2O addition in organic acid-based DESs causes decrease of the solvent polarity since these solvents are more polar than H2O. Therefore, for targeted components it would be more suitable to lower H2O addition (which is consistent with the results obtained). As can be seen from Figure A1, the solvents substantially differ in their ability to extract carnosic acid and carnosol. In addition to the influence of HBD, the amount of H2O added also plays an important role for the extraction efficiency. For certain solvents, like choline chloride:malonic acid (1:1 molar ratio), the amount of carnosic acid was increased with increased H2O content that may be due to the viscosity lowering effect. For DES choline chloride:citric acid (1:1 molar ratio), the highest amount of carnosic acid and carnosol was obtained with 30% H2O addition that may be the consequence of a high viscosity of the solvent with 10% H2O addition. H2O amount was changed to reduce the viscosity which causes a slow mass transfer, thus affecting the extraction process. The viscosity of DESs can be reduced by the addition of a certain amount of H2O as well as by increasing the temperature [12]. Several solvents such as choline chloride:glucose (1:1 molar ratio) were too viscous even with the addition of H2O at 50% (v/v). Although the addition of H2O can decrease the viscosity, an excessive concentration of H2O can decrease the interactions between the components of DES as well the interactions between DES and desired components [11]. This is the reason why the focus was on H2O addition in the range of 10–50% (v/v).
Carnosol can be extracted with all DESs applied, but choline chloride based DESs with butane-1,4-diol (1:2 molar ratio) (ChClB) and ethane-1,4-diol (1:2 molar ratio) (ChClE) were the most effective. The result of extraction with choline chloride:glucose (1:1 molar ratio) with 10% H2O were not shown because of the high viscosity preventing further analysis. The same limitation was observed with choline chloride:fructose (1:1 molar ratio) (ChClF) and choline chloride:citric acid (1:1 molar ratio) (ChClC) at 10% of H2O and at 30 °C. The higher amount of carnosol was observed at lower H2O content (Figure A1). With choline chloride:urea (1:2) (ChClU) as the solvent, the highest amount of carnosol was extracted at 30 °C. According to the literature, higher content of carnosol is usually present in the extracts obtained at higher temperatures since it is one of the degradation products of carnosic acid [20].
On the other hand, not all applied solvents could extract carnosic acid. Basic solvents, such as ChCl:U, choline chloride:N-methlyurea (1:3 molar ratio) (ChClmU), and choline chloride:thiourea (1:2 molar ratio) (ChCltU), were not efficient for carnosic acid extraction. The highest amount of carnosic acid was extracted using acidic DESs, with emphasis on choline chloride:lactic acid (1:2 molar ratio) (ChClLa). Such solvents are significantly acidic (pH < 3) compared to the solvents where HBDs were sugars or alcohols (pH > 6) [7,12]. Additionally, the polarity of DESs should also be considered as an important criterion for the evaluation and selection of the solvents to achieve maximum extraction efficiency. Carnosic acid and carnosol are polar constituents, soluble in polar solvents (which is in agreement with the obtained results), such as DESs with organic acids as HBDs, which are more polar than the DESs with sugars as HBDs [12]. The highest amount of carnosic acid was obtained with the lowest amount of added H2O (10%) in most solvents. Okamura et al. [21] have investigated the effect of temperature on the degradation of carnosic acid in acetone solution and reported that the increase of temperature affected the degradation of carnosic acid. In case of the extraction with DESs such as ChClLa and choline chloride:levulinic acid (1:2 molar ratio) (ChClL) the maximum amount of carnosic acid was extracted at 30 °C.
Since carnosol can be extracted with all DESs applied and due to the highest amount of extracted carnosic acid in the case of choline chloride:lactic acid (1:2 molar ratio) and the lactic acid properties as natural component, this solvent was selected for further optimization of the extraction with three extraction methods (stirring and heating, UAE, and MCE).

2.2. Comparison of the Used Extraction Methods

After selection of the appropriate solvent, the extractions performed by stirring and heating and UAE, applying the same temperature and H2O content as well as MCE were compared. Both, stirring and heating and UAE increase mass transfer and speed up diffusion of the compounds. In the case of ultrasound, acoustic cavitation phenomenon leads to the disruption of cell walls and consequently improves the yield of extraction compared to maceration [22]. However, MCE can decrease the processing time and solvent consumption and reduce noise and radiation compared to UAE and to stirring and heating extraction.
Table 1 shows that slightly higher amounts of carnosol and carnosic acid were extracted by stirring and heating, compared to UAE. Such results can be explained by the positive influence of stirring on the mass transfer in such viscous solvent. For MCE, the utilization of the glass beads led to much better mixing of the plant material and solvent, thus extracting significant amounts of carnosic acid and carnosol in a shorter time compared to the other two extractions (Table 2).
For the constant H2O content in all extraction methods, the extracted amounts of carnosic acid and carnosol obtained by different extractions were compared. The extracted amounts of selected compounds (8.26 and 7.92 µg mg−1 for carnosic acid and 1.87 and 2.02 µg mg−1 for carnosol) obtained by MCE at Run 12 and 17 can be compared to Run 6 and 9 obtained with stirring and heating extraction and UAE. The difference between the parameters of these extractions was the extraction time, so at 10% H2O for MCE, 2 min were enough to obtain similar amounts of targeted compounds as for 30 min of stirring and heating extraction and UAE. In the case of 30% H2O by MCE, 3 min were sufficient to obtain the amount of extracted components similar to the amount extracted for 90 min by stirring and heating extraction and UAE. It is important to note that MCE was carried out at room temperature (24–28 °C). In fact, by using mill, we wanted to show how much time was needed for the extraction at room temperature, and prolonging the extraction time would result in warming of the samples without the possibility of heating control.

2.3. Influence of Various DES Extraction Parameters on the Content of Carnosol and Carnosic Acid

The effect of H2O addition, temperature or vibration speed and extraction time on carnosol and carnosic acid was investigated for three extraction techniques using DES choline chloride:lactic acid (1:2 molar ratio). In these experiments, the content of carnosic acid in sage extract obtained by stirring and heating was 2.55–14.43 µg mg−1, depending on the applied extraction parameters. The lowest content of carnosic acid was obtained at 50% (v/v) H2O added at 30 °C and 60 min, while the highest content was obtained at 10% (v/v) H2O added at 50 °C and 90 min (Table 1). The content of carnosic acid obtained by UAE varied, depending on the parameters used, in the range 1.62–13.99 µg mg−1. The lowest content of carnosic acid was obtained at 30% (v/v) H2O added, 70 °C, and 30 min and the highest yield at 10% (v/v) H2O added, 70 °C and 60 min (Table 1). The content of carnosic acid obtained by MCE varied depending on the parameters used in the range 1.80–8.26 µg mg−1. The lowest content of carnosic acid was at 50% (v/v) H2O added, vibration speed of 1 m/s and 2 min and the highest yield at 10% (v/v) H2O added, 5 m/s and 2 min (Table 2). The content of carnosol obtained by mixing and heating was 0.81–4.83 µg mg−1 depending on the applied extraction parameters. The lowest content of carnosol was obtained at 50% (v/v) H2O addition, 50 °C and 30 min, while the highest yield was obtained at 10% (v/v) of H2O, 50 °C and 90 min. The content of carnosol, depending on the parameters used in UAE, was 0.56–4.18 µg mg−1 with the lowest content at 30% (v/v) H2O addition, 30 °C and 30 min and the highest yield at 10% H2O addition, 70 °C and 60 min (Table 1). The content of carnosol obtained by MCE was 0.57–2.02 µg mg−1 depending on the applied extraction parameters (Table 2). The lowest content of carnosol was obtained at 50% of H2O (v/v), vibration speed of 1 m/s and time of 1 min, while the highest content was obtained at 30% of H2O (v/v), 5 m/s and 3 min.
The addition of H2O and extraction time (Figure 1 and Table A1) showed statistically significant influence on the content of carnosic acid (p < 0.0001; p = 0.0202) in the extracts obtained by stirring and mixing. The content of carnosic acid increased with prolonged extraction time and decreased with the increase of H2O amount.
The interactions between amount of H2O added and extraction time (p = 0.0259) also showed a significant influence on the content of carnosic acid. In the extracts obtained by UAE, H2O addition and temperature showed statistically significant influence on the content of carnosic acid (p = 0.0025; p = 0.0144). For this extraction technique, interactions between the amount of added H2O and temperature (p = 0.0433) also showed a significant influence in terms of content of carnosic acid. The content of carnosic acid increased with increased extraction temperature and decreased with the increase of H2O amount. In the extracts obtained by MCE, H2O addition, time, and vibration speed (p = 0.0006; p = 0.0266; p = 0.0002) as well as the interactions between H2O addition and vibration speed (p = 0.0221) showed statistically significant influence on the content of carnosic acid. The content of carnosic acid increased with prolonged extraction time and vibration speed and decreased with the increase of H2O amount.
As can be seen from Figure 2 and Table A2, H2O addition, extraction time, and temperature showed statistically significant influence on the content of carnosol (p < 0.0001; p = 0.0008; p = 0.0003) in the extracts obtained by stirring and mixing. The content of carnosol is increased with increased time and temperature of the extraction and with decreased H2O amount.
Interactions between amount of H2O added and the extraction time and between the amount of H2O added and temperature (p = 0.0184; p = 0.0234) also showed a significant influence for the content of carnosol. In the extracts obtained by MCE, H2O addition, time, and vibration speed (p = 0.0055; p = 0.0187; p = 0.0012) showed statistically significant influence on the content of carnosol. The content of carnosol increased with prolonged extraction time and vibration speed and decreased with the increase of H2O amount. Since model according to RSM is not significant for the extraction of carnosol with ultrasound (p = 0.0708), the results obtained for that extraction are not discussed. To optimize the extraction conditions of two different phenolic diterpenes 17 runs determined by BBD with three variables (percentage of H2O added, time and temperature or vibration speed) at three levels were used to fit a second-order response surface. The amount of carnosic acid and carnosol were observed as the response (Table A1 and Table A2).
The data describing the optimal conditions for the extraction of carnosic acid and carnosol from sage using DESs are not available in the literature, but there are few papers investigating the optimal conditions with other solvents. In paper by Fatma Ebru et al. [23] it was shown that 70% of ethanol was the most efficient solvent since it extracted 3.45 mg carnosol + carnosic acid per g of the extract. According to the optimization carried out, they showed that the amount of these bioactive components was in the function of extraction time. In addition, they also demonstrated that carnosol and carnosic acid degraded easily at higher temperatures over a longer period of time. Therefore, they have shown that the optimum conditions were temperatures of 40–50 °C, the extraction time 3–6 h, solvent-to-sage ratio 6:1 (v/w) and 70–80 wt.% ethanol for maceration. Similar results were also showed in paper by Durling et al. [24]. According to the optimization carried out, the amount of targeted components depended on several parameters such as particle size, temperature, time, and a solvent-to-sage ratio. The highest concentration of targeted components was obtained with the particle size 1 mm, 40 °C, the extraction time of 3 h, the solvent-to-sage ratio of 6:1 (v/w) and 55–75 wt.% ethanol. Under these conditions, the extract containing 10.6% carnosic compounds was obtained.
The optimization process of extraction is important for determining the most favorable conditions for achieving maximum yields of desired components in the extracts. Based on BBD, estimated coefficients of second order response models for carnosol and carnosic acid in sage extracts are given in Table A1 and Table A2. R2 for carnosic acid was 0.9630 and for carnosol was 0.9607 in the extracts obtained by stirring and heating, and for UAE R2 for carnosic acid was 0.8660. In the case of MCE, R2 for carnosic acid was 0.9442 and for carnosol R2 was 0.9032. According to ANOVA, statistically significant models for carnosic acid (Table A3) and carnosol in the extraction by stirring and heating (Table A4) (p ≤ 0.05) were obtained. Additionally, the obtained models showed non-significant lack of fit (p = 0.2042–0.4491), except in the case of MCE for carnosic acid (p = 0.0008).
According to RSM, optimum conditions are expressed as those at which it is possible to achieve the maximum amount of carnosic acid and carnosol. They are slightly different depending on the extraction technique used, so for the extraction with heating and mixing they were 10% H2O addition, 90 min and 70 °C, while for UAE they were 11.05% of H2O addition, 82.36 min and 69.84 °C. Under these optimal conditions, the content of carnosic acid and carnosol was calculated as 14.20 µg mg−1 and 6.47 µg mg−1 in case of stirring and heating and 14.72 µg mg−1 of carnosic acid for ultrasound extraction. The desirability for these optimizations was 0.990 and 1.0, respectively. The experimental results for the amount of carnosic acid and carnosol obtained at optimum conditions were 13.73 ± 0.26 and 6.15 ± 0.33 µg mg−1 for the extraction with stirring and heating, while for UAE this amount was 14.24 ± 0.21 µg mg−1. Optimum conditions for MCE were 11.13% H2O addition, time of extraction 2.90 min, and vibration speed 4.98 m s−1. Under these optimal conditions, the content of carnosic acid and carnosol is calculated as 8.95 µg mg−1 and 2.02 µg mg−1 with the desirability 1.0 which was confirmed experimentally (8.90 ± 0.10; 2.03 ± 0.04 µg mg−1).

2.4. Comparison with Other Extraction Methods

According to the literature, the most common solid–liquid extraction of sage has been performed with methanol. Due to the toxic effect of methanol, it is preferable to use ethanol which can be classified as bio-solvent and is much safer for the use [25,26]. In the paper by Abreu et al. [27] the content of carnosic acid and carnosol in methanolic extract of sage was 14.6 mg g−1 of dry weight and 0.4 mg g−1, respectively. This is similar to our results for Run 2 (mixing and heating) and Run 3 (UAE), but with a significantly higher amount of carnosol in our case. Sage extraction with 80% methanol over 24 h at room temperature led to the extraction of carnosic acid only with the content of 273.8 mg 100 g−1 of the plant dry weight [28], much lower than our results. In other case, the extraction with 50% methanol during 60 min in ultrasound bath has brought carnosic acid content of 2.1 g kg−1 extract and carnosol content of 4.1 to 15.1 mg g−1 of plant dry weight [29].
According to Table 3, which shows our results obtained by the stirring with heating extraction of the same sage material with common solvents, it is observed that the most effective solvent is absolute ethanol, while H2O is the least effective solvent for the extraction of carnosic acid and carnosol. The preparation of aqueous solutions of ethanol in the range of 30–70% (v/v) shows that the increase in the volume of ethanol (v/v) increased the amount of extracted components. In this case, methanol as the extraction solvent shows lower extraction efficiency compared to ethanol. In addition, the influence of extraction parameters such as extraction time and temperature can be observed in Table 3. However, when ethanol is used as the extraction solvent and with the most efficient extraction conditions applied (50 ° C and 90 min), lower amount of carnosic acid and carnosol was obtained compared to the selected DES (choline chloride:lactic acid 1:2).
Considering the adverse properties of organic solvents and in order to overcome their disadvantages, such as low selectivity for antioxidant compounds [30], safe or green solvents and processes have been used. Supercritical fluid extraction (SFE) has been used in the plant material extraction due to its ability to provide clean extracts without residual solvent [31]. In addition, SFE can be performed at low temperatures in short time, which is suitable for carnosic acid oxidation prevention during the extraction, also supported by the absence of air and light during the extraction process thus reducing its degradation [32]. In our previous work [33] we used the same herbal material for carnosic acid and carnosol extraction using SFE with CO2 (SC-CO2). Comparing the results, the highest amount of extracted carnosic acid using SC-CO2 was 855.8 mg 100 g−1 of the plant material (30 MPa, 50 °C, 1 kg h−1 CO2), while the extraction yield using DESs was 1443.22 mg 100 g−1 and 1399.22 mg 100 g−1, depending on the extraction technique employed. In the case of carnosol, the highest amount was extracted under the same conditions of SC-CO2 (446.35 mg 100 g−1), and similar results were achieved using DESs (483.34 and 418.39 mg 100 g−1 of plant, depending on the extraction technique employed). However, certified reference material was not used and therefore minor changes in the composition of the plant material are possible with respect to the same sample used in our previously published data. In the paper published by Babovic et al. [34] the content of carnosic acid obtained by SC-CO2 was 13.76 g per 100 g of the extract and carnosol content was 6.97 g per 100 g of the extract similar to our results (11.63 g carnosic acid per 100 g and 8.55 g carnosol per 100 g) [32]. Despite the fact that SC-CO2 extraction conditions may reduce carnosic acid degradation, we still notice that more carnosic acid was extracted and preserved by DESs extraction even at higher extraction temperatures. On the other hand, preparing DESs is simple and inexpensive, i.e., the price is comparable to the cost of the conventional solvents. Moreover, this is sustainable process theoretically without generated waste [10] which makes this extraction process suitable for the extraction of bioactive components including carnosic acid and carnosol.

3. Materials and Methods

3.1. Chemicals

The standard compounds carnosic acid (≥95.0%) and carnosol (99.2%) (Sigma Chemical Co., St. Louis, MO, USA) were used for the chemical analyses. All solvents were of analytical grade and purchased from J.T. Baker (Avantor, Phillipsburg, NJ, USA).

3.2. Plant Material

Dried sage leaves (Salvia officinalis L.) were used for experiments. Prior to the extraction, the dried leaves were grounded and sieved using a vertical vibratory sieve shaker (LabortechnikGmbh, Ilmenau, Germany) as described in paper by Jokić et al. [35].

3.3. Preparation of DES

The choline chloride based DESs were prepared as described in our paper [36]. In this study, seventeen different choline chloride based DESs were prepared using inexpensive components as shown in Table 4.

3.4. Extraction of Carnosic Acid and Carnosol with DESs

Grounded Salvia officinalis L. dried leaves (50 mg) were mixed with 1 mL of the selected solvent, a pure DES or a mixture of DES and ultrapure H2O (Millipore Simplicity 185, Darmstadt, Germany). Prepared samples were stirred at 1500 rpm in aluminum block (Stuart SHB) on a magnetic stirrer or ultrasound treated in temperature-controlled ultrasonic bath at specified temperature for the certain time (Table 1). The temperature-controlled ultrasonic bath (Elma P70 H, Singen, Germany) was set with frequency at 37 Hz and power at 50 W at the same temperature over the same time as in case of mixing in aluminum block (Table 1). Prepared samples (50 mg of plant + 1 g of glass beads with 1 mL of solvent) were also extracted on the BeadRuptor 12 ball mill (Omni International, Kennesaw, GA, USA) according to parameters in Table 2 at room temperature (24–28 °C). After the extraction, the mixture was centrifuged for 15 min and then decanted. The supernatant liquid was then diluted with methanol, filtered through a PTFE 0.45 μm filter, and subjected to HPLC analysis.

3.5. Extraction of Carnosic Acid and Carnosol with Conventional Solvents

Grounded Salvia officinalis L. dried leaves (50 mg) were mixed with 1 mL of selected solvent (Millipore Simplicity 185, Darmstadt, Germany). Prepared samples were stirred at 1500 rpm in aluminum block (Stuart SHB) on a magnetic stirrer at specified temperature for the certain time (Table 3).

3.6. Chemical Characterization of the Extracts

HPLC analyses of carnosic acid and carnosol was performed on an Agilent 1260 Infinity II (Agilent, Santa Clara, California, USA) with chromatographic separation obtained on a ZORBAX Eclipse Plus C18 (Agilent, Santa Clara, CA, USA) column (100 × 4.6 mm, 5 µm).
The separation of analyzed compounds was made with method described in our previous paper [31], but since analysis was performed on different device, linearity of the calibration curve, LOQ and LOD was confirmed. Standard stock solutions for carnosic acid and carnosol were prepared in a methanol and calibration was obtained at eight concentrations (concentration range 10.0, 20.0, 30.0, 50.0, 75.0, 100.0, 150.0, and 200.0 mg L−1). Due to R2 = 0.99789 for carnosic acid and R2 = 0.99968 for carnosol, calibration curve was confirmed. Limit of detection were 0.795 mg L−1 and 0.971 mg L−1 for carnosic acid and carnosol, respectively. Limit of quantification were 2.648 mg L−1 and 7.416 mg L−1 for carnosic acid and carnosol, respectively. Retention time for carnosic acid was 7.416 min, while for carnosol was 4.217 min. The chromatograms of the standard and real sample are shown in the Appendix A (Figure A2). For the validation of the HPLC method for the determination of carnosic acid and carnosol, in addition to linearity, retention time comparison and absorption spectrum comparison with standards, repeatability of measurements and solution preparation as well as accuracy were performed, which is also shown in the Appendix A (Table A5).

3.7. Statistical Experimental Design

BBD explained in detail by Bas and Boyaci [37] was used for determination of optimal DES (stirring and heating), UAE-DES and MCE-DES extraction conditions in terms of getting higher amount of carnosic acid and carnosol in the S. officinalis extracts. Independent variables in design were H2O content (X1), time (X2) and temperature (X3) and vibration speed (X3) and tested levels were reported in Table 5. Design-Expert® Commercial Software (ver. 9, Stat-Ease Inc., Minneapolis, MN, USA) was used for data analysis. The analysis of variance (ANOVA) was also used to evaluate the quality of the fitted model, and the test of statistical difference was based on the total error criteria with a confidence level of 95.0%.

4. Conclusions

In present study, determination of suitable deep eutectic solvent and optimization of the extraction of carnosol and carnosic acid from sage were performed. Among 17 different solvents, choline chloride:lactic acid (1:2 molar ratio) was selected for the extraction by heating and mixing, as well as for ultrasound and mechanochemical extraction. The content of carnosic acid and carnosol was slightly higher in the extracts obtained by stirring and heating and mechanochemical extraction. The influence of H2O content, extraction time and temperature (for stirring and heating and for ultrasound-assisted extraction (UAE)), H2O content, extraction time and vibration speed for mechanochemical extraction on the content of targeted compounds were investigated. Optimal extraction conditions determined by response surface methodology (RSM) were in accordance with experimentally demonstrated values.
Compared to SC-CO2 extraction, we observed that more carnosic acid is extracted using DESs, with emphasis on ChClLa, while the amount of carnosol detected in the extract obtained by ChClLa is similar to that obtained by SC-CO2. In addition, the comparison with the solvents such as ethanol, H2O, aqueous solutions of ethanol (30–70% (v/v)) and methanol under the same extraction conditions, showed that choline chloride:lactic acid (1:2 molar ratio) was more efficient for the extraction of carnosic acid and carnosol compared to used conventional solvents.
Given the amounts of carnosic acid achieved at high temperatures in DES in further research it would be useful to examine the stability of the component over the certain period of time.

Author Contributions

Conceptualization, M.M. and M.J.; methodology, M.J., S.J., M.M., and I.J.; formal analysis, M.J. and S.J.; investigation, M.J. and M.M.; resources, I.J.; data curation, M.M.; writing—original draft preparation, M.J.; writing—review and editing, S.J., M.M., and I.J.; visualization, S.J., M.M., and I.J.; supervision, M.M., S.J., and I.J.; funding acquisition, I.J. All authors have read and agreed to the published version of the manuscript.

Funding

This research was funded by Croatian Government and the European Union (European Regional Development Fund—the Competitiveness and Cohesion Operational Programme—KK.01.2.2.03) for funding this research through project CEKOM 3LJ (KK.01.2.2.03.0017), granted to Institution for research and knowledge development of nutrition and health CEKOM 3LJ.

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

The data presented in this study are available from the authors.

Acknowledgments

We would like to thank Croatian Government and the European Union (European Regional Development Fund—the Competitiveness and Cohesion Operational Programme—KK.01.2.2.03.0017) for funding this research through project CEKOM 3LJ (KK.01.2.2.03.0017), granted to Institution for research and knowledge development of nutrition and health CEKOM 3LJ.

Conflicts of Interest

The authors declare no conflict of interest.

Appendix A

Table
Table A1. Regression coefficient of polynomial function of all response surfaces for carnosic acid.
Table A1. Regression coefficient of polynomial function of all response surfaces for carnosic acid.
TermsCoefficientsStandard ErrorF-Valuep-Value
Carnosic acid (stirring)
Intercept4.930.42
X1−3.970.33145.190.0001
X20.980.338.950.0202
X30.400.331.490.2619
X121.600.4512.510.0095
X220.710.452.460.1608
X320.280.450.390.5530
X1X2−1.310.477.940.0259
X1X30.460.470.980.3562
X2X30.470.471.000.3495
R2= 0.9630
Carnosic acid (UAE)
Intercept4.760.87
X1−3.170.6921.240.0025
X21.080.692.450.1617
X32.220.6910.450.0144
X121.390.952.140.1871
X22−0.520.950.300.6019
X32−0.570.950.370.5645
X1X2−0.340.970.120.7349
X1X3−2.390.976.060.0433
X2X31.460.972.240.1780
R2= 0.8660
Carnosic acid (MCE)
Intercept3.440.28
X1−1.340.2235.660.006
X20.630.227.820.0266
X31.590.2250.460.0002
X12−0.380.311.500.2608
X220.160.310.270.6209
X321.050.3111.490.0116
X1X20.0660.320.0430.8409
X1X3−0.930.328.560.0221
X2X30.540.322.950.1294
R2 = 0.9442
Table
Table A2. Regression coefficient of polynomial function of all response surfaces for carnosol.
Table A2. Regression coefficient of polynomial function of all response surfaces for carnosol.
TermsCoefficientsStandard ErrorF-Valuep-Value
Carnosol (stirring)
Intercept2.150.16
X1−1.070.1370.760.0001
X20.720.1331.740.0008
X30.860.1345.540.0003
X12−0.0930.180.280.6146
X220.220.181.520.2580
X320.260.182.260.1768
X1X2−0.550.189.340.0184
X1X3−0.220.181.480.2630
X2X30.520.188.340.0234
R2= 0.9607
Carnosol (MCE)
Intercept1.090.077
X1−0.240.06115.650.0055
X20.190.0619.280.0187
X30.320.06127.850.0012
X12−0.180.0844.610.0690
X220.0290.0840.120.7436
X320.210.0846.330.0401
X1X26.381 × 10−30.0865.511 × 10−30.9429
X1X3−0.0960.0861.260.2988
X2X30.0740.0860.740.4189
R2= 0.9032
Table
Table A3. Analysis of variance (ANOVA) of the modelled responses for carnosic acid.
Table A3. Analysis of variance (ANOVA) of the modelled responses for carnosic acid.
SourceSum of SquaresDegree of FreedomMean SquareF-Valuep-Value *
Carnosic acid (mixing)
The recovery
Model157.64917.5220.220.0003
Residual6.0670.87
Lack of fit3.9231.312.440.2042
Pure error2.1440.54
Total163.7016
Carnosic acid (UAE)
The recovery
Model171.12919.015.030.0224
Residual26.4873.78
Lack of fit13.9934.661.490.3444
Pure error12.4943.12
Total197.6016
Carnosic acid (MCE)
The recovery
Model47.4995.2813.170.0013
Residual2.8170.40
Lack of fit2.7530.9264.440.008
Pure error0.05740.014
Total50.3016
*p < 0.01 highly significant; 0.01 ≤ p < 0.05 significant; p ≥ 0.05 not significant.
Table
Table A4. Analysis of variance (ANOVA) of the modelled responses for carnosol.
Table A4. Analysis of variance (ANOVA) of the modelled responses for carnosol.
SourceSum of SquaresDegree of FreedomMean SquareF-Valuep-Value *
Carnosol (mixing)
The recovery
Model22.2892.4819.040.0004
Residual0.9170.13
Lack of fit0.4130.141.090.4491
Pure error0.5040.13
Total23.1916
Carnosol (UAE)
The recovery
Model18.2992.033.180.0708
Residual4.4870.64
Lack of fit2.8130.942.240.2256
Pure error1.6740.42
Total22.7716
Carnosol (MCE)
The recovery
Model1.9390.217.260.0080
Residual0.2170.030
Lack of fit0.1730.055
Pure error0.04240.010
Total2.1416
*p < 0.01 highly significant; 0.01 ≤ p < 0.05 significant; p ≥ 0.05 not significant.
Table
Table A5. HPLC method validation parameters.
Table A5. HPLC method validation parameters.
Carnosic Acid
(µg mg−1)		Mean Value
(µg mg−1)		SDRSD (%)Carnosol
(µg mg−1)		Mean Value
(µg mg−1)		SDRSD (%)
Repeatability of measurements100.406100.390.430.43%99.999
100.042100.004
100.913100.100
100.84299.947
100.30599.977
99.83199.987100.000.050.05%
Repeatability of solution preparation 104.65107.462.402.24%102.231
108.45101.996
109.22103.260
109.09102.161
109.24101.677
104.13101.996102.220.540.53%
Added amount of carnosic acid (µg mg−1)Expected value of carnosic acid (µg mg−1)Obtained value of carnosic acid (µg mg−1)Recovery (%)Added amount of carnosol (µg mg−1)Expected value of carnosol (µg mg−1)Obtained value of carnosol (µg mg−1)Recovery (%)
AccuracySample 10.36 6.50
Sample + std 1 (1:1)22.57016.46116.42699%21.32913.91513.21395%
Sample + std 2 (1:1)100.40655.38555.79799%99.94753.22352.99999%
Sample + std 3 (1:1)212.859111.608107.04996%209.221107.860106.99599%
Plants 10 00080 g0a1 550
Figure A1. Carnosol and carnosic acid content obtained by stirring and heating with DESs depending on the temperature and H2O content (n = 3). The columns represent determined amount of carnosol and carnosic acid in the samples, and the color of the column indicates DES used according to the abbreviations recorded in the legend to the right and Table 4.
Figure A1. Carnosol and carnosic acid content obtained by stirring and heating with DESs depending on the temperature and H2O content (n = 3). The columns represent determined amount of carnosol and carnosic acid in the samples, and the color of the column indicates DES used according to the abbreviations recorded in the legend to the right and Table 4.
Plants 10 00080 g0a1
Plants 10 00080 g0a2 550
Figure A2. Obtained chromatogram of carnosol and carnosic acid standards (picture above) and chromatogram of real sample (picture below).
Figure A2. Obtained chromatogram of carnosol and carnosic acid standards (picture above) and chromatogram of real sample (picture below).
Plants 10 00080 g0a2

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Plants 10 00080 g001a 550Plants 10 00080 g001b 550
Figure 1. Three-dimensional plots for obtained content of carnosic acid as a function of the extraction time, temperature, and H2O content for the extraction with mixing and heating (a,b), UAE (c,d) and for the extraction time, vibrational speed, and H2O content for MCE (e,f).
Figure 1. Three-dimensional plots for obtained content of carnosic acid as a function of the extraction time, temperature, and H2O content for the extraction with mixing and heating (a,b), UAE (c,d) and for the extraction time, vibrational speed, and H2O content for MCE (e,f).
Plants 10 00080 g001aPlants 10 00080 g001b
Plants 10 00080 g002 550
Figure 2. Three-dimensional plots for obtained content of carnosol as a function of the extraction time, temperature, and H2O content in the extraction with mixing and heating (a,b) and MCE (c,d).
Figure 2. Three-dimensional plots for obtained content of carnosol as a function of the extraction time, temperature, and H2O content in the extraction with mixing and heating (a,b) and MCE (c,d).
Plants 10 00080 g002
Table
Table 1. Experimental matrix and values (µg mg−1 of the plant material) of observed response for the extraction with choline chloride:lactic acid (1:2 molar ratio) obtained by stirring with heating and by ultrasound-assisted extraction (UAE). The results are expressed as mean value ± standard deviation (n = 3).
Table 1. Experimental matrix and values (µg mg−1 of the plant material) of observed response for the extraction with choline chloride:lactic acid (1:2 molar ratio) obtained by stirring with heating and by ultrasound-assisted extraction (UAE). The results are expressed as mean value ± standard deviation (n = 3).
RunH2O
(%)		Time
(min)		Temperature
(°C)		DES-MIXINGDES-UAE
Carnosic Acid
(µg mg−1)		Carnosol
(µg mg−1)		Carnosic Acid
(µg mg−1)		Carnosol
(µg mg−1)
13060503.86 ± 0.821.99 ± 0.057.37 ± 0.343.06 ± 0.21
210905014.43 ± 0.284.83 ± 0.099.94 ± 0.223.92 ± 0.09
310607010.16 ± 0.053.90 ± 0.3714.00 ± 0.024.18 ± 0.05
43060504.53 ± 0.492.27 ± 0.094.18 ± 0.212.22 ± 0.14
53060505.16 ± 0.452.70 ± 0.175.04 ± 0.052.46 ± 0.29
61030508.71 ± 0.262.10 ± 0.068.48 ± 0.063.34 ± 0.10
73030705.64 ± 0.112.51 ± 0.221.62 ± 0.290.70 ± 0.02
85090503.16 ± 0.141.34 ± 0.212.09 ± 0.370.84 ± 0.29
93090707.41 ± 0.064.79 ± 0.388.06 ± 0.132.93 ± 0.02
1010603010.68 ± 0.662.35 ± 0.032.66 ± 0.410.83 ± 0.38
115060703.87 ± 0.191.85 ± 0.153.69 ± 0.241.85 ± 0.11
125030502.68 ± 0.260.81 ± 0.012.00 ± 0.070.82 ± 0.13
133060505.65 ± 0.361.99 ± 0.094.37 ± 0.092.25 ± 0.17
145060302.55 ± 0.040.89 ± 0.031.94 ± 0.210.92 ± 0.09
153060505.44 ± 0.211.79 ± 0.112.46 ± 0.051.27 ± 0.16
163090305.27 ± 0.181.70 ± 0.082.80 ± 0.251.22 ± 0.12
173030305.37 ± 0.011.50 ± 0.192.18 ± 0.230.56 ± 0.02
Table
Table 2. Experimental matrix and values (µg mg−1 of the plant material) of observed response for the extraction with choline chloride:lactic acid (1:2 molar ratio) obtained by mechanochemical extraction (MCE). The results are expressed as mean value ± standard deviation (n = 3).
Table 2. Experimental matrix and values (µg mg−1 of the plant material) of observed response for the extraction with choline chloride:lactic acid (1:2 molar ratio) obtained by mechanochemical extraction (MCE). The results are expressed as mean value ± standard deviation (n = 3).
RunH2O
(%)		Time
(min)		Vibration Speed
(m s−1)		Carnosic Acid
(µg mg−1)		Carnosol
(µg mg−1)
130313.50 ± 0.351.25 ± 0.02
230233.38 ± 0.201.23 ± 0.06
350332.51 ± 0.340.86 ± 0.02
450132.01 ± 0.160.71 ± 0.04
550252.98 ± 0.021.03 ± 0.13
610334.29 ± 0.251.16 ± 0.04
750211.80 ± 0.020.57 ± 0.11
810213.37 ± 0.171.02 ± 0.20
910134.06 ± 0.261.04 ± 0.37
1030154.69 ± 0.611.27 ± 0.11
1130233.31 ± 0.421.01 ± 0.09
1210258.26 ± 0.451.87 ± 0.33
1330233.63 ± 0.181.14 ± 0.01
1430233.45 ± 0.281.09 ± 0.12
1530112.45 ± 0.070.79 ± 21
1630233.41 ± 0.240.98 ± 0.03
1730357.92 ± 0.292.02 ± 0.14
Table
Table 3. The values (µg mg−1 of the plant material) of carnosic acid and carnosol for the extraction obtained by stirring with heating. The results are expressed as mean value ± standard deviation (n = 3).
Table 3. The values (µg mg−1 of the plant material) of carnosic acid and carnosol for the extraction obtained by stirring with heating. The results are expressed as mean value ± standard deviation (n = 3).
SolventTime
(min)		Temperature
(°C)		Carnosic Acid
(µg mg−1)		Carnosol (µg mg−1)
30% ethanol (v/v)30301.11 ± 0.032.63 ± 0.21
601.33 ± 0.552.26 ± 0.02
901.45 ± 0.532.18 ± 0.20
30502.32 ± 0.072.04 ± 0.05
602.64 ± 0.041.99 ± 0.04
902.26 ± 0.301.51 ± 0.00
30702.82 ± 0.032.92 ± 0.16
602.13 ± 0.142.92 ± 0.311
900.93 ± 0.172.27 ± 0.38
50% ethanol (v/v)30305.91 ± 0.194.65 ± 0.22
603.07 ± 0.399.31 ± 0.29
903.02 ± 0.159.73 ± 0.86
30507.17 ± 0.058.39 ± 0.47
603.15 ± 0.029.06 ± 0.11
902.11 ± 0.1511.25 ± 0.35
30707.63 ± 0.446.73 ± 0.38
604.43 ± 0.208.79 ± 0.79
901.91 ± 0.0011.23 ± 0.13
70% ethanol (v/v)30308.28 ± 0.533.04 ± 0.01
607.40 ± 0.054.82 ± 0.29
907.63 ± 0.05.93 ± 0.22
30507.73 ± 0.226.17 ± 0.59
608.54 ± 0.287.21 ± 0.44
908.71 ± 0.285.43 ± 0.51
30708.73 ± 0.144.37 ± 0.07
607.53 ± 0.066.55 ± 0.22
906.85 ± 0.326.89 ± 0.26
ethanol303011.21 ± 0.512.72 ± 0.27
6011.13 ± 0.133.57 ± 0.25
9012.77 ± 0.222.83 ± 0.06
305011.74 ± 0.093.57 ± 0.47
6012.80 ± 0.193.14 ± 0.06
9013.64 ± 0.103.47 ± 0.01
307013.36 ± 0.374.46 ± 0.11
6012.27 ± 0.113.29 ± 0.21
9011.27 ± 0.053.11 ± 0.09
methanol30308.71 ± 0.872.88 ± 0.48
609.26 ± 0.064.44 ± 0.19
9010.50 ± 0.584.69 ± 0.58
30509.68 ± 0.255.03 ± 0.08
6011.85 ± 0.055.24 ± 0.07
9010.72 ± 0.304.85 ± 0.40
30709.69 ± 0.583.67 ± 0.24
6010.11 ± 0.434.41 ± 0.10
9010.41 ± 0.124.80 ± 0.03
H2O30300.000.00
600.000.24 ± 0.00
900.000.24 ± 0.00
30 0.000.29 ± 0.01
60 0.000.27 ± 0.00
90 0.75 ± 0.030.24 ± 0.00
30 0.000.26 ± 0.03
60 0.000.25 ± 0.01
90 0.74 ± 0.000.42 ± 0.02
Table
Table 4. Preparation of deep eutectic solvents (DESs).
Table 4. Preparation of deep eutectic solvents (DESs).
NameCombinationMolar Ratio
ChClUCholine chloride:urea1:2
ChClmUCholine chloride:N-methylurea1:3
ChCltUCholine chloride:thiourea1:2
ChClGCholine chloride:glucose1:1
ChClFCholine chloride:fructose1:1
ChClXCholine chloride:xylitol1:1
ChClSCholine chloride:sorbitol1:1
ChClBCholine chloride:butane-1,4-diol1:2
ChClECholine chloride:ethane-1,2-diol1:2
ChClGlCholine chloride:glycerol1:2
ChClACholine chloride:acetamide1:2
ChClMCholine chloride:malic acid1:1
ChClCCholine chloride:citric acid1:1
ChClMaCholine chloride:malonic acid1:1
ChClOCholine chloride:oxalic acid1:1
ChClLaCholine chloride:lactic acid1:2
ChClLCholine chloride:levulinic acid1:1
Table
Table 5. Coded and real levels of independent variables for the designed experiment.
Table 5. Coded and real levels of independent variables for the designed experiment.
Type of ExtractionIndependent VariableSymbolLevel
Low (−1)Middle (0)High (+1)
Stirring and heatingH2O (%)X1103050
Time (min)X2306090
Temperature (°C)X3305070
Ultrasound assisted extractionH2O (%)X1103050
Time (min)X2306090
Temperature (°C)X3305070
Mechanochemical extractionH2O (%)X1103050
Time (min)X2123
Vibration speed (ms−1)X3135
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Jakovljević, M.; Jokić, S.; Molnar, M.; Jerković, I. Application of Deep Eutectic Solvents for the Extraction of Carnosic Acid and Carnosol from Sage (Salvia officinalis L.) with Response Surface Methodology Optimization. Plants 2021, 10, 80. https://doi.org/10.3390/plants10010080

AMA Style

Jakovljević M, Jokić S, Molnar M, Jerković I. Application of Deep Eutectic Solvents for the Extraction of Carnosic Acid and Carnosol from Sage (Salvia officinalis L.) with Response Surface Methodology Optimization. Plants. 2021; 10(1):80. https://doi.org/10.3390/plants10010080

Chicago/Turabian Style

Jakovljević, Martina, Stela Jokić, Maja Molnar, and Igor Jerković. 2021. "Application of Deep Eutectic Solvents for the Extraction of Carnosic Acid and Carnosol from Sage (Salvia officinalis L.) with Response Surface Methodology Optimization" Plants 10, no. 1: 80. https://doi.org/10.3390/plants10010080

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