Antioxidant Activity and Bioactive Compounds of Lamium album Flower Extracts Obtained by Supercritical Fluid Extraction

: In this research, supercritical CO 2 extraction is applied to extract bioactive compounds from Lamium album (white dead nettle, Lamiaceae ). Extraction was performed at various temperatures (40, 50, and 60 ◦ C) using methanol as co-solvent at a constant ﬂow rate of CO 2 , methanol, and pressure. The collected extracts were characterized in terms of antioxidant capacity by using DPPH, ABTS and FRAP in vitro antioxidant activity assays, whereas the Folin–Ciocalteu procedure was employed to estimate the total phenols content (TPC). On the other hand, phenolic compounds in the extracts were quantitated by liquid chromatography coupled with a photodiode array detector (UPLC-PDA) and conﬁrmed with a mass detector (TQD). The extracts have shown high TPC ranged between 234.17 to 650.17 mg GAE/g extract. DPPH scavenging of the extracts was estimated and obtained EC50 values ranged from 0.12 to 0.37 mg/mL of solution. The ABTS radical scavenging activity ranged from 43.20 to 44.53 µ g TE/g. The FRAP value was found within the range of 19.48 to 44.74 µ mol TE/g of extract. Differences between extraction conditions were observed. In this research, 50 ◦ C/250 bar was efﬁcient for the TPC, DPPH, ABTS, and FRAP assays; moreover, statistically, TPCs and FRAP assay showed signiﬁcant differences between the conditions at α = 0.05. The identiﬁcation of phenolic compounds in the obtained extract of Lamium album ﬂowers, using UPLC/PDA, revealed that chrysin, pinostrobin, myricetin, and trans -3-hydroxycinnamic acid were the signiﬁcant molecules present, which may be responsible for the high content of polyphenols and antioxidant activity. The results obtained indicated that SC-CO 2 could be considered an alternative method for extracting bioactive compounds of Lamium album . High antioxidant activity and the presence of various bioactive compounds indicate the potential of this plant from the Lamiaceae family and the possibility of its application in various industries, including agriculture, food technology, pharmacy.


Introduction
Plants have been used by humans as both food and medicine since prehistoric times. Currently, there is an interest in the use of bioactive compounds, especially polyphenols, derived from plant materials in food preservation, pharmaceuticals, cosmetics, and natural pesticides. These bioactive compounds can play a preventive or supportive role in the treatment of various metabolic disorders and diseases due to their antioxidant, antimicrobial, anticancer, and anti-inflammatory properties [1]. Lamium album, widely known as nonsting nettle or white dead nettle, is a perennial herbaceous plant with white blooms that is inherent to Europe, Western Asia, and North Africa [2]. It belongs to the Lamiaceae family, which is recognized for producing plant species high in different bioactive compounds that generally differ in structures, biological properties, and mechanisms of action. Furthermore, the genus Lamium contains nearly 40 species; among them, the Lamium album is the most widely distributed species [3]. It has a wide variety of biological activities due to its various phytochemicals such as iridoids, flavonoids, triterpenes, fatty acids, polysaccharides, saponines, phytoecdysteroids, phenolic acids, amines, essential oils, tannins, and mucilage [4]. Flowers and leaves of the Lamium album are considered food for humankind [2]. They can be eaten raw or cooked. It is also used in teas, dietary supplement products, and its intake is primarily connected with its health benefits [2,5]. The dried flowers of this plant have demonstrated uterotonic, astringent, antispasmodic, and anti-inflammatory activities and consequently are used in menorrhagia, uterine hemorrhage, vaginal and cervical inflammation, and leukorrhea treatment [3,6]. Additionally, L. album flowers have been reported to possess antioxidant, free radical scavenging, and antiproliferative properties [3]. Nowadays, the beneficial understanding of natural products has been substantially increased and scientifically proven, allowing a better grasp of their valuable features. Therefore, a significant quantity of information regarding the efficacy of L. album extracts and raw material has been accumulated, and several health-related benefits have been successfully verified. Various studies in vivo or in vitro of Lamium album extracts (methanol, ethyl acetate and heptane, butanol, ethanol, and chloroform) have been done, and their antioxidant, cytoprotective, anticancer, antiviral, antimicrobial, and antiproliferative activities have been reported [5,[7][8][9]. Additionally, bioactive phenolic compounds of this plant were also studied, and the results have shown that the crucial compounds mainly include; phenylpropanoid verbascoside, isoscutellarein derivatives, and isoverbascoside, some phenolic acids such as caffeic acid, ferulic acid, syryngic acid, and flavonoids [4,5]. Various conclusions from the mentioned studies have shown a possible correlation between phenolic compounds and the antioxidant activity of this plant and its natural health benefits [8].
Despite all of the positive attributes claimed to the Lamium album, there are very few publications on L. album, and the data are incomplete. It is vital to carefully study the properties of this plant using modern techniques, including advanced techniques for bioactive extraction such as ultrasound, pulsed electric field, extrusion, microwave heating, ohmic heating, supercritical fluids, and accelerated solvents as they improve the quantity, quality, and selectivity of bioactive components extracted from plant matrix [10] and advanced analytical techniques for identifying and quantitating different bioactive components such as ultrahigh-performance liquid chromatography with photodiode array or/and mass spectrometer (UPLC/PDA or LC/MS/MS), gas chromatography, etc., which have been claimed to be cost-effective, repeatable, accurate, linear, precise, and resilient. However, no unique extraction method is recognized to be the best one for extracting bioactive compounds from plants due to their diversity. Therefore, to optimize the qualitative and quantitative properties of the bioactive compounds, the selection of an appropriate extraction technique and conditions are critical [11].
Supercritical fluid extraction (SFE) is an advanced and environmentally friendly technique used to extract bioactive compounds from different materials. Supercritical CO 2 (SC-CO 2 ) is one of the most often used supercritical solvents due to its good features, including non-toxic, cheap, non-explosive, and mild critical conditions (critical temperature 31.7 • C and critical pressure approximately 73.8 bar) [12]. Moreover, SC-CO 2 has physicochemical qualities that are intermediate between those of a liquid and a gas, with low viscosity, high density, and diffusivity that allow it to be an excellent alternative to traditional extraction technologies [13]. This technique can be used for a broad spectrum of chemical and biochemical extraction processes [14] because of its selectivity property, which can be adjusted by minor changes in pressure and/or temperature. SC-CO 2 produces excellent extracts with yields that are equivalent to those made using organic solvent extraction. Some results have shown the highest antioxidant and antifungal properties of SC-CO 2 extract compared to the conventional method [15,16]. In addition to these, CO 2 has the benefit of being appropriate for extracting thermo-labile chemicals since it does not require extensive solvent heating. However, one of the limitations of this technique is that CO 2 is a non-polar solvent and may not be effective alone to extract polar compounds such as phenolics. As a result, there is an application of methanol, water, or ethanol as co-solvent or modifier to enhance the solvation power of SC-CO 2 , improve its affinity for poorly soluble solutes (alkaloids, phenolics, and glycosidic compounds), increase solubility, as well as the extraction yield with respect to operating pressure and temperature [13].
The basic goals of this research were to extract the dried Lamium album flower by using SC-CO 2 with methanol as co-solvent, to investigate in vitro antioxidant capacity of these extracts using different radical scavenging assays (DPPH and ABTS), reducing power assay (FRAP), total phenols estimation using Folin-Ciocalteu, and phenolic compounds quantitation by using UPLC-PDA (Waters, Manchester, MA, USA). This approach should complement the previously known extraction techniques of the Lamium album and improve the dissemination of this green technology and the possibility of using Lamium album flower extract in agriculture, food, cosmetics, and pharmaceutical industries.

Plant Material
High-quality of dried Lamium album flowers were collected from ecological area (Podlasie) in Poland and certified by herbal company Dary Natury.

Supercritical Carbon Dioxide (SC-CO 2 ) Extraction
The extraction process was carried out on a laboratory scale by using MV-10ASFE (Waters, Manchester, MA, USA) consisted of a CO 2 cylinder and a cooling system, fluid delivery module, column oven, back pressure regulator, heat exchanger and fraction collection module with ChromScope v1.20 software (Waters, Manchester, MA, USA). Then, 2 g of Lamium album flower was kept in the extraction vessel of 25 mL and placed in the oven set at the desired different temperatures (40,50 and 60 • C) and pressure (250 bar). The CO 2 flow rate was 4 mL/min, and methanol was fixed at 1 mL/min. Once the set temperature and pressure (at solvent pumps and back pressure regulator) were achieved after turning on the injection valve and the system was in equilibrium, the extraction was carried out for 180 min in each experimental run, which was composed (based on the trial experiments) of 1st dynamic time 45 min, static time 15 min and 2nd dynamic time of 120 min. Lamium album extracts were collected in flasks placed in a fraction collection module, and it was stored at −20 • C before further analysis of polyphenols and antioxidant activity.

Quantification of Total Phenolic Compounds
Total phenolic content (TPC) of Lamium album extract was estimated spectrophotometrically according to the Folin-Ciocalteu method by following the protocol of Arabshahi-Delouee and Urooj (2007) [17] with minor modifications. Gallic acid (50-500 mg/mL) [18] was used for the standard calibration curve and distilled water as a blank sample. In a test tube, 1.60 mL of distilled water were mixed with 20 µL of samples, blank or standard to be analyzed. 100 µL of Folin-Ciocalteu reagent was then directly added and vortexed. After 3 min, 300 µL of 75 g/L Na 2 CO 3 was added and mixed toughly. The obtained solution was incubated at room temperature for 45 min in absence of light after which absorbance readings were taken at 760 nm using a Varian Cary 300bio UV-VIS spectrophotometer (Agilent, Santa Clara, CA, USA). All measurements were performed at least in triplicate and the total phenolic content estimation was calculated by using this formula according to Mabrouki et al. (2018) [19]: where c is the concentration of gallic acid established from the calibration curve (mg/mL), v is the volume of extract solution (mL) and m is the weight of the sample extract (g). the results were expressed as mg gallic acid equivalent per gram of the extract (mg GAE/g of extract).

Evaluation of Antioxidant Activity
scavenging capacity assay is a decolorization assay that directly measures the scavenging capacity of antioxidants with DPPH radicals by monitoring its absorbance at 517 nm with a spectrophotometer [20].
The free radical scavenging activity of Lamium album extract was measured by DPPH assay according to the method described by Moradi et al. (2016) [21] with minor modifications. The working solution was prepared by making a methanolic solution of DPPH (0.1 mM). A 2850 µL of this solution was mixed with 150 µL of the sample, standard (Trolox) at different concentrations or blank (methanol). The reaction mixture was shaken well and incubated in the dark for 30 min at room temperature. After this time, the absorbance was taken at 517 nm using Varian Cary 300bio UV-VIS spectrophotometer (Agilent, Santa Clara, CA, USA). Low absorbance of the reaction mixture indicated high free radical scavenging activity. The experiment was carried out in triplicate, and the results are average values. The scavenging activity was estimated based on the percentage of DPPH radical scavenged as the following equation: where Ab is the absorbance of the blank and As is the absorbance of the sample. The EC50 value, the amount of antioxidant necessary to halve the initial DPPH concentration, was estimated using linear regression of plots of DPPH radical inhibition percentages versus the concentrations of the tested extracts of Lamium album flowers. The results were used for comparing the quality of the antioxidant extracts. The experiment was repeated three times at each concentration.

ABTS Assay
The assay estimates the capacity of antioxidants to scavenge the stable radical cation ABTS + (2,2 -azinobis (3-ethylbenzothiazoline-6-sulphonic acid). Antioxidant activity was determined with the modified method proposed by Re et al., 1999 [22], where the bluegreen color of ABTS +• was decreased in the presence of antioxidants. The ABTS + radical was prepared by mixing equal amounts of two stock solutions (7 mM ABTS solution and 2.45 mM potassium persulfate solution) and allowing them to react for 16 h at room temperature in the dark. The working solution was then prepared by mixing 3.9 mL of ABTS + with 140 mL of 5 mM phosphate buffered-saline (pH 7.4) to obtain an absorbance of (0.70 ± 0.02) at 734 nm using the spectrophotometer. Fresh ABTS +• working solution was prepared daily. Then, 2850 µL of ABTS + working solution were allowed to react with 150 µL of plant extracts in a test tube for 8 min in water bath incubation at 30 • C. The absorbance was measured at 734 nm using a Varian Cary 300bio UV-VIS spectrophotometer (Agilent, Santa Clara, CA, USA). Trolox was used as standard, PBS as the blank. The results are expressed in µg Trolox equivalents/g of extract mass (µg(TE)/g) on the basis of the calibration curve according to the following formula: where c is the Trolox concentration (µg/mL) of the corresponding standard curve of the plant extract, v is the sample volume (mL), and m is the weight of the plant extract (g) [23].

Ferric Reducing Antioxidant Power (FRAP) Assay
The ferric reducing power of Lamium album extract was determined using a modified version of the FRAP assay [24]. This method is based on the reduction of a colored pale yellow ferric complex (Fe 3+ -tripyridyl triazine) to a blue-colored ferrous complex (Fe 2+tripyridyl triazine) by the action of electron-donating antioxidants at low pH. The working FRAP reagent was prepared daily by mixing 10 mL of 300 mM acetate buffer of 3.6 pH, with 1 mL of 10 mM TPTZ (2,4,6-tri(2-pyridyl)-s-triazine) in 40 mM hydrochloric acid and with 1 mL of 20 mM ferric chloride. The reaction mixture was incubated for 15 min at 37 • C in a water bath before used. Then, 3 mL of freshly prepared FRAP reagent was added to 100 µL of sample solutions or standard (Trolox) and incubated for 5 min at 37 • C in a water bath before analysis. Then, the absorbance of the samples was measured at 593 nm by using Varian Cary 300bio UV-VIS spectrophotometer (Agilent, Santa Clara, CA, USA). All measurements were carried out in triplicate. The results were expressed as the FRAP value calculated into µmol/L Trolox on the calibration curve, which was prepared using a methanolic solution of Trolox at the concentration 150-3000 µmol/L. The following formula was used: where AS is absorbance of the sample and AC is the absorbance of the standard (Trolox) at 593 nm and concentration of Trolox (µmol/L). From the obtained FRAP value, the final antioxidant activity in each sample was expressed as Trolox equivalents (TE) in terms of µmol TE/g extract, and the following equation according to Tomasina et al. (2012) [25] was employed: AA (µmol TE/g extract) = Trolox (µmol/L)/sample (g/L)

Quantitative Analysis of Polyphenols Using UPLC-PDA
The concentrations of bioactive compounds in the methanolic extracts were determined using a UPLC-PDA-TQD system, which consisted of the Acquity UPLC chromatograph (Waters, Manchester, MA, USA) coupled with a photodiode detector (PDA eλ Detector) (Waters, Manchester, MA, USA) and an electrospray ionization (ESI) triple quadrupole mass spectrometer (TQD) (Waters, Manchester, MA, USA). Mobile phase consisted of two solutions: line A-water containing 0.1% HCOOH and line B methanol containing 0.1% HCOOH. The phenolics were separated at 30 • C on the analytical columna Waters ACQUITY UPLC BEH C18 (150 × 2.1 mm/ID, with 1.7 µm particle size) (Waters, Manchester, MA, USA) with flow rate 0.35 mL/min and using gradient elution: from 10 to 60% of B line during 15 min followed by the return to the initial conditions. Temperature of samples in the autosampler was 10 • C. UV spectral data for all peaks were recorded in the range of 190-450 nm. Data processing was done using Empower 3 (Waters, Manchester, MA, USA). All samples of Lamium album extracts were filtered through a 0.20 µm syringe filter (Chromafil, Macherey-Nagel, Duren, Germany) before analyses and were injected to the chromagraphic system in triplicate. Identification of bioactive compounds was done using matching retention times, UV and mass spectra (MRM) data of standards.

Statistical Analysis
The experimental data were statistically evaluated using the Statgraphics 4.1 software package (Graphics Software System, STCC, Inc., Rockville, MD, USA). A one-way ANOVA was used to assess the significance of the differences between the antioxidant activity and polyphenols concentration in the tested extracts. Fisher's Least Significant Difference (LSD) test at α = 0.05 was used for the paired tests.

Total Phenolic Content
The use of an environmentally friendly, modern extraction technique (SFE) allowed obtaining pure fractions collected at different temperatures. Supercritical CO 2 is a nonpolar solvent, but its polarity can be modified by temperature and pressure variations. Polyphenols with high molecular mass are hardly soluble in pure CO 2 , but their solubility can be enhanced by adding a polar co-solvent or increasing pressure [26]. In our research, methanol commonly used for extraction and high pressure (250 bar) were used. Testing the antioxidant activity allowed us to check the differences between fractions obtained at different temperatures. The TPCs of the extracts obtained from dry Lamium album flower by SC-CO 2 with methanol as co-solvent were determined quantitatively using a spectrophotometric method with Folin-Ciocalteu reagent as the most and commonly used method for total phenols estimation. A calibration curve was established with gallic acid as standard at different concentrations. The results were expressed in mg of gallic acid equivalent (GAE)/g of extract. All measurements were taken in triplicate, and mean values were calculated. The results of determination of the polyphenols are presented in Table 1. Values are mean ± s.d., n = 3, values with the same lowercase letters in the same column indicate no significant difference at level of 5% (p < 0.05).
As shown in Table 1, the results varied from 234.17 to 650.17 mg GAE/g of extract for the studied conditions, which represent a variation of approximately three folds. The extract at 50 • C showed the highest TPCs of 650.17 mg GAE/g of extract, followed by 60 • C, which showed 418.50 mg GAE/g of extract, and 40 • C showed the lowest value of 234.17 mg GAE/g of extract. All studied conditions showed a considerable amount of total phenols and they were significantly different as expected due to the effect of temperature on the density and selectivity of the solvent during SC-CO 2 . However, a degradation effect may be suspected between 50 • C and 60 • C at 250 bar during the extraction process, which has caused a decrease in TPCs.
The total phenolic content obtained in this work is not directly comparable to other studies of Lamium album extracts because the extraction methods are different. In the previously published papers, most of them have used solvent extraction methods to extract Lamium album. Matkowski and Piotrowska (2006) [27] reported 192 mg GAE/g of extract of TPC in methanolic extract of Lamium album, Pereira et al. (2012) [5] reported 500.7 ± 50.0 mg/g of extract of phenolic compounds in the ethanolic extract of L. album [5], also other species of Lamium have been reported to have high content of polyphenols [7,27,28] and methanol have been reported as a good solvent [28]. The high TPC value obtained for our extract (especially for the fraction at 50 • C) compared to the research of other authors indicates a very effective extraction using the SFE technique.

Antioxidant Activity Determination
An antioxidant is any chemical that, when present at lower concentrations than those of an oxidizable substrate, considerably slows or inhibits its oxidation. Natural antioxidants and their health advantages have received a lot of attention in recent years. Antioxidant-based medication compositions are used to prevent and cure a wide range of diseases and ailments. Plants are a significant source of natural antioxidants; they produce a diverse spectrum of secondary metabolites with antioxidative activity and therapeutic potential [29]. The antioxidative activity are mostly based on two reaction mechanisms such as hydrogen atom transfer (HAT) and single electron transfer (SET) [30].
Currently, there is no unique method that has been standardized for antioxidant activity determination due to the various reaction features, mechanisms as well as variable phase localizations that are frequently involved in the process [30]; however, while extracting valuable bioactive compounds from various plants, it is very important to select the appropriate method and optimize the extraction conditions, since this has a direct impact on the production of extracts with high activity. In this study, the assessment of antioxidant activity of Lamium album flower extract was conducted by two free radical-scavenging methods, the DPPH free radical scavenging assay and the ABTS radical cation decolorization assay; and by ferric reducing antioxidant power assay (FRAP) in order to have a better estimation on the antioxidant capacity of the Lamium album extract. These assays were conducted using a UV-VIS spectrophotometer.
The antioxidant activity of the sample extracts was examined, and the findings were slightly different. However, all of the assays could be used to determine the antioxidant activity of Lamium album flower extract obtained by SC-CO 2 with methanol as a co-solvent because they all yielded similar rankings among the extracts and demonstrated that extracting the antioxidants at 50 • C and 250 bar was the best condition in this study. The results are summarized in Table 2. Values are mean ± s.d., n = 3, values with the same lowercase letters in the same column indicate no significant difference at level of 5% (p < 0.05).

DPPH Scavenging
This approach has been introduced for the 1st time by Blois (1958) [31], and now is one of the commonly used to assess the free radical scavenging activity of various antioxidant compounds due to its accuracy [32] and it is known to give reliable information concerning the antioxidant ability of the tested compounds. It is based on the reduction of DPPH in alcoholic solutions (methanol or ethanol) in the presence of a hydrogen-donating antioxidant. The dark violet color of the DPPH radical becomes yellowish or colorless due to the antioxidant compound, causing a decrease in the absorbance at 517 nm [33,34]. Table 2 showed that the DPPH EC50 results varied from 0.12 to 0.37 mg/mL, which is the quantity of antioxidant required to reduce the initial DPPH radical concentration by 50% [20]. The lower the value, the higher the antioxidant activity. The overall results showed that the extract obtained at 50 • C had the highest ability to scavenge the DPPH radical. However, the conditions 50 • C and 60 • C were not significantly different at p-value = 0.05.
In similar studies, Paduch et al. (2007) [8] with solvents extraction, has reported free radical scavenging activity of methanol and ethyl acetate extracts of Lamium album, compared to Trolox and their results showed that methanol extract had free radical scav-enging properties and an average EC50 of 0.4659 ± 4.4 mg/mL while ethyl acetate extracts did not exhibit DPPH radical reduction activity [8]. Additionally, Bubueanu et al. (2013) demonstrated DPPH free radical scavenging activity of butanolic extract of Lamium album in EC50 value to be 19.29 mg/mL [7].
Furthermore, the antioxidant tests were performed using the scavenging activity of the synthetic stable 1,1-diphenyl-2-picrylhydrazyl (DPPH) free radical and two oxygen radicals spontaneously produced in the cells-superoxide radicals and hydroxyl radicals, both of which are hazardous to the cell at high levels. In comparison to reference compounds like vitamin E and quercetin, the aqueous component of L. album hydro-alcoholic extract demonstrated modest antioxidant activity. However, among all examined aqueous fractions from 16 medicinal plants, the extract from L. album shown a considerable scavenging impact on DPPH radicals (EC50 = 0.28 mg/mL) [35].

ABTS Assay
This method was developed by Miller and Rice-Evans [36]. It is based on the scavenging ability of antioxidants to the ABTS radical and it can be used to analyze both hydrophilic and hydrophobic antioxidant capacities of extract [30]. Table 2 in this study shows that ABTS radical scavenging activities of Lamium album extracts varied from 43.20 to 44.53 µg TE/g. The extract at 50 • C showed the highest antioxidant capacity (44.53 µg TE/g), followed by 60 • C which showed a very similar value-44.52 µg TE/g and at 40 • C was the lowest-43.20 µg TE/g. Statistical analysis has shown a significant difference of the extract at 40 • C to the other two remainders.

FRAP Assay
This method has been developed by Benzie and strain (1996) [30]. It is based on the reduction of ferric ions (Fe 3+ ) to ferrous ions (Fe 2+ ) by an antioxidant under acidic solution to maintain iron solubility [24,30]. The ferric salt solution is a pale-yellow color, but when reduced to the ferrous form, this changes to blue, and absorbance at 593 nm increases. However, this method is not convenient to the compounds that act as radical quenching or hydrogen transfer, particularly thiols and protein, and it does not react with glucose and fructose [20,24]. Table 2 shows that the ferric reducing potential of Lamium album extracts varied significantly (p = 0.05) from 19.48 to 44.74 µmol TE/g of extract, which represents a variation of twofolds. The extract at 50 • C showed very strong ferric ion reducing activities 44.74 µmol TE/g of extract, followed by 60 • C which showed 28.32 µmol TE/g of extract and 40 • C showed the lowest value of 19.48 µmol TE/g of extract. Furthermore, the reducing power of plant extracts by FRAP assay have been reported in various studies [37][38][39].
In similar studies, Dudenno et al. (2009) [38] investigated antioxidant activities and the total phenolic content of 30 commonly used plants using DPPH, ABTS, FRAP, ORAC, and SOD assays. Their findings show that the ferric ion reducing activities of the 30 plant extracts tested did not differ significantly from their DPPH and ABTS scavenging activities [38]. Additionally, Katalinic et al. (2004) [39] examined the total phenolic content and total antioxidant potential in 70 medicinal plant infusions. Their results revealed significant differences in total antioxidant capacity (FRAP) between the medicinal plant infusions, with FRAP values ranging from 59 to 25,234 µmol FeII/L of infusion. Additionally, the significant linear correlation between total phenolics and FRAP of medicinal plant extracts was confirmed.

Profile of Phenolic Compounds
Phenolic compounds are a class of natural secondary metabolites highly present in a different part of plants that has gained a lot of scientific and medicinal attention because of the wide variety of beneficial properties such as antioxidant and anti-inflammatory qualities that may be beneficial in the prevention and/or treatment of cardiovascular disease, neurological diseases, cancer, and obesity [40].
As can be seen in Table 3, the present study identified 13 out of 22 analyzed phenolic compounds in Lamium album flower extract obtained by SC-CO 2 , which comprised flavones, phenylethanoid isomers and flavanone. The mean phenolic compounds concentration varied from 0.09 (trans-cinnamic acid, at 40 • C) to 22.68 ng/µL (chrysin, at 50 • C). Apart from chrysin, high levels of concentration for extracts obtained at 50 • C have been reported for myricetin, pinostrobin, and trans-3-hydroxycinnamic acid. The concentration of the most analyzed bioactive compounds was statistically higher (p = 0.05) for the extract obtained at the temperature of 50 • C, especially in comparison with the extraction conditions at the lower temperature of 40 • C. On the other hand, for the extraction carried out at the highest temperature 60 • C, the level of most bioactive compounds was significantly lower compared to the extraction at 50 • C, except for ritin, quercitin and trans-cinnamic acid. The obtained results are consistent with the highest antioxidant activity for the extract obtained at 50 • C, confirmed by four methods (Tables 1 and 2). In the literature, very little information is available concerning the phenolic compounds of the studied plant (Lamium album flowers) and their application. However, in the previous studies, some flavonoids in forms of glycosides (rutin, isoquercitrin, tyliroside) and aglycones (quercetin) and phenolic acids (protocatechuic, chlorogenic, vanillic, caffeic, coumaric, and ferulic acids) have been found in methanol and ethyl acetate extracts of L. album by using HPTLC combined with densitometry and HPLC method [8]. For the first time, Pereira et al. (2012) [5] identified derivatives of unusual flavone isoscutellarein in purified ethanol extract of flowers, leaves and stems from L. album, and were found to represent approximately one third of the total phenolics quantified and also phenylethanoid glycosides verbascoside and iso-verbascoside have been reported [5].
To the best of our knowledge, most of those phenolic compounds were identified in Lamium album for the first time in the present study. Chrysin (5,7-dihydroxyflavone) is a major compound detected in Lamium album extract in this study. It is a flavone, naturally present in flowers of various plants, honey and some mushrooms [41], it has a lot of health importance for humans. Chrysin was reported to have enormous biological activities such as antibacterial, antidiabetic, anticancer, anti-inflammatory, and anti-aging [42,43]. Furthermore, a recent clinical trial found that using chrysin can result in body weight loss and a lower postprandial blood-glucose level [41]. In addition to its medicinal use as an ingredient in pharmaceutical preparations, chrysin is widely utilized as a functional additive in teas, meals, and cosmetics.
Myricetin is a common plant-derived flavonoid that has also identified in the present study of Lamium album flower extract at high concentration. Myricetin is widely found in vegetables, fruits, nuts, berries, herbs, medicinal plants and beverages such as tea and wine [44]. This flavonoid has also been shown to have strong antioxidant capabilities as well as free radical scavenging properties. These activities appear to support a wide range of beneficial outcomes, including anti-platelet aggregation, antihypertensive, immunomodulatory, anti-inflammatory, anti-allergic, analgesic, and anticancer effects [44,45]. The rich composition of bioactive compounds of Lamium album extracts along with high antioxidant activity indicates the great potential of this poorly-so far-known plant.

Conclusions
Lamium album flowers extracts were obtained by SC-CO 2 with methanol as co-solvent. The antioxidant properties of the obtained extracts were estimated spectrophotometrically by using DPPH, ABTS, and FRAP assays. The findings of our study revealed that the obtained extracts from L. album flowers possess considerable antioxidant potential. The differences in antioxidant activities and total phenolic content in the extracts can be attributed to different extracting conditions, especially temperature in this study as it can have positive or negative effect on the solubility of bioactive compounds during SC-CO 2 extraction at constant pressure. The most efficient temperature was 50 • C. The phenolic composition of the extracts was assessed by UPLC/PDA and chrysin, pinostrobin, myricetin and trans-3-hydroxycinnamic acid were higher compared to other compounds in this study. Therefore, this work confirms that phenolic compounds and antioxidants can be effectively extracted from Lamium album flowers using green SFE technology. Our results indicate wide possibilities of using Lamium album flower extract in agriculture, food, cosmetics, and pharmaceutical industries as a source of bioactive compounds.

Data Availability Statement:
The data that support the findings of this study are available from the corresponding author, upon request.

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