2.1 General

If not indicated otherwise, all chemicals, solvents, media and standards were purchased from Sigma/Aldrich at high purity (>99%).

Optical rotation was measured on a JASCO DIP-1000 polarimeter. IR spectra were measured using a Shimadzu FTIR-8400S. ¹H and ¹³C NMR spectra were recorded on a Varian Unity 600 system at 600 and 150 MHz, respectively. 1D and 2D NMR data were also obtained using the same system, and spectra were measured and reported in ppm. Tetramethylsilane (TMS) at 0.0 ppm or the solvent CDCl₃ was used as reference internal standard. HRMS analyses were obtained on a Jeol JMS-AX 500 system. GC and GC–MS analyses were carried out by Hewlett Packard 6890 and Hewlett–Packard GCD systems using a Innowax FSC column (60 m × 0.25 mm ∅, with 0.25 μm film thickness), respectively (see for analytical details as in Demirci et al. [9]).

2.2 Plant material

The aerial parts of the plants were collected from different regions and identified by one of us. Voucher specimens were deposited at the Herbarium of Erciyes University, Faculty of Science and Letters. Detailed information on the plant materials used is given in Table 1.

2.3 Isolation of the essential oils

The plant materials were dried in the shade at room temperature and were subjected to hydrodistillation for 3 h using a Clevenger-type apparatus [10] to produce essential oils. The percentage yields were calculated on a dry weight basis as given in Table 2. The oils were obtained neat, dried over anhydrous sodium sulfate to remove the water and stored at +4 °C until analyzed and tested further.

2.4 Isolation of (−)-8(14),15-isopimaradiene-11α-ol (1)

Compound 1 was isolated initially from P. monocephala (PM) essential oil (65.8 mg) by column chromatography. Silica Gel 60 G (ca. 3 g, Merck 7734) was used as a packing material, and filled with wet n-hexane (column size: 10 × 500 mm). n-Hexane:diethyl ether (100 → 0) was used as an eluant in a gradient system. The essential oil was applied and eluted with n-hexane:diethyl ether (90:10) to yield 1 (3.2 mg) as a colorless oily material. [α]_D −17.0° (CHCl₃; c 0.38), EI-MS m/z (rel. int.): 288 [M]⁺ (5), 273(4), 270(3), 255(8), 137(100), 123(28), 95(31), 81(35), 69(28). HRMS: 288.2458 [M]⁺ calcd for C₂₀H₃₂O, 220.2453. FT-IR (liquid film: CHCl₃) ν_max cm⁻¹: 3546 (–OH), 1635, 1602, 1458, 1436, 1367, 1020, 1004 (¹H, ¹³C and 2D NMR data are given in Table 3).

2.5 Preparation of 4-methoxycarbonyl-7-methyl cyclopenta[c]pyrane (2)

Ipolamiide (5 mg) was treated with 0.1 N HCl at pH 5 and stirred vigorously at approx. 100 °C. After 1 h all ipolamiides were converted into its aglycone. The solution extracted with Et₂O and evaporated under nitrogen gave a red-orange residue (2 mg). The sample was analyzed by GC–MS. EI-MS m/z (rel. int.): 190[M]⁺ (100), 189(69), 175(61), 131(15), 129(23), 103(10), 102(15), 77(21), 51(13). MS data were in agreement with those reported by Bianco et al. [11].

2.6 Bioassays

3.1 Determination of essential oil components

Except for P. lunariifolia all other investigated species are endemic plants of Turkey [1]. The essential oils were obtained by hydrodistillation from the aerial parts of P. lunariifolia Sm., P. amanica Vierh., P. monocephala P.H. Davis, P. sieheana Rech. fil, P. armeniaca Willd., respectively. The oils were subsequently analyzed using both GC and GC–MS systems with which the individual components were identified according to their relative retention indices (RR_I) and their relative percentages (see Table 2).

A sum of 68 individual compounds were identified in the oil of P. lunariifolia (PL), representing 74.2% of the total essential oil. This oil was characterized by a high content of hexadecanoic acid (9.7%), β-caryophyllene (9.0%), germacrene-D (7.7%), and (Z)-β-farnesene (6.5%). Overall, the oil was found to be rich in sesquiterpene hydrocarbons.

In the oil of P. amanica (PAm), 60 components were identified representing 83.7% of the total oil. This oil was characterized by germacrene-D (14.7%), bicyclogermacrene (10.7%), (Z)-β-farnesene (8.3%) and spathulenol (6.3%).

Analysis of P. monocephala (PM) oil revealed 78 components, representing 72.8% of the total oil. An unknown compound was detected as the major compound (22.8% and 12.7%) in both the essential oils of PAm and PM, respectively.

A total of 76 and 93 compounds were characterized in P. sieheana (PS) and Phlomis armenica (PAr) essential oils, representing 79.8% and 77.1% of the total oils, respectively. Germacrene-D (16.6% and 23.4%) and (Z)-β-farnesene (11.7% and 6.2%) were identified as the major constituents of PS and PAr essential oils, respectively.

Altogether a 143 volatile compounds were identified within the investigated Phlomis species in this study. To the best of our knowledge, this is the first report on the essential oil chemistry of these species. GC–MS analyses showed two interesting compounds to be present in some of the investigated Phlomis essential oils, a diterpene (1) and an iridoid derivative (2).

3.2 Structure elucidation

The unknown compound (1) was isolated from PM essential oil by column chromatography. The IR spectrum of 1 showed the absorption band characteristic for a hydroxyl group at 3546 cm⁻¹. Its EI-mass spectrum gave a molecular ion peak at m/z 288, and a fragment peak at m/z 273 [M⁺ − CH₃] among others. The HR-EI-MS analysis of the molecular ion peak at m/z 288.2458 suggested a molecular formula of C₂₀H₃₂O, confirming 5° of unsaturation for 1. The ¹H NMR spectrum (data given in Table 3) of 1 showed the presence of four tertiary methyl groups at δ 0.83, 0.85, 0.89 and 1.05, an oxygenated methine group at δ 4.03 (ddd, J = 5, 7, 7 Hz) and an sp² methine proton at δ 5.30 (br t, J = 2 Hz), and vinyl group protons, which were mutually spin coupled at δ 4.92 (dd, J = 1, 10 Hz), 5.01 (dd, J = 1, 17 Hz) and 5.88 (dd, J = 10, 17 Hz). The ¹³C NMR spectrum of 1 indicated the presence of 20 carbons, including 4 sp² carbons and the oxygenated methine group at δ 66.2. Conclusively, the spectral data suggested that 1 was a tricyclic compound.

Analysis of the HMQC and HMBC spectra supported the structural assignment (details in Table 3). The long range ¹H–¹³C correlation of two tertiary methyls at δ_H 0.85 and 0.89 (H₃-19, 18) with a methylene carbon at δ_C 42.0 (C-3), a quaternary carbon at δ 33.4 (C-4) and a methine carbon at δ 54.8 (C-5), and mutual ¹H–¹³C correlation between the both methyl groups, supported that the two methyls were gem-dimethyl structure in compound 1. Further correlation between the methyl proton signal at δ_H 0.83, the methine carbon at δ_C 54.8, and δ_C 59.9 was observed, respectively. The signal at δ_C 59.9 showed ¹J-direct coupling with a broad doublet signal at δ_H 1.75 in the HMQC spectrum. The methine proton at δ_H 1.75 showed spin–spin coupling with the oxygenated methine proton at δ_H 4.03 in the ¹H–¹H COSY spectrum of 1. The remaining methyl group at δ_H 1.05 correlated with sp² carbon at δ_C 149.1 which was attached by the vinyl proton at δ_H 5.88, and methylene carbon at δ_C 43.4 whose proton showed spin–spin coupling with the oxygenated methine proton.

Consideration of these spectral data and further ¹H–¹³C correlations (summarized in Table 2) led to the conclusion that the structure of 1 was 8(14),15-isopimaradiene-11α-ol.

Extensive NOESY (also summarized in Table 3) spectral analysis allowed us to define the stereochemistry of the hydroxyl group at C-11. Since NOE correlation (as shown in Fig. 2) between C-11 proton and H₃-17, 20 and H-1_eq protons was observed, the hydroxyl group at C-11 of compound 1 should have α-equatorial orientation. Further NOE correlation (summarized in Table 3) between H-5 proton and H-1_ax and H-9 protons was in particular important for the confirmation of the stereochemistry of the ring junction of 1 which was assigned in trans position. Accordingly, the structure of compound 1 was elucidated as 8(14),15-isopimaradiene-11α-ol (=11α-hydroxy-sandaracopimara-8(14),15-diene). To the best of our knowledge this is the first report on this compound isolated from essential oils. However, a very recent report coincides with the same structure; also isolated from a Turkish endemic P. amanica where all the spectroscopic data are in agreement with amanicadol [8].

3.3 Determination of fulvoiridoid

GC–MS analyses of the essential oils showed an unknown minor compound with a molecular weight of 190 corresponding to C₁₁H₁₀O₃ from the computer peak matching against the commercial Wiley GC–MS Library [15]. As the relative contents of 2 were in minor amounts within the oils, chemical derivatization aided in the structure elucidation. The suggested iridoid agylcone (2) was obtained from the iridoid (3) frequently occurring in Phlomis species [5–8] including the investigated species in this study.

For the identification of compound 2, the iridoid ipolamiide (3) was subjected to acid hydrolysis. The resulting compound 4-methoxycarbonyl-7-methyl cyclopenta[c]pyrane (2) was characterized by co-injection of the Phlomis essential oils to confirm its presence in the oils of PAr (1.4%) and PS (0.2%). This compound was previously also reported as a transformation product of ipolamiide after acid hydrolysis, and was classified as a fulvoiridoid (or pseudoazulene) [11]. To the best of our knowledge, this is the first report of the rare compound 2 in an essential oil as a natural product. The presence of 3 in Phlomis species supports the hydrolytic formation of compound 2 from hydrodistillations possibly as an artifact as shown in Scheme 1.

3.4 Antimicrobial activity

Phlomis essential oils were investigated first for their antifungal properties using a TLC bioautographic assay where the diterpene (1) was shown as the active principle against C. albicans and C. tropicalis when compared to the standard antifungal agent. A strong inhibitory zone was observed in the bioautographic assay when compared with the antifungal standards, especially PAm essential oil was followed by PM and PL oils. Minimum inhibitory concentrations (MICs) against various human pathogenic bacteria and C. albicans were determined using a microdilution assay. As seen in Table 4, weak to moderate antibacterial activity of the tested essential oils was observed (from MICs 500 to >1000 μg/ml) with exception against the pathogen Bacillus cereus (125–500 μg/ml). PM oil showed relatively good inhibition against B. cereus. The activity observed in the bioautographic assay against Candida sp. was repeated with a strong inhibitory effect of the PAm essential oil with decreasing action of PM and PL, respectively (62.5–1000 μg/ml). The relative percentage amount of the diterpene 8(14),15-isopimaradiene-11α-ol (1) showed correlation with the anticandidal effect in a dose response fashion.

In conclusion, the essential oils of Phlomis species are a natural source for antimicrobial and in particular antifungal applications. It is worthwhile to investigate further parts and species from this widespread genus.