Cyclonerane Derivatives from the Algicolous Endophytic Fungus Trichoderma asperellum A-YMD-9-2

Abstract

Seven previously unreported cyclonerane derivatives, namely, 3,7,11-trihydroxycycloneran-10-one, cycloneran-3,7,10,11-tetraol, cycloneran-3,7,11-triol, 11,12,15-trinorcycloneran-3,7,10-triol, 7,10S-epoxycycloneran-3,15-diol, 7,10R-epoxycycloneran-3,15-diol, and (10Z)-15-acetoxy-10-cycloneren-3,7-diol, were isolated in addition to the known (10Z)-cyclonerotriol, (10E)-cyclonerotriol, catenioblin C, and chokol E from the culture of Trichoderma asperellum A-YMD-9-2, an endophytic fungus obtained from the marine red alga Gracilaria verrucosa. The structures of previously unreported compounds were established by spectroscopic techniques, including 1D/2D NMR, MS, and IR. The isolation of these new cyclonerane derivatives greatly adds to the structural diversity of unusual cyclonerane sesquiterpenes, and several isolates exhibit potent inhibition against some marine phytoplankton species.

1. Introduction

Trichoderma species have proven to be prolific sources of diterpenes and sesquiterpenes, especially some unusual terpene skeletons, such as harziane, proharziane, wickerane, citrinovirin, trichaspin, and cyclonerane [1,2,3,4,5,6,7,8]. Of the cyclonerane-type sesquiterpenes, cyclonerodiol and its analogs have been isolated from several species of Trichoderma [4,5,6,9,10,11,12,13,14]. To date, around 30 cyclonerane sesquiterpenes have been characterized, and almost half of them occurred in Trichoderma species. In our ongoing search for new and bioactive metabolites from marine algicolous fungi [15], an endophytic strain (A-YMD-9-2) of Trichoderma asperellum, isolated from the marine red alga Gracilaria verrucosa, was chemically examined. As a result, seven new cyclonerane derivatives, namely, 3,7,11-trihydroxycycloneran-10-one (1), cycloneran-3,7,10,11-tetraol (2), cycloneran-3,7,11-triol (3), 11,12,15-trinorcycloneran-3,7,10-triol (4), 7,10S-epoxycycloneran-3,15-diol (5), 7,10R-epoxycycloneran-3,15-diol (6), and (10Z)-15-acetoxy-10-cycloneren-3,7-diol (7), together with four known compounds, namely, (10Z)-cyclonerotriol (8) [16], (10E)-cyclonerotriol (9) [16,17], catenioblin C (10) [18], and chokol E (11) [19], were isolated and identified (Figure 1). Herein, the isolation, structure elucidation, and bioactivity of these compounds are described in detail.

2. Results and Discussion

Compound 1 was obtained as a colorless oil. The molecular formula C₁₅H₂₈O₄ was determined by HREIMS m/z 272.1991 [M]⁺ (calculated for C₁₅H₂₈O₄, 272.1988), requiring two degrees of unsaturation. Its IR absorption bands at 3440 and 1713 cm⁻¹ suggested the presence of hydroxy and carbonyl groups. In combination with HSQC data, the ¹H NMR spectrum (

Table 1. ¹H NMR Data for 1–7 (500 MHz, in CDCl₃, δ in ppm, J in Hz).

Position	1	2	3	4	5	6	7
1 (β)	1.03, d (6.8)	1.03, d (6.8)	1.03, d (6.8)	1.05, d (6.8)	1.02, d (6.8)	1.02, d (6.8)	1.04, d (6.8)
2 (α)	1.56, m	1.55, m	1.59, m	1.60, m	1.50, m	1.54, m	1.60, m
4a	1.67, m	1.69, m	1.67, m	1.69, m	1.68, m	1.68, m	1.68, m
4b	1.56, m	1.56, m	1.55, m	1.56, m	1.59, m	1.58, m	1.55, m
5a	1.88, m	1.88, m	1.85, m	1.88, m	1.89, m	1.89, m	1.85, m
5b	1.63, m	1.56, m	1.54, m	1.55, m	1.49, m	1.40, m	1.55, m
6 (β)	1.97, m	1.89, m	1.85, m	1.87, m	1.95, m	2.00, m	1.84, m
8a	2.12, m	1.73, m	1.44, m	1.57, m	1.75, m	1.86, m	1.50, t (8.3)
8b	1.89, m	1.59, m			1.64, m	1.69, m
9a	2.51, m	1.61, m	1.44, m	1.68, m	1.92, m	1.83, m	2.16, m
9b		1.40, m			1.71, m	1.79, m
10		3.38, br d (10.3) a	1.45, m	3.68, m	4.07, ddd (7.6, 6.9, 4.1)	4.04, ddd (9.8, 5.6, 4.3)	5.41, t (7.3)
11					1.93, m	2.00, m
12	1.30, s	1.16, s	1.22, s		0.93, d (7.0)	0.90, d (7.1)	1.74, br s
13 (α)	1.25, s	1.25, s	1.25, s	1.26, s	1.24, s	1.25, s	1.25, s
14	1.19, s	1.15, s	1.16, s	1.17, s	1.14, s	1.17, s	1.16, s
15a	1.29, s	1.21, s	1.22, s		3.65, d (10.8, 6.1)	3.69, dd (10.8, 6.9)	4.62, d (11.9)
15b					3.61, d (10.8, 4.1)	3.58, dd (10.8, 3.7)	4.57, d (11.9)
CH3CO							2.06, s

^a H-10 is coupled with H-9a and H-9b, but one of the couplings only results in broad resonance.

) showed one methyl doublet, four methyl singlets, and an array of signals at δ_H 1.5–2.6 for four methylenes and two methines. Aided by the 90° and 135° DEPT experiments, 15 resonances in the ¹³C NMR spectrum (

Table 2. ¹³C NMR data for 1–7 (125 MHz, in CDCl₃, δ in ppm).

Position	δC, Type
	1	2	3	4	5	6	7
1	14.4, CH3	14.5, CH3	14.7, CH3	14.6, CH3	14.0, CH3	13.8, CH3	14.7, CH3
2	44.9, CH	44.7, CH	44.4, CH	44.5, CH	45.4, CH	45.3, CH	44.4, CH
3	81.4, C	81.5, C	81.5, C	81.4, C	81.3, C	81.4, C	81.4, C
4	40.4, CH2	40.4, CH2	40.5, CH2	40.5, CH2	40.5, CH2	40.4, CH2	40.5, CH2
5	24.8, CH2	24.5, CH2	24.4, CH2	24.6, CH2	25.1, CH2	25.4, CH2	24.5, CH2
6	55.1, CH	54.5, CH	54.3, CH	54.9, CH	54.2, CH	54.1, CH	54.6, CH
7	76.0, C	75.1, C	75.0, C	74.8, C	85.7, C	86.0, C	74.8, C
8	31.5, CH2	37.0, CH2	41.1, CH2	36.8, CH2	35.7, CH2	34.8, CH2	40.5, CH2
9	32.8, CH2	25.8, CH2	18.7, CH2	27.2, CH2	28.1, CH2	27.4, CH2	22.5, CH2
10	215.1, C	79.0, CH	44.5, CH2	63.6, CH2	80.3, CH	84.2, CH	131.1, CH
11	79.4, C	73.4, C	71.2, C		38.2, CH	37.4, CH	130.0, C
12	27.8, CH3	23.5, CH3	29.4, CH3		11.8, CH3	12.0, CH3	21.6, CH3
13	26.3, CH3	26.2, CH3	26.2, CH3	26.2, CH3	26.2, CH3	26.2, CH3	26.2, CH3
14	23.5, CH3	25.0, CH3	25.2, CH3	25.2, CH3	23.1, CH3	26.4, CH3	25.0, CH3
15	28.0, CH3	26.7, CH3	29.5, CH3		66.9, CH2	66.7, CH2	63.3, CH2
CH3CO							171.3, C
CH3CO							21.1, CH3

) were assigned to five methyls, four methylene sp³, two methine sp³, three quaternary sp³ and one quaternary sp² carbons. The ¹³C NMR spectrum of 1 exhibited the signals at δ_C 79.4 and 215.1, attributed to an oxygenated quaternary sp³ carbon and a ketone carbonyl group, respectively, instead of the signals for the vinyl group in cyclonerodiol [20]. HMBC correlations from H₃-12 (δ_H 1.30) to C-10 (δ_C 215.1), C-11 (δ_C 79.4), and C-15 (δ_C 28.0) and from H₃-15 (δ_H 1.29) to C-10, C-11, and C-12 (δ_C 27.8) established the connectivity between C-10 and C-11, which then extended to C-8 (δ_C 31.5) as corroborated by the HMBC correlation from H₂-9 (δ_H 2.51) to C-10 as well as by the COSY correlation from H₂-8 (δ_H 2.12 and 1.89) to H₂-9. The connectivity around ring A was deduced to be the same as those of cyclonerodiol based on their identical NMR data, and this was confirmed by the COSY correlations from H₃-1 (δ_H 1.03)/H-2 (δ_H 1.56)/H-6 (δ_H 1.97)/H₂-5 (δ_H 1.88 and 1.63)/H₂-4 (δ_H 1.67 and 1.56) and HMBC correlations from H₃-1 to C-2 (δ_C 44.9), C-3 (δ_C 81.4), and C-6 (δ_C 55.1), from H₃-13 (δ_H 1.25) to C-2, C-3, and C-4 (δ_C 40.4), and from H₃-14 (δ_H 1.19) to C-6, C-7 (δ_C 76.0), and C-8 (δ_C 31.5) (Figure 2). The NOESY correlation from H₃-1 to H-6 further verified that Me-1 was syn to H-6, while the NOESY correlations from H₃-1 to H-5a (δ_H 1.88) and from H₃-13 to H-5b (δ_H 1.63) suggested Me-1 to be opposite to Me-13. The above information evidenced 1 to be 3,7,11-trihydroxycycloneran-10-one.

Compound 2 was isolated as a colorless oil, and its molecular formula was established as C₁₅H₃₀O₄, which has two more hydrogen atoms than that of 1, based on the (+)-HREIMS m/z 297.2037 [M + Na]⁺ (calculated for C₁₅H₃₀O₄Na, 297.2042). A detailed comparison of its NMR signals (Table 1 and Table 2) with those of 1 revealed the presence of ring A and its affiliated groups in 2. In addition, this compound exhibited a deshielded broad doublet (J = 10.3 Hz) at δ_H 3.38 in the ¹H NMR spectrum. Combined with the HSQC correlation of this proton signal to the carbon signal at δ_C 79.0, this signal was attributed to the oxymethine proton on C-10. This was supported by the HMBC correlations from oxymethine sp³ carbon at δ_C 79.0 (C-10) to H₃-12 (δ_H 1.16) and H₃-15 (δ_H 1.21) as well as a COSY correlation from H-10 to H₂-9 (δ_H 1.61 and 1.40) (Figure 2). Thus, 2 was deduced to be cycloneran-3,7,10,11-tetraol. Previously, cyclonerodiol B from the mangrove-derived endophytic fungus Trichoderma sp. Xy24 was assigned the same structure as 2, but it should be revised to epicyclonerodiol oxide in view of their identical NMR data [9,13]. To confirm the absolute configuration at C-10, Mosher’s reactions were performed under the conditions described previously [21]. Unfortunately, no esterified products were obtained after the purification via preparative thin-layer chromatography (TLC).

Compound 3 was purified as a colorless oil, and its HREIMS m/z 258.2198 [M]⁺ (calculated for C₁₅H₃₀O₃, 258.2195) produced the molecular formula C₁₅H₃₀O₃, which has one oxygen atom less than that of 2. Its ¹³C NMR spectrum (Table 2) showed a close similarity to that of 2, except for the lack of the signal for an oxymethine group and the presence of the signal for a methylene group of C-10 (δ_C 44.5), which was supported by its HMBC correlations to H₃-12 (δ_H 1.22) and/or H₃-15 (δ_H 1.22). Other HMBC and COSY correlations, as shown in Figure 2, further confirmed 3 to be cycloneran-3,7,11-triol, a 10-deoxy derivative of 2.

Compound 4 was also isolated as a colorless oil. A molecular formula C₁₂H₂₄O₃ was assigned by HREIMS m/z 216.1724 [M]⁺ (calculated for C₁₂H₂₄O₃, 216.1725), implying one degree of unsaturation. Its ¹H and ¹³C NMR data (Table 1 and Table 2) resembled those of 2, except for the lack of signals for a 2-hydroxy-2-propyl group (δ_H 1.16 and 1.21, δ_C 23.5, 26.7, and 73.4) and the presence of signals for a hydroxymethylene group (δ_H 3.68 and δ_C 63.6). This group was deduced to be situated at the side chain terminus on the basis of HMBC correlations from H₃-14 (δ_H 1.17) to C-6 (δ_C 54.9), C-7 (δ_C 74.8), and C-8 (δ_C 36.8) and COSY correlations from H₂-10 (δ_H 3.68) to H₂-9 (δ_H 1.68) and from H₂-9 to H₂-8 (δ_H 1.57). HMBC correlations (Figure 2) from H₃-1 (δ_H 1.05) to C-2 (δ_C 44.5), C-3 (δ_C 81.4), and C-6, and from H₃-13 (δ_H 1.26) to C-2, C-3, and C-4 (δ_C 40.5), and COSY correlations from H₃-1 to H₂-4 (δ_H 1.69 and 1.56) via H-2 (δ_H 1.60), H-6 (δ_H 1.87), and H₂-5 (δ_H 1.88 and 1.55), further verified the connectivity of ring A. Thus, 4 was proposed to be 11,12,15-trinorcycloneran-3,7,10-triol, possibly a degradation product of 1 or 2. To ascertain the relative configuration at C-7, the energy-minimized conformers, regardless of the rotation of the methyl and hydroxy groups as well as the side chain, of 7α- and 7β-methyl isomers optimized at the B3LYP/6-31G(d) level in chloroform, were subjected to the ¹³C NMR calculations using the gauge-independent atomic orbital (GIAO) method at the B3LYP/6-31+G(d,p) level via Gaussian 09 software [22]. Both experimental and calculated shifts were input into Sarotti’s DP4+ sheet (see https://sarotti-nmr.weebly.com) [23], and the calculated data for 7α- and 7β-methyl isomers displayed 73.74% and 26.26% DP4+ probabilities, respectively. Thus, the methyl group at C-7 was tentatively assigned as α orientation.

Compound 5 was obtained as a colorless oil, and the HREIMS spectrum afforded the molecular formula C₁₅H₂₈O₃, suggesting two degrees of unsaturation. However, examination of the ¹H and ¹³C NMR data (Table 1 and Table 2) indicated the absence of any unsaturated bond. Thus, this compound was suggested to possess a bicyclic skeleton. As the NMR data of 5 resembled those of 7,10-epoxycycloneran-3,11,12-triol, the presence of a 7,10-epoxycyclonerane framework was proposed [5]. However, the signal for a methine group appeared in the ¹³C NMR spectrum of 5 instead of that for an oxygenated quaternary carbon in the ¹³C NMR spectrum of 7,10-epoxycycloneran-3,11,12-triol. The fact that the methine group was located at C-11 (δ_C 38.2) of 5 was corroborated by its HMBC correlations with H₃-12 (δ_H 0.93) and H₂-15 (δ_H 3.65 and 3.61). HMBC correlations (Figure 2) from H₃-12 and H₂-15 to C-10 (δ_C 80.3), from H₃-1 (δ_H 1.02) to C-2 (δ_C 45.4), C-3 (δ_C 81.3), and C-6 (δ_C 54.2), from H₃-13 (δ_H 1.24) to C-2, C-3, and C-4 (δ_C 40.5), and from H₃-14 (δ_H 1.14) to C-6, C-7 (δ_C 85.7), and C-8 (δ_C 35.7) further confirmed the structure of 5 as 11-deoxy derivative of 7,10-epoxycycloneran-3,11,12-triol. Additionally, H-10 (δ_H 4.07) and Me-14 (δ_H 1.14) were on the same face of ring B by their NOESY correlation (Figure 3). The NOESY correlations from H₃-1 to H-5a (δ_H 1.89) and H-6 (δ_H 1.95) and from H₃-13 to H-5b (δ_H 1.49) validated the relative configurations around ring A. However, the relative configuration at C-11 remains unsolved.

Compound 6 was isolated as a colorless oil and has the same molecular formula as that of 5 by HREIMS m/z 256.2028 [M]⁺ (calcd for C₁₅H₂₈O₃, 256.2038). Its ¹H and ¹³C NMR data (Table 1 and Table 2) also resembled those of 5, except for the deshielded signal for C-10 (δ_C 84.2). Thus, 6 was deduced to be a C-10 epimer of 5, as supported by the NOESY correlation from H₃-12 (δ_H 0.90) to H₃-14 (δ_H 1.17). The similar chemical shifts of C-7 (δ_C 86.0) and C-10 (δ_C 84.2) to those of epicyclonerodiol oxide further evidenced the opposite orientation of H-10 and C-14 [9]. The relative configurations around ring A and at C-7 were deduced to be the same as those of 5 based on their identical ¹H and ¹³C NMR data. Moreover, because both C-6 and C-7 are chiral centers, the rotation of the C-6–C-7 single bond is restricted to some extent. Thus, the relative configuration at C-7 could be locked by the NOESY correlations from H₃-14 to H-2 (δ_H 1.54) and H-5b (δ_H 1.40) and from H-8a (δ_H 1.86) to H₃-1 (δ_H 1.02) and H-2 (Figure 3). As is the case for 5, the relative configuration at C-11 (δ_C 37.4) is not determined.

Compound 7 was obtained as a colorless oil. Its molecular formula was determined to be C₁₇H₃₀O₄ by HREIMS (m/z 298.2138), corresponding to three degrees of unsaturation. The carbonyl signal at δ_C 171.3 and the methyl signals at δ_H 2.06 and δ_C 21.1 as well as their HMBC correlation indicated the presence of an acetyl group. The remaining NMR data (Table 1 and Table 2) showed a close similarity to those of (10Z)-cyclonerotriol (8) [16]. Thus, 7 was speculated to be an acetylated derivative of 8, and the acetoxy group was attached to C-15, as evidenced from the HMBC correlation from H₂-15 (δ_H 4.62 and 4.57) to the carbonyl carbon (δ_C 171.3). Other HMBC and COSY correlations (Figure 2) further validated the structure of 7, and the Z geometry was corroborated by the NOESY correlations between H₂-15 and H₂-9 (δ_H 2.16) and between H₃-12 (δ_H 1.74) and H-10 (δ_H 5.41).

To develop new inhibitors against harmful microalgae that seriously threaten marine aquaculture, 1–11 were evaluated for their growth inhibition against four marine phytoplankton species (Chattonella marina, Heterosigma akashiwo, Karlodinium veneficum, and Prorocentrum donghaiense) [24]. The results (

Table 3. Inhibition against four marine phytoplankton species by 1–11.

Compound	IC50 (μg/mL)
	Chattonella marina	Heterosigma akashiwo	Karlodinium veneficum	Prorocentrum donghaiense
1	5.2	8.0	10	9.9
2	8.8	21	76	6.5
3	61	73	71	40
4	13	73	6.3	34
5	2.4	26	3.9	20
6	5.8	37	5.5	15
7	59	14	35	7.3
8	42	50	12	3.4
9	15	53	43	1.1
10	1.6	1.8	1.6	2.0
11	62	9.4	13	6.0

) show that 10, with IC₅₀ values ranging from 1.6 to 2.0 μg/mL, is the most potent to inhibit the four phytoplankton species tested. An analysis of the structure–activity relationship suggested that the carboxyl group at C-15 may greatly contribute to the inhibitory ability of cyclonerane sesquiterpenes. Moreover, the toxicity of 10 to the marine zooplankton Artemia salina was also assayed [7], but it does not exhibit any lethal effect at the concentration of 100 μg/mL.

3. Materials and Methods

3.1. General Experimental Procedures

Optical rotations and ECD curves were determined on a Chirascan CD spectrometer (Applied Photophysics Ltd., Surrey, UK). IR spectra were obtained on a Nicolet iS10 FT-IR spectrometer (Thermo Fisher Scientific, Waltham, MA, USA). NMR spectra were recorded on a Bruker Avance III 500 NMR spectrometer (Bruker Corp., Billerica, MA, USA). Low- and high-resolution EI and ESI⁺ mass spectra were measured on an Autospec Premier P776 mass spectrometer (Waters Corp., Milford, MA, USA) and an Agilent G6230 TOF mass spectrometer (Agilent Technologies Inc., Santa Clara, CA, USA), respectively. Column chromatography (CC) was carried out with silica gel (200–300 mesh, Qingdao Haiyang Chemical Co., Qingdao, China), RP-18 (AAG12S50, YMC Co., Ltd., Kyoto, Japan), and Sephadex LH-20 (GE Healthcare, Uppsala, Sweden). Thin-layer chromatography (TLC) was performed with precoated silica gel plates (GF-254, Qingdao Haiyang Chemical Co., Qingdao, China). Quantum chemical calculations were run with Gaussian 09 software (Gaussian, Inc., Wallingford, CT, USA).

3.2. Fungal Material and Fermentation

The fungal strain Trichoderma asperellum A-YMD-9-2 (Moniliaceae) was obtained from the inner tissue of the marine red alga Gracilaria verrucosa collected from Yangma Island, Yantai, China in August 2016. The fungus was identified by morphological observation and by analysis of the ITS regions of its rDNA, whose sequence data were deposited at GenBank with the accession number MH819724. The fermentation was performed statically at room temperature for 40 days in 200 × 1 L Erlenmeyer flasks, each containing 50 g rice, 0.6 g peptone, 50 mL pure water, and 50 mL natural seawater from the coast of Yantai, China.

3.3. Extraction and Isolation

The mycelia and broth were separated by filtration at the end of the fermentation, and the former were dried in the shade and exhaustively extracted with CH₂Cl₂ and MeOH (1:1, v/v). After removing organic solvents under a vacuum, the residue was partitioned between EtOAc and H₂O to afford an EtOAc-soluble extract (202.1 g). The broth was directly extracted with EtOAc and then concentrated to give an extract (10.3 g). Based on the similar TLC profiles, these two parts were combined and subjected to silica gel CC with step-gradient solvent systems consisting of petroleum ether (PE)/EtOAc (50:1 to 0:1) and then CH₂Cl₂/MeOH (10:1 to 0:1) to give eight fractions (Frs. 1–8). Fr. 3 eluted with PE/EtOAc (2:1) and was further purified by CC on RP-18 (MeOH/H₂O, 3:2) and silica gel (PE/EtOAc, 6:1) to obtain 1 (11.3 mg), 5 (5.2 mg), and 6 (5.9 mg). Fr. 4 eluted with PE/EtOAc (1:1) and was further purified by CC on RP-18 (MeOH/H₂O, 1:1 to 3:2) and Sephadex LH-20 (MeOH) and preparative TLC (CH₂Cl₂/MeOH, 15:1) to yield 7 (8.1 mg), 8 (33.8 mg), 10 (10.1 mg), and 11 (3.6 mg). Fr. 5 eluted with EtOAc and was further purified by CC on RP-18 (MeOH/H₂O, 2:3 to 3:2) and Sephadex LH-20 (MeOH) and preparative TLC (CH₂Cl₂/MeOH, 10:1) to give 2 (26.0 mg), 4 (1.7 mg), and 9 (10.0 mg). Fr. 6 eluted with CH₂Cl₂/MeOH (10:1) and was further purified by CC on RP-18 (MeOH/H₂O, 1:1) and Sephadex LH-20 (MeOH) and preparative TLC (CH₂Cl₂/MeOH, 7:1) to produce 3 (12.0 mg).

3,7,11-Trihydroxycycloneran-10-one (1): Colorless oil; [α]²⁰_D − 24 (c 0.44, MeOH); IR (KBr) v_max 3440, 2960, 2932, 1713, 1460, 1663, 1374, 1239, 1125, 1013, 921 cm⁻¹; ¹H and ¹³C NMR data, Table 1 and Table 2 (Figures S1 and S2); 2D NMR data, Figures S3–S6; EIMS m/z (%) 272 [M]⁺ (<1), 196 (12), 178 (45), 141 (95), 136 (44), 121 (39), 95 (39), 71 (40), 56 (40), 44(100); HREIMS m/z 272.1991 [M]⁺ (calcd for C₁₅H₂₈O₄, 272.1988) (Figure S7).

Cycloneran-3,7,10,11-tetraol (2): Colorless oil; [α]²⁰_D − 30 (c 1.0, MeOH); IR (KBr) v_max 3416, 2967, 1654, 1460, 1378, 1266, 1162, 1074, 1032, 921, 885 cm⁻¹; ¹H and ¹³C NMR data, Table 1 and Table 2 (Figures S8 and S9); 2D NMR data, Figures S10–S13; ESI⁺MS m/z 297 [M + Na]⁺; HRESI⁺MS m/z 297.2037 [M + Na]⁺ (calcd for C₁₅H₃₀O₄Na, 297.2042) (Figure S14).

Cycloneran-3,7,11-triol (3): Colorless oil; [α]²⁰_D − 18 (c 0.62, MeOH); IR (KBr) v_max 3406, 2965, 1654, 1460, 1377, 1164, 920, 885 cm⁻¹; ¹H and ¹³C NMR data, Table 1 and Table 2 (Figures S15 and S16); 2D NMR data, Figures S17–S20; EIMS m/z (%) 258 [M]⁺ (<1), 207 (25), 157 (28), 139 (81), 127 (70), 109 (81), 95 (38), 81(45), 44(100); HREIMS m/z 258.2198 [M]⁺ (calcd for C₁₅H₃₀O₃, 258.2195) (Figure S21).

11,12,15-Trinorcycloneran-3,7,10-triol (4): Colorless oil; [α]²⁰_D − 39 (c 0.062, MeOH); IR (KBr) v_max 3426, 2928, 1720, 1635, 1460, 1383, 1054, 920 cm⁻¹; ¹H and ¹³C NMR data, Table 1 and Table 2 (Figures S22 and S23); 2D NMR data, Figures S24–S27; EIMS m/z (%) 216 [M]⁺ (<1), 165 (11), 157 (11), 139 (79), 103 (31), 96 (40), 85 (98), 81(58), 44(100); HREIMS m/z 216.1724 [M]⁺ (calcd for C₁₂H₂₄O₃, 216.1725) (Figure S28).

7,10S-epoxycycloneran-3,15-diol (5): Colorless oil; [α]²⁰_D +11 (c 0.20, MeOH); IR (KBr) v_max 3426, 2965, 2931, 2876, 1654, 1460, 1376, 1205, 1092, 1024, 919 cm⁻¹; ¹H and ¹³C NMR data, Table 1 and Table 2 (Figures S29 and S30); 2D NMR data, Figures S31–S34; EIMS m/z (%) 256 [M]⁺ (<1), 183 (20), 143 (100), 139 (32), 125 (35), 113 (30), 59 (42), 44(100); HREIMS m/z 256.2034 [M]⁺ (calcd for C₁₅H₂₈O₃, 256.2038) (Figure S35).

7,10R-epoxycycloneran-3,15-diol (6): Colorless oil; [α]²⁰_D +6.5 (c 0.31, MeOH); IR (KBr) v_max 3426, 2965, 2931, 2868, 1635, 1460, 1376, 1206, 1152, 1093, 1024, 919 cm⁻¹; ¹H and ¹³C NMR data, Table 1 and Table 2 (Figures S36 and S37); 2D NMR data, Figures S38–S41; EIMS m/z (%) 256 [M]⁺ (<1), 237 (8), 179 (10), 143 (90), 125 (32), 95 (28), 56 (41), 44(100); HREIMS m/z 256.2028 [M]⁺ (calcd for C₁₅H₂₈O₃, 256.2038) (Figure S42).

(10Z)-15-Acetoxy-10-cycloneren-3,7-diol (7): Colorless oil; [α]²⁰_D − 11 (c 0.31, MeOH); IR (KBr) v_max 3452, 2963, 2932, 1735, 1654, 1460, 1370, 1240, 1025, 920, 885 cm⁻¹; ¹H and ¹³C NMR data, Table 1 and Table 2 (Figures S43 and S44); 2D NMR data, Figures S45–S48; EIMS m/z (%) 256 [M]⁺ (<1), 139 (33), 125 (98), 107 (28), 81 (27), 44(100); HREIMS m/z 298.2138 [M]⁺ (calcd for C₁₇H₃₀O₄, 298.2144) (Figure S49).

4. Conclusions

Chemical examination of the marine-alga-endophytic fungus Trichoderma asperellum A-YMD-9-2 led to the isolation and identification of seven new (1–7) and four known (8–11) cyclonerane derivatives, including an unprecedented trinorcyclonerane (4). The discovery of these new isolates greatly diversifies the unusual cyclonerane sesquiterpenes. Among the isolates, 10 displays significant inhibition of the four phytoplankton species and features no toxicity to any of the zooplankton tested.