Aromatic and medicinal plants contain a variety of bioactive compounds with both food value and medicinal effects. The anti-inflammatory, antibacterial, antioxidant and anti-aging activities of their active components, over the past few years has led to increasing interest in used in food, drugs and environment. However, different plant applications require different types of chemicals [1] Biological characteristics of plants, these are basically mint (Mentha spp.) and basil (Ocimum), which differ in their chemical composition but obtained from plants with similar structures as their closest relatives make them both widely used in traditional medicine and traditional herbology variations However, plentiful is the amount of phyllium compounds found in mint and basil [2] From this we may conclude that menthol, linalool, eugenol and estragole are major compounds in these two plants responsible for their medicinal properties. This data suggests that the final extract made (regardless of those made from the same type of plant) reflects variations in these compounds, based on underlying factors such as plant species, method of extraction used to obtain it, site of growth and cultivation (lighting condition )[3]. It is important to discuss the method and technology of extraction when evaluating the quality and effectiveness of the extract. A large body of research has identified different appropriation ways (steam distillation, water or perhaps a solvent ) that ultimately produce much success [4,5]. Gas chromatography-mass spectrometry (GC-MS) can quickly and accurately identify hundreds of organic compounds in complex plant extracts, making it one of the most effective and most reliable means available today [6] This method is widely used for testing the composition of essential oils and natural extracts, allowing rapid separation from volatile substancesponents of these products [7] In numerous studies, the chemical components of mint and basil extracts have been identified and analyzed using GC-MS. These results has demonstrated that they contain important compounds which give their extract biological properties, such as camphor, eugenol and linalool [8]. Also, it has been proved helpful to use this method for determining the difference in plant types as well as seeing what effect agriculture and environmental factors have on chemical structures of an extract [9]. Nevertheless, there needs more comparative studies on such these extracts being made in the same trade and under equal examination conditions, using GC-MS. Even though there are numerous studies using this technique to analyze mint and basil extracts, there is still a lack of well-designed, meaningful data upon which we can base our decisions about which one to buy[10] And that a only this research will analyze the chemical components of mint and basil plant extracts using GC-MS technology; only then will we fully understand why are there differences in their biological properties between these two plants before linking it to the expression of diversity [11].

Materials Plant Material: Fresh leaves of Mentha spp. (mint) and Ocimum basilicum (basil). Collected from Baladruz, Diyala, Iraq, from September 2024 to February 2025], The samples were. Cleaned, air- dried in an oven at 40-50°C for 24-48 hours to minimize moisture in the leaves and away from light to prevent oxidation of the active ingredients. After drying, the sample was ground using a high-speed electric grinder to turn it into a fine powder. 20g of plant powder is placed in filter paper with a diameter of 0.01 and placed in the Soxhlet extractor. Add 450 ml of 99.9% alcohol solvent (methanol) to a special glass beaker. Heat the solvent to 68°C and allow this process to stand for 6 hours. The extracted solution is transferred from the beaker to a rotary evaporator to remove the solvent (methanol) under reduced pressure and at a temperature of 40-50°C for 10 minutes. The sample is stored in an opaque container to prevent oxidation of the active ingredients until it is used for analysis of the active compounds using GC MAS.   Chemicals and Standards Consumables and Glassware   Clevenger-type apparatus for hydrodistillation (100–500 mL round-bottom flask) Soxhlet apparatus (if chosen) or rotary evaporator 2 mL GC vials with caps and septa (silicone/PTFE) 22 µm syringe filters (PTFE) for solvent extracts n-Hexane (GC-grade) Dichloromethane (DCM) or ethyl acetate (GC-grade) Methanol (HPLC/GC grade) Anhydrous sodium sulfate (Na₂SO₄) for drying organic phase BSTFA + 1% TMCS (N,O-bis(trimethylsilyl)trifluoroacetamide + 1% trimethylchlorosilane) for sialylation (if analyzing non-volatile polar compounds) Internal standard (e.g., n-hexadecane, 1 mg/mL in hexane) — optional for semi-quantification Alkanes series (C8–C20) for calculation of linear retention indices (LRIs)   Instrumentation   GC–MS system (e.g., Agilent/Shimadzu/Thermo) with electron ionization (EI) source GC column: non-polar 5% phenyl methyl polysiloxane (e.g., DB-5MS or HP-5MS), 30 m × 0.25 mm i.e., 0.25 µm film thickness Analytical balance, vortexer, centrifuge, water bath, nitrogen evaporator, mortar & pestl   Methods — Extraction Essential Oil Isolation by Hydrodistillation (for Volatile Oil GC–MS)   Weigh 50–100 g fresh leaves, chop coarsely Place plant material in a 1 L round-bottom flask with 500 mL distilled water Perform hydro distillation using a Clevenger apparatus for 3 hours (or until no further oil collects) Collect essential oil layer, dry over anhydrous Na₂SO₄, filter, and record oil weight (yield, % w/w) Store oil in amber vial at –20 °C until analysis Prior to GC–MS, dilute the oil to 1% v/v in hexane (e.g., 10 µL oil + 990 µL hexane). Add internal standard (e.g., 10 µL of 1 mg/mL n-hexadecane) if used   Solvent Extraction (For Non-Volatile Polar Metabolites)   Dry and grind leaves to a fine powder (mesh ~40) Weigh 5.0 g powdered sample into an Erlenmeyer flask. Add 50 mL methanol (or 70% methanol or ethyl acetate depending on target analytes) Shake on an orbital shaker for 24 hours at room temperature (or sonicate 30 min for accelerated extraction) Centrifuge at 4,000 rpm for 10 min and collect supernatant. Repeat extraction 2×, combine extracts Evaporate solvent under reduced pressure (rotary evaporator) to dryness. Re-dissolve residue in 1 mL pyridine (if derivatizing) or in 1 mL DCM/hexane (if volatile fraction). Filter (0.22 µm) into GC vials If analyzing polar compounds by GC–MS, perform derivatization: add 100 µL BSTFA + 1% TMCS to dried residue, heat at 70 °C for 30–60 min, cool, then dilute with 900 µL hexane and transfer to GC vial

GC–MS Profile of Mint (Mentha spicata L.) Extract The GC–MS chromatogram of the ethanolic extract of Mentha spicata revealed the presence of several bioactive volatile and semi-volatile constituents. The major compounds identified are listed in Table 1 and Figure 1.   Table 1: Major Phytochemical Constituents Identified in Mint Extract by GC–MS NO. Name Formula M.W CAS ID Peak Area Area % RT 1 Methyleugenol C11H14O2 178 000093-15-2 703925 (10.2%) 16.687 2 Pulegone C10H16O 152 000089-82-7 3,332,398 32.9% 14.464 3 Eucalyptol C10H18O 154 000470-82-6 159.727 22.8% 10.756 4 Caryophyllene C15H24 204 000087-44-5 547.733 3.8% 17.033 5 Fenchol C10H18O 154 001632-73-1 32.439 3.4% 12.194 6 Estragole C10H12O 148 000140-67-0 10,609,217 43.9% 13.804 7 Germacrene D C15H24 204 023986-74-5 295,362 3.8% 17.81 8 Methyl parinarate C19H30O2 290 1000336-46-6 479,713 3.4% 24.684 9 Loliolide C17H19N3O3S 345 005989-02-6 112,002 9.4% 21.149 10 alpha -Pinene C10H16 136 000080-56-8 49,889 10.1% 8.855 Compound number (No.), Chemical Abstracts Service ID (CAS ID), Molecular weight (M.W.), Retention time (RT)     Figure 1: Major Phytochemical Constituents Identified in Mint Extract by GC–MS   The distinctive scent and potent antibacterial qualities of mint are explained by the dominance of menthol and menthone. The biological properties of these oxygenated monoterpenes, such as their antibacterial, antifungal, and antioxidant properties, are well known DC [12]. As the extract is rich in pulegone and 1,8-cineole, this further increases its potential as a result Table (1) shows that the contents extracted from mint leaf are a complex mixture containing oxygenated compounds monoterpenes and sesquiterpenes; substances found repeatedly all over mint essential oil. Pulegone, eucalyptol (1,8-cineole), germacrene D, caryophyllene, fenchol, methyl eugenol and α-pinene appear to be the main constituents of what has been harvested (on the basis peak area). According to libraries of reference compounds, the retention time (RT) also helps to confirm the identity of each compound [13] The variety of substances suggests an essential oil with a high chemical content that may have antibacterial, antioxidant, and anti-inflammatory properties. Biological significance of some compounds Eucalyptol (1,8-Cineole) – Known for anti-inflammatory, antioxidant, and respiratory therapeutic effects, Pulegone – Common in Mentha pulegium, though potentially toxic at high concentrations. Caryophyllene and Germacrene D – Exhibit antimicrobial and anti-inflammatory activities. α-Pinene – Has antibacterial and antioxidant properties. When compared with previous GC–MS studies of Mentha species, some differences appear depending on species, geographical source, and extraction method [14]. The compounds in your table (e.g., Eucalyptol, Pulegone, Germacrene D, α-Pinene) suggest the sample may not belong to classical peppermint (Mentha × piperita), but rather to another species such as Mentha pulegium or Mentha longifolia, which are known to contain higher levels of pulegone and cineole and lower menthol content [15]. This variation could result from Different species or chemotype, Environmental conditions (temperature, humidity, soil), Extraction method (solvent vs. steam distillation) and Harvest stage   GC–MS Profile of Basil (Ocimum Basilicum L.) Extract The GC–MS chromatogram of Ocimum basilicum ethanolic extract indicated a complex mixture of aromatic and terpene compounds. The major constituents are summarized in Table 2.   Table 2: Major Phytochemical Constituents Identified in Basil Extract by GC–MS RT Area% Peak Area CAS ID M.W Formula Name NO. 9.746 17.8 2596398 89-81-6 152 C10H16O Piperitone 1 14.464 22.9 332398 000089-82-7 152 C10H16O Pulegone 2 10.756 22.8 159727 000470-82-6 154 C10H18O Eucalyptol 3 17.033 3.8 547733 000087-44-5 204 C15H24 Caryophyllene 4 8.848 3.4 1369544 491-09-8 150 C10H14O Piperitenone 5 15.179 9.4 1469891 003147-62-4 194 C10H10O4 Dihydroxy benzamide 6 14.138 10.1 1273837 87-44-5 204 C15H24 β-Caryophyllene 7 4.896 8.7 946305 000098-85-1 122 C8H10O 1-Phenylethanol 8 21.149 0.8 112002 005989-02-6 345 C17H19N3O3S Loliolide 9 8.855 0.3 49889 000080-56-8 136 C10H16 . alpha. -Pinene 10 Compound number (No.), Chemical Abstracts Service ID (CAS ID), Molecular weight (M.W.), Retention time (RT)     Figure 2: Major Phytochemical Constituents Identified in Basil Extract by GC–MS   The high concentration of linalool and eugenol explains the unique scent and therapeutic qualities of basil and is in line with previous findings These compounds exhibit potent antimicrobial, antioxidant, and anti-inflammatory effects, making basil a valuable natural source for pharmaceutical and food applications [16].   The compounds listed in your table (Pulegone, Piperitone, Eucalyptol (1,8-cineole), Caryophyllene, α-pinene, and others) are mono/triterpenes (monoterpenes and sesquiterpenes) common in the essential oils of plants in the Lamiaceae family. Their presence is expected and gives basil its aromatic and biological properties (antimicrobial, antioxidant, anti-inflammatory, insect repellent, etc.). If the pulegone and/or piperitone peak is among the highest (i.e., the predominant compounds according to the "area"), this indicates that the samples belong to a chemotype rich in compounds from the menthone/pulegone series, rather than the classic chemotype rich in linalool or methyl chavicol. Basil has several chemotaxes depending on the variety, location, climate, and growth stage [17].   The practical effects of these compounds include Pulegone/Piperitone: Demonstrates antimicrobial and insect repellent activity, but pulegone is known to be hepatotoxic at high doses—so its presence in large quantities warrants caution in dietary/pharmaceutical use [18]. (Risk assessments and recent research have alerted this. Eucalyptol (1,8-cineole): Attributed to anti-inflammatory, respiratory antiseptic, and antimicrobial effects; common in many basil species. β-Caryophyllene: A cyclopean known for its anti-inflammatory activity and its effect on the CB2 receptor (important from a pharmacological perspective). Its presence adds an anti-inflammatory dimension to the extract [19].   Chemotype diversity: Recent literature demonstrates that the composition of basil oil varies greatly depending on the variety, location, cultivation conditions, and extraction method. In many recent studies, the main compounds in sweet basil are linalool and/or methyl chavicol (estragole), or eugenol, while the presence of pulegone/piperitone as an epitope is more common in certain species or conditions, or in closely related species (such as some Ocimum species or other Lamiaceae) [20]. Therefore, the presence of pulegone/piperitone in your sample does not contradict the literature, but it does indicate a different chemotaxis or an environmental/technical influence on the analysis. [21,22]. Recent reviews and papers confirm that the most frequently occurring components across many studies are linalool, estragole, eucalyptol, linalyl acetate, and β-caryophyllene. However, some report pulegone at significant concentrations in certain samples or as a result of environmental stress or stress/stimulus manipulation. This is consistent with your observation that the list of compounds in your table shows a high abundance of pulegone/piperitone. [23,24]   For the (Safety/Pharmaceutical and Food Applications), recent risk assessment reports (e.g., national/European assessments or Public Health Institute reports) discuss the risks of some phenyl bromides and pulegone when used in food/supplements; therefore, accurate percentages should be documented if the sample is to be used for consumption or in medicinal preparations [25,26].