Phytochemical, Antioxidant, Antihyaluronidase, Antityrosinase, and Antimicrobial Properties of Nicotiana tabacum L. Leaf Extracts

Nicotiana tabacum L. (tobacco) is an important and valuable crop for the cigarette industry. However, cigarette cessation has been encouraged worldwide. Therefore, this study aimed to investigate the potential of N. tabacum leaf extract use in other industries besides cigarette production, especially cosmeceutical industries, which are of interest for increasing the value and widening the applications of N. tabacum. The leaves of N. tabacum var. Virginia and Turkish were extracted by maceration using 95% v/v ethanol or petroleum ether. The extracts were evaluated for their phytochemical compositions, antioxidant capacity, and anti-aging, antimelanogenic, and antimicrobial activities. The phytochemical screening of the extracts revealed terpenoids, steroids, alkaloids, tannins, and carbohydrates in all of the N. tabacum leaf extracts. The total phenolic content was detected to be the highest in the ethanolic extract of Virginia tobacco leaf, which had the most significantly potent antioxidant and antihyaluronidase activity (P < 0.05). On the contrary, the extracts from the Turkish variety demonstrated the most powerful antimicrobial activity against Staphylococcus aureus. Thus, ethanolic extracts of N. tabacum var. Virginia are suggested as good natural anti-aging ingredients with potent antioxidant and antihyaluronidase effects, whereas the leaf of N. tabacum var. Turkish is suggested as a good source of natural antimicrobial components, particularly for S. aureus inhibition. In summary, in addition to the cigarette industry, N. tabacum leaf could be a source of pharmaceutical and cosmeceutical compounds, particularly natural anti-aging and antimicrobial ingredients.


Introduction
Nicotiana tabacum L., or tobacco, is a member of the Solanaceae family. It is one of the most commercially valuable agricultural crops in the world and is usually used in the cigarette industry. In ailand, N. tabacum is grown in the northern and northeastern regions, and is also used as a raw material for the manufacture of cigarettes. Although cigarettes have adverse effects on humans and the environment, N. tabacum contains several useful phytochemical components that could be applied in other industries. N. tabacum has been reported to contain large numbers of secondary metabolites exerting many biological and pharmacological activities [1,2]. For example, previous research found that alkaloids derived from plant extracts had an antiinsect effect, which is important in agriculture, as well as exerting health benefits for Alzheimer's and Parkinson's diseases [3][4][5]. In addition, solanesol and its derivatives have antibacterial, anticancer, anti-inflammatory, and antioxidant properties [6]. Its polyphenols also presented antioxidant capacity, along with playing an important role in the prevention of various diseases, such as hyperlipidemia, arthrosclerosis, cardiovascular disease, and cancer [7,8]. Moreover, the phenolic acids, particularly chlorogenic acid and rutin, contributed to the potential for both antioxidant and antimicrobial activities [9]. Overall, extracts of N. tabacum show the presence of abundant bioactive molecules that can provide many health benefits in humans. Apart from the pharmaceutical industries, the cosmeceutical industries are also an interesting market that could promote the value of natural resources. Since N. tabacum has been reported to display various pharmaceutical effects, it could be applied in the cosmeceutical industries. Regarding the various biological functions of N. tabacum, different parts of the plant have been examined. A variety of phytochemical components have been found in various parts of N. tabacum, resulting in numerous biological activities. Antimicrobial activity has been detected in the leaves, stems, and roots [10][11][12][13][14]. Similarly, antioxidant activities were also found in various parts of N. tabacum, including the leaves, roots, and stems [13,15,16]. According to the mentioned properties, N. tabacum has the potential to be used as an active ingredient in pharmaceutics and cosmetics, leading to the greatly increased value of this plant. However, the leaves are easier to utilize than the roots and stems since the plant does not need to be uprooted or exterminated.
Among several varieties of N. tabacum, the Virginia and Turkish varieties are widely cultivated in the northern regions of ailand. erefore, our research team was interested in evaluating the phytochemical components and their biological and pharmacological activities, including antioxidant, anti-aging, whitening, and antimicrobial effects, of N. tabacum var. Virginia and Turkish leaf extracts. Since there was no previous study on the anti-aging and antimelanogenic properties of N. tabacum extract, the goal of this research was to investigate the potential of tobacco for use in cosmeceuticals for the further development of tobacco-based cosmeceutical products.  [17]. Glycosides were evaluated by the Keller-Kiliani test [18]. Terpenoids were evaluated by the Salkowski test [18]. Steroids were evaluated by the Liebermann-Burchard test [19]. Alkaloids were evaluated using different reagents, including Dragendorff's, Mayer's, Wagner's, and Hager's reagents [20,21]. All the experiments were carried out in triplicate. Tannins were evaluated using different reagents, including 0.5% gelatin, 1% quinine sulfate, 1% lead acetate, and vanillin reagents [21][22][23]. Anthraquinones were evaluated using Borntrager's test [23]. All the experiments were carried out in triplicate.

Total Phenolic Content.
e Folin-Ciocalteu method was used to determine the total phenolic content of N. tabacum extracts [24]. e reaction mixture consisted of 20 μl of extract, 80 μl of freshly prepared Folin-Ciocalteu reagent, and 100 μl of 7.5% sodium carbonate, which were then incubated at room temperature and in the dark for 2 h. e mixture was measured for absorbance at 765 nm, and we calculated the phenolic content using gallic acid as a standard; results were expressed as gallic acid equivalents (GAE).
ree independent experiments, repeated in triplicate, were performed. Evidence-Based Complementary and Alternative Medicine

Determination of Nicotine Content Using High-Performance Liquid Chromatography (HPLC).
e identification of nicotine in N. tabacum extracts was performed via the high-performance liquid chromatography (HPLC) method (Hewlett-Packard, Inc., Palo Alto, CA, USA). A C-18 reverse phase column (Hypersil ODS, 4.6 × 150 mm, Agilent Technologies, Inc., CA, USA) was used to evaluate the nicotine content. e mobile phases consisted of solvent A containing sodium acetate: methanol: triethylamine in a ratio of 88 : 12 : 0.5 (v/v) and solvent B containing methanol with a flow rate of 1 mL/min. e samples (5 μl) were injected and separated in peak areas for 30 min, and then detected with an UV detector at a wavelength of 259 nm. Peak areas of the eluted compounds were recorded and integrated with the HPLC software. Persisting nicotine compounds were identified by comparison with nicotine standard [25]. All experiments were carried out in triplicate.

DPPH Assay.
e radical scavenging activity of N. tabacum extracts against DPPH radicals (DPPH•) was assessed using the method established by Chaiyana et al. [24]. e reaction mixture contained 20 μL extract and 180 μL of 167 μM DPPH solution, incubated in dark conditions at ambient temperature for 30 min, and measured at absorbance of 520 nm (Microplate Reader EZ Read 2000, Biochrom Ltd., Cambridge, UK). ree independent experiments, repeated in triplicate, were performed. e percentage of DPPH inhibition was computed using the following calculation: % DPPH inhibition � [(A − B)/A] × 100, where A is the absorbance of the control, and B is the absorbance of the sample.

ABTS Assay.
e radical scavenging activity of N. tabacum extracts against ABTS cationic radicals (ABTS •+ ) was assessed using the method described by Laosirisathian et al. [26]. ABTS •+ was produced by combining 2 mL of 7 mM ABTS and 3 mL of 2.45 mM potassium persulfate oxidant under 16-24 h incubation, in dark conditions, at ambient temperature. e working solution was prepared by diluting ABTS •+ with ethanol until the OD reached 0.7 ± 0.1 at 750 nm. For the scavenging reaction, 20 μL of sample was mixed with 180 μL of ABTS •+ solution, incubated in dark conditions at ambient temperature for 5 min, and measured at absorbance of 750 nm (Microplate Reader EZ Read 2000, Biochrom Ltd., Cambridge, UK). e results were demonstrated in terms of Trolox equivalent antioxidant capacity (TEAC). ree independent experiments, repeated in triplicate, were performed. e results were recorded in terms of equivalent capacity (EC 1 ) when compared to the ferric sulfate (FeSO 4 ) standard curve. ree independent experiments, repeated in triplicate, were performed.
ree independent experiments, repeated in triplicate, were performed. e percentage of lipid peroxidation inhibition was computed using the following calculation: % Lipid peroxidation inhibition � [(A − B)/A] × 100, where A is the absorbance of the control, and B is the absorbance of the sample.

Antihyaluronidase Activity Determination.
e antihyaluronidase activity of N. tabacum extracts was evaluated following the method of Chaiyana et al. [28]. e reaction mixture consisted of 20 μL of extract and 100 μL of 15 U/mL hyaluronidase solution, which was then incubated at 37°C for 10 min. e incubated mixtures were combined with 0.1 mL of 0.03% w/v hyaluronic acid dissolved in 0.02 M phosphate buffer (pH 5.35), which was then incubated at 37°C for 45 min. After incubation, 1 mL of 0.1% w/v bovine serum albumin was added, and the mixture was incubated at room temperature for 10 min and measured at absorbance of 600 nm (Microplate Reader EZ Read 2000, Biochrom Ltd., Cambridge, UK). ree independent experiments, repeated in triplicate, were performed. e percentage of hyaluronidase inhibition was computed using the following calcu- where A is the absorbance of the control, and B is the absorbance of the sample.

Antityrosinase Activity Determination.
e antityrosinase activity of N. tabacum extracts was assessed following the method established by Prommaban et al. [29]. e reaction mixture contained 10 μL of extract and 30 μL of tyrosinase, incubated at room temperature for 10 min. en, the mixtures were combined with 0.1 mL of substrate and 2.5 mM of L-tyrosine or L-DOPA, incubated at room temperature for 30 min, and measured at absorbance of 450 nm (Microplate Reader EZ Read 2000, Biochrom Ltd., Cambridge, UK). ree independent experiments, repeated in triplicate, were performed. e percentage of tyrosinase inhibition was computed using the following calculation: Evidence-Based Complementary and Alternative Medicine absorbance of the control, and B is the absorbance of the sample.

Antimicrobial Activity Determination.
e antimicrobial activity of N. tabacum extracts was examined against 4 reference bacterial strains obtained from the American Type Culture Collection (ATCC): Staphylococcus aureus (ATCC25923), Staphylococcus epidermidis (ATCC12228), Propionibacterium acnes (ATCC6919), and Pseudomonas aeruginosa (ATCC27853). Antimicrobial assays were performed using the agar disc diffusion, minimum inhibitory concentration (MIC), and minimum bactericidal concentration (MBC) techniques by following previously established methods.

Agar Disc Diffusion Method.
e bacterial inoculum was diluted in phosphate-buffered saline (pH 7.4) to obtain turbidity visually comparable to the McFarland N°0.5 standard (1 × 107 CFU/mL). Each inoculum was spread over tryptic soy agar (TSA) plates. For disc preparation, 10 μl of each extract was dropped onto a 5 mm diameter paper disc and then plated on a TSA plate containing bacteria, and incubated at 37°C for 24 h. Reference antibiotics used in this study were 25 μg of Ampicillin ® and Penicillin ® . e inhibitory zones around the discs were observed, measured, and expressed in mm [30]. All the experiments were carried out in triplicate.

Minimum Inhibitory Concentration (MIC) Method.
MIC was characterized by the lowest concentration that inhibited the visible bacterial growth. Briefly, Mueller-Hinton Broth (MHB) was plated in a 96-well plate, and then, the extracts were twofold diluted in MHB at a ratio of 1 : 2 to 1 : 64. e bacteria were added to test wells with a final concentration of 1 × 10 5 CFU/mL and incubated in 37°C for 24 h. e growth of bacteria was observed; a clear solution indicated no growth, and a turbid cloudy solution indicated bacterial growth [31]. All experiments were carried out in triplicate.

Minimum Bactericidal Concentration (MBC) Method.
e concentration presenting no growth visible in MIC was used to test the MBC. e same concentration of MHB, along with the extracts, was spread over Mueller-Hinton agar (MHA) plates and then incubated at 37°C for 24 h. e growth of bacteria was observed and reported as the bactericidal concentration [31]. All experiments were carried out in triplicate.

Statistical Analysis.
All experimental data were expressed as mean ± SD. Statistical data were analyzed using Tukey's post hoc test and one-way analysis of variance (ANOVA) in GraphPad Prism (version 8.0; GraphPad Software). Statistically significant differences were demonstrated when P < 0.05.

Results and Discussion
3.1. Yield of N. tabacum Extracts. Different varieties and solvent extractions of N. tabacum leaves are presented as percent yields according to Table 1. e ethanolic extracts from both N. tabacum varieties (VL-E and TL-E) exhibited higher percent yields than those obtained with petroleum ether extraction (VL-P and TL-P). is could indicate that N. tabacum extracts contain both nonpolar and polar compounds, but they were composed of huge amounts of polar compounds, which can be extracted with a polar solvent such as ethanol. However, there were no differences in the amount of yield between the two varieties in ethanolic extraction, but N. tabacum var. Turkish had a slightly higher yield than Virginia during part of the petroleum ether extraction process.

Chemical Constituents of N. tabacum Extracts.
Preliminary phytochemical screening of N. tabacum extracts was performed to detect carbohydrates, glycosides, terpenoids, steroids, alkaloids, tannins, and anthraquinones, with the results provided in Table 2. Some phytochemical compounds-terpenoids, steroids, alkaloids, and tannins-were found in all extracts, but only carbohydrates were found in the ethanolic extracts of both varieties. Interestingly, steroids were more abundant in Turkish than in Virginia varieties. However, glycosides and anthraquinones were not detected in the extracts. As is known, the phytochemical composition of a plant demonstrates its various pharmacological and health benefits. Terpenoids are secondary metabolites found in many plants and widely used for flavoring and fragrance in the food and pharmaceutical industries [8]. Alkaloids display various biological properties, such as anti-inflammatory, antioxidant, antibacterial, and anticancer activities [8,32]. Steroids show anti-inflammatory, anticancer, antioxidant, and anti-atherogenicity activities [33]. Tannins, a component of natural polyphenols, are widely used in medical applications, including as anti-inflammatory and diuretic agents against stomach and duodenal tumors [34]. is investigation presented some phytochemical compounds similar to the reports of Peter et al. and Kaushik et al. [21,35], who also determined the compounds in extracts of N. tabacum leaves. In addition to the carbohydrates, alkaloids, phenolic compounds, tannins, flavonoids, steroids, and terpenoids reported in the current study, Peter et al. revealed the presence of resins and essential oil in the N. tabacum leaves [21], whereas Kaushik et al. revealed the presence of saponins and terpenes [35]. Moreover, different parts of N. tabacum, such as the root and stem,  [36]. In brief, variations in phytochemical composition could depend on the plant parts, varieties, solvents, and methods of extraction. Phenolic compounds from plants display a variety of biological functions, especially as antioxidant agents with high reactive oxygen species (ROS) radical scavenging capacity. In this study, the total phenolic content of N. tabacum extracts was calculated using a gallic acid calibration curve and represented as gallic acid equivalents (GAE) per gram dry extract weight. According to Table 3, ethanolic extracts of both N. tabacum varieties had higher total phenolic content than petroleum ether extracts. VL-E showed significantly higher amounts than TL-E, TL-P, and VL-P.
ese results could imply that the polarity of the solvent used in extraction influences the concentrations of phenolic compounds in plant extracts. Because phenols are highly soluble in polar solvents, they can provide higher concentrations of phenols than nonpolar solvents [37]. e amounts of phenolics found in ethanolic extracts in this study were significantly higher than previously reported by Zou et al., who reported that the methanolic extract of N. tabatum had the highest amount in terms of total phenolic content, at 24.82 ± 0.07 mg GAE/g extract [38]. However, different solvents and extraction methods were considered. Moreover, Soumeya et al. found that the leaf extract has higher amounts of phenols than the other parts of N. tabacum [39], which could indicate that N. tabacum leaf extracts might contain a large number of phenolic compounds that exert antioxidant and other biological properties.
Nicotine is a major and common alkaloid that is generated by ornithine metabolism [40]. It is frequently found in N. tabacum or tobacco and is accumulated in tobacco leaves. Despite the fact that nicotine in tobacco causes disease and death in a large number of people, a mild, safe degree of purified nicotine exhibits potential medical uses-for instance, in the reduction of body weight, reduction of stress, and protection against some diseases [41]. e HPLC fingerprint of the nicotine compound presented a retention time of approximately 4.5 min (Figure 1(a)). Nicotine compound was found in VL-E and VL-P extracts and expressed as 5.27 ± 0.13% and 1.01 ± 0.16%, respectively (Figures 1(b) and 1(c)). Nonetheless, no peak area for the nicotine compound was found in TL-E and TL-P extracts. It is possible that nicotine content varies according to the N. tabacum variety. e results were well in line with the previous work from Ghaleb et al., who found that the dry weight of N. tabacum var. Virginia leaf extract expressed nicotine in an amount of 6.7% and an even lower amount was detected in other species such as Burlip, Kstrina, and Zegrin [42]. ese results indicated that N. tabacum var. Virginia contained higher nicotine content than other varieties, supporting our investigation. Another report also found that the concentrations of nicotine in samples in Bangladesh were in the relative range of 0.9 to 3.6% dry weight [43], representing a slightly lower amount than in our study. Moreover, the research by Mirjana and Kelly reported  Evidence-Based Complementary and Alternative Medicine that several cultivated varieties of N. tabacum presented alkaloid content in the range of 0.17 to 4.93%. It was implied that the variation in the alkaloid content depended on the type, the process of tobacco production, and product development, resulting in a variety of nicotine concentrations [44].

Antioxidant Activities of N. tabacum Extracts.
Regarding chemical composition properties, several methods were used for determining the antioxidant activity of N. tabacum extracts. e antioxidant activities of the extracts are shown in Figure 2. At the same concentration of the extracts, ethanolic extracts, especially VL-E, exerted potent antioxidant power, with significantly decreased radicals for both DPPH and ABTS, as well as significantly potent ferric reducing power (P < 0.05). It could be suggested that the phenolic compounds of N. tabacum extracts were responsible for its potent antioxidant effects, since VL-E contained the significantly highest total phenolic content. On the contrary, petroleum ether extracts, TL-P and VL-P, inhibited lipid peroxidase more significantly than ethanolic extracts. is could be due to nonpolar extracts facilitating a large decrease in lipid peroxidase activity. However, the inhibitory activity against lipid peroxidase was only observed at a low level (below 20% inhibition).
Previous research focused on N. tabacum leaf extract, which was relevant to the present study. Wang et al. reported that ethanolic-extracted polyphenols from tobacco leaf possessed strong antioxidant activity when measured for the radical scavenging and lipid peroxidation inhibition activity [14]. Similarly, a previous investigation revealed that N. tabacum extracts exhibited strong antioxidant activities, including radical scavenging activity against DPPH and ABTS, as well as ferric reducing power, due to their polyphenols [38]. With regard to different methods to evaluate the antioxidant activity of tobacco, it was found that tobacco presented antioxidant capacity in the range of 66 to 230 μmol Trolox equivalent/g dry weight using the ORAC method [45]. Furthermore, there was some evidence of antioxidant activity observed in various parts of N. tabacum, such as roots, stems, and flowers. According to a previous study by Al Lahham et al., n-hexane-extracted N. tabacum root extract showed the most potent antioxidant power, which was measured by the DPPH assay [9]. In addition, N. tabacum stem extract was found to contain important antioxidant enzymes such as superoxide dismutase and glutathione transferase, which also enhance the antioxidant activity [13]. erefore, our study and the published literature indicate that polyphenols from tobacco plants exert antioxidant power.

Antihyaluronidase Activity of N. tabacum Extracts.
Hyaluronic acid, or hyaluronan, is an important component of skin that is found in the epidermis and dermis. e function of hyaluronic acid is the maintenance of skin hydration and tissue homeostasis. Hyaluronic acid can be degraded by the hyaluronidase enzyme, resulting in small fragments, associated with loss of skin moisture and the subsequent induction of skin aging [46]. Recently, an alternative bioactive compound from plants was demonstrated as a potential ingredient in anti-aging agents. Several studies have investigated the anti-aging activities involving anti hyaluronidase activity in plant extracts [47,48]. In a recent study, the inhibition of hyaluronidase activity achieved by N. tabacum extracts was assessed, as shown in Figure 3. Hyaluronidase activity was significantly inhibited by TL-E (29.5 ± 0.4% inhibition), similar to the effect of oleanolic acid (OA) (34.1 ± 1.3% inhibition), which is a reference standard for anti-aging activity. Moreover, VL-E and TL-P also strongly inhibited hyaluronidase activity, with 24.5 ± 6.4 and 20.9 ± 5.3% inhibition, respectively. e antihyaluronidase activity of N. tabacum extracts has not been reported to date. However, some previous studies reported that plant extracts containing polyphenols had a strong capacity for hyaluronidase inhibition [49,50]. erefore, plant extracts rich in phenolic compounds, including N. tabacum extracts, could enhance antihyaluronidase activity.

Antityrosinase Activity of N. tabacum Extracts.
Melanogenesis is a biosynthetic pathway for the formation of the pigment melanin in human skin. Tyrosinase is a key enzyme in this process, as it converts L-tyrosine to L-DOPA, which is then oxidized to DOPA-quinone, and eventually synthesizes the melanin pigment [51]. In this regard, tyrosinase inhibitors are considered for skin whitening agents, which are important for the cosmetic industry. erefore, various plant extracts have been tested as pharmaceuticals and cosmetics to prevent excessive melanin production in human skin. Despite the lack of previous research on N. tabacum's antityrosinase activities, the presence of polyphenols, terpenoids, steroids, alkaloids, and tannins in the leaf extract suggests that N. tabacum has antityrosinase activities. A previous study revealed that several families of compounds contain molecules with antityrosinase properties, including phenols, polyphenols, steroids, and triterpenoids [52]. In this study, the inhibition of tyrosinase activity of N. tabacum extracts was assessed, as demonstrated in Figure 4. Kojic acid (KA) was used as a reference standard and exerted the highest tyrosinase inhibition (96.7 ± 0.5% inhibition). Meanwhile, VL-E and TL-E slightly reduced the tyrosinase activity. Several natural plant products have previously been described to attenuate the enzymatic activity involved in the melanogenesis process [53,54]. Researchers suggested that plant extracts rich in bioactive compounds such as polyphenols and flavonoids, along with potent antioxidant properties, were correlated with the inhibition of tyrosinase enzyme activity [53]. is could suggest that the ethanol extracts of both varieties of N. tabacum, containing abundant phenolic compounds, support their capacity for tyrosinase inhibition.  disc diffusion method, all extracts inhibited the growth of S. aureus, S. epidermidis, P. acnes, and P. aeruginosa with different inhibition zones. TL-E and TL-P were most effective against S. aureus, while VL-E and VL-P were most effective for P. acnes. On the contrary, VL-P and TL-E reduced S. epidermidis and P. aeruginosa growth ( Table 4). e standard antibiotics, Penicillin and Ampicillin, exhibited the largest inhibition zones, respectively. ese results indicate that all extracts inhibited various bacteria involved in human skin. e susceptibility of bacteria depended on the N. tabacum varieties and solvent extraction method. Tables 5 and 6 show the MIC and MBC values of N. tabacum extracts against the tested bacterial strains. TL-P and TL-E exhibited the most susceptibility to S. aureus, which was presented in ≥15.62 and ≥31.25 μg/ mL of extracts, respectively, in both MIC and MBC tests. In addition, the antibiotics, Ampicillin and Penicillin, revealed the lowest concentrations required to inhibit bacterial growth in all strains. Nevertheless, the other bacterial strains were susceptible to higher concentrations of all the extracts in the range of ≥125 to ≥500 μg/mL. It could be concluded that the Turkish leaf extracts, TL-E and TL-P, were found to be effective antimicrobial agents against S. aureus.
Nowadays, researchers use extracts of plants for their pharmacological activities and antimicrobial activities. Several phytochemical compounds in tobacco plants, including polyphenols, terpenes, and polysaccharides, also exert antimicrobial activities [2]. Tandon and coworkers reported that the methanolic extract of N. tabacum leaf exhibited remarkable antimicrobial activity against S. aureus and E. coli [55]. Moreover, Akinpelu and Obuotor discovered that N. tabacum leaf extracts inhibited both Grampositive and Gram-negative bacterial growth, such as B. subtilis, P. aeruginosa, and S. aureus [56]. In addition, previous studies indicated that the Nicotiana plant could be used as an effective antimicrobial agent [11,14]. e investigation of the polyphenols extracted from tobacco leaf revealed high antioxidant and antimicrobial activity against S. aureus (17.66 ± 0.86 mm inhibition zone) [14] that was consistent with our findings. As previously reported, four types of bacteria caused skin infection and opportunistic infection in human skin. According to these results, N. tabacum var. Turkish (TL-E and TL-P) displayed a high percentage of inhibition and low concentrations of extracts in MIC and MBC tests, and it could be used to treat bacteria, especially S. aureus.

Conclusions
N. tabacum leaf extracts are enriched with various important phytochemical components, including alkaloids, terpenoids, steroids, and polyphenols. Ethanolic extracts of N. tabacum presented higher amounts of total phenolic compounds than petroleum ether extracts. e major alkaloid in tobacco, nicotine, was found in only the Virginia variety, and could not be observed in the Turkish one. e different types and amounts of phytochemical components depended on the varieties and solvent extraction methods. According to their polyphenols, both varieties also exhibited potent antioxidant and antihyaluronidase activities. Interestingly, the ethanolic extracts displayed excellent effects, especially VL-E. On the contrary, the extracts from the Turkish variety (both TL-E and TL-P) demonstrated the most powerful antimicrobial activity against S. aureus. erefore, it could be suggested that the ethanolic extracts of N. tabacum var. Virginia are good natural anti-aging ingredients with potent antioxidant and antihyaluronidase effects, whereas the leaf of N. tabacum var. Turkish is suggested as a good source of natural antimicrobial compounds, especially for S. aureus inhibition. In brief, besides the cigarette industry, N. tabacum leaf would be a potential source of pharmaceutical and cosmeceutical ingredients. However, the principal component analysis was proposed for additional research. Besides, the safety of N. tabacum extracts should be assessed in a further study, in terms of both the cytotoxicity and the irritation potential.

Abbreviations
Data Availability e datasets used and/or analyzed during the current study can be obtained from the corresponding author upon reasonable request.

Conflicts of Interest
e authors declare no conflicts of interest in association with this study.

Authors' Contributions
W. C. conceptualized the study; A. P., K. K., C. C., S. S., and W. C. developed the methodology; A. P., K. K., C. C., S. S., and W. C. carried out formal analysis; A. P. investigated the study; K. H. collected the resources; A. P. and W. C. wrote and prepared the original draft; A. P., K. K., C. C., S. S., and W. C. wrote, reviewed, and edited; W. C. supervised the study; W. C. administrated the project; W. C. carried out funding acquisition. All authors have read and agreed to the published version of the manuscript.