Citriquinolinones A and B: Rare Isoquinolinone-Embedded Citrinin Analogues and Related Metabolites from the Deep-Sea-Derived Aspergillus versicolor 170217

A systematic chemical investigation of the deep-sea-derived fungus Aspergillus versicolor 170217 resulted in the isolation of six new (1–6) and 45 known (7–51) compounds. The structures of the new compounds were established on the basis of exhaustive analysis of their spectroscopic data and theoretical–statistical approaches including GIAO-NMR, TDDFT-ECD/ORD calculations, DP4+ probability analysis, and biogenetic consideration. Citriquinolinones A (1) and B (2) feature a unique isoquinolinone-embedded citrinin scaffold, representing the first exemplars of a citrinin–isoquinolinone hybrid. Dicitrinones K–L (3–4) are two new dimeric citrinin analogues with a rare CH-CH3 bridge. Biologically, frangula-emodin (32) and diorcinol (17) displayed remarkable anti-food allergic activity with IC50 values of 7.9 ± 3.0 μM and 13.4 ± 1.2 μM, respectively, while diorcinol (17) and penicitrinol A (20) exhibited weak inhibitory activity against Vibrio parahemolyticus, with MIC values ranging from 128 to 256 μM.


Introduction
Natural products play a dominant role in the discovery of drug leads for the treatment of human diseases [1,2].Marine organisms living in harsh surroundings, such as high salt, high pressure, and hypoxic environments, are expected to produce unique secondary metabolites when compared with their terrestrial counterparts in terms of structural diversity and functional features, making them a promising storehouse of new bioactive entities for drug leads discovery [3,4].Of all marine-derived fungi, the genus Aspergillus has been the most studied, as it is ubiquitous among almost all ecosystems and it is rich in bioactive secondary metabolites, with multifarious and intricate structures [5].These include the citrinin family, a compound class that features a 6,8-dihydroxyl-3,4,5-trimethyl-chromene core and exhibits abundant structural diversity by decomposition, dimerization, and trimerization through various pathways [6,7].Therefore, the biological behaviors of these compounds extend from anticancer to antimicrobial activities, influenza neuraminidase inhibitory and anti-osteoporosis effects.However, citrinin derivatives embedded with alkaloid moiety are rarely reported in the literature, with the exception of citrinidines A-E, whose structures involve a proline-derived unit [8].
As part of our ongoing investigation into the chemistry of deep-sea-derived fungi, we obtained an A. versicolor fungus from the intestinal contents of a whale Mesoplodon densirostris from the East China Sea which was stranded in Ningde, China.The primary chromatographic analysis of the extract from a PDA culture revealed the rich chemical diversity of the metabolites; therefore, we conducted an in-depth investigation of this strain to discover novel and active compounds.As a result, four new dimeric citrinin derivatives (1)(2)(3)(4), one new isochromene derivative (5), and one new acetamide (6) (Figure 1), together with 45 known compounds, were obtained.The structures of the new compounds were established on the basis of exhaustive analysis of their spectroscopic data and theoretical-statistical approaches including GIAO-NMR, TDDFT-ECD/ORD calculations, DP4+ probability analysis, or biogenetic consideration.Intriguingly, citriquinolinones A-B (1-2) bear a citrinin scaffold embedded with an unusual isoquinolinone unit, which has not been previously reported in this compound class.and theoretical-statistical approaches including GIAO-NMR, TDDFT-ECD/ORD calc tions, DP4+ probability analysis, or biogenetic consideration.Intriguingly, citriqu linones A-B (1-2) bear a citrinin scaffold embedded with an unusual isoquinolinone u which has not been previously reported in this compound class.

Results and Discussion
Compound 1 was isolated as a yellow powder.It was assigned a molecular formula C 24 H 27 NO 6 due to its HRESIMS peak at m/z 424.1759 [M−H] − , requiring 12 degrees of unsaturation (DOU).The 1 H and 13 C NMR spectroscopic data (Figures S1 and S2, Table 1) revealed the presence of six methyls [δ H 1.25 (3H, dd, J = 6.1 Hz, 1.7 Hz, 10-Me), 1.19 (3H, d, J = 6.8 Hz, 11-Me), 2.05 (3H, s, 12-Me), 2.67 (3H, s, 11 -Me), 2.70 (3H, s, 12 -Me), 1.60 (3H, s, 13 -Me); δ C 21.2 (q, C-10), 19.8 (q, 11-Me), 12.3 (q, C-12), 20.0 (q, C-11 ), 16.7 (q, C-12 ), 29.3 (q, C-13 )]; one methylene [δ H 3.70 (dd, J = 14.2 Hz, 2.4 Hz, H-1 ), 3.60 (dd, J =14.2 Hz, 4.4 Hz, H 2 -1 ); δ C 20.2 (t, C-1 )]; three methines [δ H 4.30 (dq, J = 6.1 Hz, 3.9 Hz, H-2); δ H 2.90 (dq, J = 6.8 Hz, 3.9 Hz, H-3), 8.86 (s, H-10 ); δ C 87. 6   The relative configuration of 1 was partially determined by NOESY experiments.The correlations observed from H-2 to H 3 -11 and H-3 to H 3 -10 indicated that 3-Me and 2-Me are trans-configured (Figure 2).To furtherly determine the relative configuration between C-5 and C-2/3, we performed a quantum chemical calculation of NMR data for the two possible isomers of 1, 2R*,3S*,5 R* and 2R*,3S*,5 S*, along with a DP4+ probability analysis.As a result, the theoretical prediction of the chemical shift of the former showed a better correspondence with the experimental data, with an average probability of 83.04% (Figure 3).Finally, the absolute configuration of 1 was established by a TD-DFT based ECD calculation of the two enantiomers of 1 at the B3LYP/6-31+g (d, p) level, as well as comparison with the experimental data, which indicated the correct configuration as The relative configuration of 1 was partially determined by NOESY experiments.The correlations observed from H-2 to H3-11 and H-3 to H3-10 indicated that 3-Me and 2-Me are trans-configured (Figure 2).To furtherly determine the relative configuration between C-5′ and C-2/3, we performed a quantum chemical calculation of NMR data for the two possible isomers of 1, 2R*,3S*,5′R* and 2R*,3S*,5′S*, along with a DP4+ probability analysis.As a result, the theoretical prediction of the chemical shift of the former showed a better correspondence with the experimental data, with an average probability of 83.04% (Figure 3).Finally, the absolute configuration of 1 was established by a TD-DFT based ECD calculation of the two enantiomers of 1 at the B3LYP/6-31+g (d, p) level, as well as comparison with the experimental data, which indicated the correct configuration as 2R,3S,5′R (Figure 4).Hence, the complete structure of 1 was assigned as shown and named citriquinolinone A. Of note, citriquinolinone A (1) represents the first exemplar of an isoquinolinone-citrinin hybrid.The relative configuration of 1 was partially determined by NOESY experiments.The correlations observed from H-2 to H3-11 and H-3 to H3-10 indicated that 3-Me and 2-Me are trans-configured (Figure 2).To furtherly determine the relative configuration between C-5′ and C-2/3, we performed a quantum chemical calculation of NMR data for the two possible isomers of 1, 2R*,3S*,5′R* and 2R*,3S*,5′S*, along with a DP4+ probability analysis.As a result, the theoretical prediction of the chemical shift of the former showed a better correspondence with the experimental data, with an average probability of 83.04% (Figure 3).Finally, the absolute configuration of 1 was established by a TD-DFT based ECD calculation of the two enantiomers of 1 at the B3LYP/6-31+g (d, p) level, as well as comparison with the experimental data, which indicated the correct configuration as 2R,3S,5′R (Figure 4).Hence, the complete structure of 1 was assigned as shown and named citriquinolinone A. Of note, citriquinolinone A (1) represents the first exemplar of an isoquinolinone-citrinin hybrid.The relative configuration of 1 was partially determined by NOESY experiments.The correlations observed from H-2 to H3-11 and H-3 to H3-10 indicated that 3-Me and 2-Me are trans-configured (Figure 2).To furtherly determine the relative configuration between C-5′ and C-2/3, we performed a quantum chemical calculation of NMR data for the two possible isomers of 1, 2R*,3S*,5′R* and 2R*,3S*,5′S*, along with a DP4+ probability analysis.As a result, the theoretical prediction of the chemical shift of the former showed a better correspondence with the experimental data, with an average probability of 83.04% (Figure 3).Finally, the absolute configuration of 1 was established by a TD-DFT based ECD calculation of the two enantiomers of 1 at the B3LYP/6-31+g (d, p) level, as well as comparison with the experimental data, which indicated the correct configuration as 2R,3S,5′R (Figure 4).Hence, the complete structure of 1 was assigned as shown and named citriquinolinone A. Of note, citriquinolinone A (1) represents the first exemplar of an isoquinolinone-citrinin hybrid.The relative configuration of 1 was partially determined by NOESY experiments.The correlations observed from H-2 to H3-11 and H-3 to H3-10 indicated that 3-Me and 2-Me are trans-configured (Figure 2).To furtherly determine the relative configuration between C-5′ and C-2/3, we performed a quantum chemical calculation of NMR data for the two possible isomers of 1, 2R*,3S*,5′R* and 2R*,3S*,5′S*, along with a DP4+ probability analysis.As a result, the theoretical prediction of the chemical shift of the former showed a better correspondence with the experimental data, with an average probability of 83.04% (Figure 3).Finally, the absolute configuration of 1 was established by a TD-DFT based ECD calculation of the two enantiomers of 1 at the B3LYP/6-31+g (d, p) level, as well as comparison with the experimental data, which indicated the correct configuration as 2R,3S,5′R (Figure 4).Hence, the complete structure of 1 was assigned as shown and named citriquinolinone A. Of note, citriquinolinone A (1) represents the first exemplar of an isoquinolinone-citrinin hybrid.The relative configuration of 1 was partially determined by NOESY experiments.The correlations observed from H-2 to H3-11 and H-3 to H3-10 indicated that 3-Me and 2-Me are trans-configured (Figure 2).To furtherly determine the relative configuration between C-5′ and C-2/3, we performed a quantum chemical calculation of NMR data for the two possible isomers of 1, 2R*,3S*,5′R* and 2R*,3S*,5′S*, along with a DP4+ probability analysis.As a result, the theoretical prediction of the chemical shift of the former showed a better correspondence with the experimental data, with an average probability of 83.04% (Figure 3).Finally, the absolute configuration of 1 was established by a TD-DFT based ECD calculation of the two enantiomers of 1 at the B3LYP/6-31+g (d, p) level, as well as comparison with the experimental data, which indicated the correct configuration as 2R,3S,5′R (Figure 4).Hence, the complete structure of 1 was assigned as shown and named citriquinolinone A. Of note, citriquinolinone A (1) represents the first exemplar of an isoquinolinone-citrinin hybrid.S13, Table 1) and 1 revealed a high degree of similarity, including resonances accounting for the isoquinocitrinin substructure, namely fragment B of 1.The primary differences were attributed to the presence of an aromatic proton (δ H 6.30, s; H-9), as well as the shielding of C-2 (∆δ C -5.5).HMBC correlations from H-1 to C-6/7/8, H-9 to C-5/C-7, together with signals observed from H 3 -11 to C-4 and COSY correlations of H 3 -10/H-2/H-3/-H 3 -11, inferred the penta-substituted benzene fragment A. Considering the molecular formula, the planar structure of 2 was assigned as shown in Figure 5.  1) and 1 revealed a high degree of similarity, including resonances accounting for the isoquinocitrinin substructure, namely fragment B of 1.The primary differences were attributed to the presence of an aromatic proton (δH 6.30, s; H-9), as well as the shielding of C-2 (ΔδC -5.5).HMBC correlations from H-1″ to C-6/7/8, H-9 to C-5/C-7, together with signals observed from H3-11 to C-4 and COSY correlations of H3-10/H-2/H-3/-H3-11, inferred the penta-substituted benzene fragment A. Considering the molecular formula, the planar structure of 2 was assigned as shown in Figure 5.As C-2/3 are not involved in a dihydrofuran ring, in this case, the NOE spectrum is useless for determining its relative configuration.However, compound 2 contains a citrinin moiety similar to that of 1, namely a phenol A unit; we therefore examined the biogenetic relationship between these two compounds.Capon et al. documented a plausible mechanism for the transformation from citrinin to 2,3,5-trimethyl-6,8-dihydrobenzofuran and phenol A, in which the stereo configurations of C-2/3 were retained in the whole process [27].This, along with the co-occurrence of citrinin (30) and phenol A ( 14) in the same extract and a comparison of the chemical shift of fragment A of 2 with that of 14, permitted the appearance of relative/absolute configurations of C-2/3 in 2 same as those observed in 1, 14, and 30.To further assign the relative configuration between C-5′and C-2/3, the NMR data of 2 in MeOH was predicted using the GIAO based calculation, followed by DP4+ analysis.The comparison of the theoretical with the experimental data showed that the 2R*,3S*,5′R* isomer exhibited a 100% probability (Figure 6).Likewise, the absolute configuration of 2 was eventually established to be 2R,3S,5′R by comparing the calculated ECD spectrum with that of the experimental data (Figure S42).Therefore, the structure of 2 was assigned, and the compound was given the trivial name citriquinolinone B.

HO
Compound 3 was isolated as a yellow oil and assigned the molecular formula C24H34O6, based on the HRESI(-)MS peak at m/z 441.2250 [M+Na] + , requiring eight DOU.   1) and 1 revealed a high degree of similarity, including resonances accounting for the isoquinocitrinin substructure, namely fragment B of 1.The primary differences were attributed to the presence of an aromatic proton (δH 6.30, s; H-9), as well as the shielding of C-2 (ΔδC -5.5).HMBC correlations from H-1″ to C-6/7/8, H-9 to C-5/C-7, together with signals observed from H3-11 to C-4 and COSY correlations of H3-10/H-2/H-3/-H3-11, inferred the penta-substituted benzene fragment A. Considering the molecular formula, the planar structure of 2 was assigned as shown in Figure 5.As C-2/3 are not involved in a dihydrofuran ring, in this case, the NOE spectrum is useless for determining its relative configuration.However, compound 2 contains a citrinin moiety similar to that of 1, namely a phenol A unit; we therefore examined the biogenetic relationship between these two compounds.Capon et al. documented a plausible mechanism for the transformation from citrinin to 2,3,5-trimethyl-6,8-dihydrobenzofuran and phenol A, in which the stereo configurations of C-2/3 were retained in the whole process [27].This, along with the co-occurrence of citrinin (30) and phenol A ( 14) in the same extract and a comparison of the chemical shift of fragment A of 2 with that of 14, permitted the appearance of relative/absolute configurations of C-2/3 in 2 same as those observed in 1, 14, and 30.To further assign the relative configuration between C-5′and C-2/3, the NMR data of 2 in MeOH was predicted using the GIAO based calculation, followed by DP4+ analysis.The comparison of the theoretical with the experimental data showed that the 2R*,3S*,5′R* isomer exhibited a 100% probability (Figure 6).Likewise, the absolute configuration of 2 was eventually established to be 2R,3S,5′R by comparing the calculated ECD spectrum with that of the experimental data (Figure S42).Therefore, the structure of 2 was assigned, and the compound was given the trivial name citriquinolinone B.
Compound 3 was isolated as a yellow oil and assigned the molecular formula C24H34O6, based on the HRESI(-)MS peak at m/z 441.2250 [M+Na] + , requiring eight DOU.
) and HMBC (  1) and 1 revealed a high degree of similarity, including resonances accounting for the isoquinocitrinin substructure, namely fragment B of 1.The primary differences were attributed to the presence of an aromatic proton (δH 6.30, s; H-9), as well as the shielding of C-2 (ΔδC -5.5).HMBC correlations from H-1″ to C-6/7/8, H-9 to C-5/C-7, together with signals observed from H3-11 to C-4 and COSY correlations of H3-10/H-2/H-3/-H3-11, inferred the penta-substituted benzene fragment A. Considering the molecular formula, the planar structure of 2 was assigned as shown in Figure 5.As C-2/3 are not involved in a dihydrofuran ring, in this case, the NOE spectrum is useless for determining its relative configuration.However, compound 2 contains a citrinin moiety similar to that of 1, namely a phenol A unit; we therefore examined the biogenetic relationship between these two compounds.Capon et al. documented a plausible mechanism for the transformation from citrinin to 2,3,5-trimethyl-6,8-dihydrobenzofuran and phenol A, in which the stereo configurations of C-2/3 were retained in the whole process [27].This, along with the co-occurrence of citrinin (30) and phenol A ( 14) in the same extract and a comparison of the chemical shift of fragment A of 2 with that of 14, permitted the appearance of relative/absolute configurations of C-2/3 in 2 same as those observed in 1, 14, and 30.To further assign the relative configuration between C-5′and C-2/3, the NMR data of 2 in MeOH was predicted using the GIAO based calculation, followed by DP4+ analysis.The comparison of the theoretical with the experimental data showed that the 2R*,3S*,5′R* isomer exhibited a 100% probability (Figure 6).Likewise, the absolute configuration of 2 was eventually established to be 2R,3S,5′R by comparing the calculated ECD spectrum with that of the experimental data (Figure S42).Therefore, the structure of 2 was assigned, and the compound was given the trivial name citriquinolinone B.
Compound 3 was isolated as a yellow oil and assigned the molecular formula C24H34O6, based on the HRESI(-)MS peak at m/z 441.2250 [M+Na] + , requiring eight DOU.
The relative and absolute configuration of C-2/2 and C-3/3 were deduced in the same manner as that used for 1-2, based on a biogenetic consideration with citrinin (30) and phenol A (14).Finally, by comparison of its calculated and experimental ECD spectra (Figure 8), the absolute configuration of 3 was thus established as 2R,3S,2 R,3 S. Herein, 3 was given the trivial name dicitrinone K.
Compound 4 was isolated as a yellow amorphous solid.The molecular formula of 4 was deduced as C 24 H 28 O 5 from the HRESI(−)MS signal m/z 395.1841 [M−H] − .The 1 H, 13 C NMR and DEPT spectroscopic data revealed 24 carbons, including seven methyl singlets, five methines, and 12 protonated carbons.Similar to those of 3, the carbon signals ure 8), the absolute configuration of 3 was thus established as 2R,3S,2′R,3′S.Herein, 3 was given the trivial name dicitrinone K.By comparison of its calculated and experimental ECD spectra, the absolute configuration was established as 2/2′R,3/3′S (Figure 8), and was given the trivial name dicitrinone L. Compound 5 was isolated as a yellow amorphous solid.Its molecular formula was established as C13H12O6, according to the pseudo molecular ion at m/z 263.0547 [M−H] − in its HRESI(-)MS spectrum, requiring eight DOU.The 1 H-NMR and 13 C NMRDEPT spectroscopic data exhibited 13 carbons (Table 3), including two methyls, one methene, two methines, and eight non-hydrogenated carbons (including one carbonyl and one ketone).According to the key HMBC correlations from H3-12 (δH 2.    Compound 5 was isolated as a yellow amorphous solid.Its molecular formula was established as C13H12O6, according to the pseudo molecular ion at m/z 263.0547 [M−H] − in its HRESI(-)MS spectrum, requiring eight DOU.The 1 H-NMR and 13 C NMRDEPT spectroscopic data exhibited 13 carbons (Table 3), including two methyls, one methene, two methines, and eight non-hydrogenated carbons (including one carbonyl and one ketone).According to the key HMBC correlations from H3-12 (δH 2.  10.Therefore, 5 was identified as (6,8-dihydroxy-4-methyl-1-oxo-1H-isochromen-3-yl) methyl acetate.

General Experimental Procedures
NMR spectra were recorded on a Bruker 400 MHz spectrometer.The HRESIMS spectra were recorded on a Waters Xevo G2 Q-TOF mass spectrometer (Waters Corporation, Milford, MA, USA).Optical rotations were obtained with an Anton Par polarimeter (MCP100).ECD spectra were measured on a Chirascan spectrometer.The semi-preparative HPLC was conducted on an Agilent instrument (1260) equipped with a 1260 Diode Array Detector (DAD) and column COSMOSIL 5 C 18 -MS-II 10 ID × 250 mm (Nacalai Tesque, Japan).Column chromatography was performed on silica gel, Sephadex LH-20, and ODS.Analytical-grade solvents, purchased from Sinopharm Chemical Reagent Co., Ltd. or Xilong Scientific Co., Ltd., were used for solvent extractions Chromatography solvents were HPLC grade, supplied by Xilong Scientific Co., Ltd. or Sigma-Aldrich.Deuterated solvents were purchased from Cambridge Isotopes.

Fungal Identification, Fermentation, and Extraction
The fungus strain 170217 was isolated from the intestinal contents of a whale Mesoplodon densirostris stranded in Ningde of the East China Sea.It was identified to be an Aspergillus versicolor (GenBank accession number SUB13826338), as the 18S rRNA gene sequence alignment demonstrated that it was 100% identical to the Aspergillus versicolor TF34 (GenBank accession number MN515366.1).For scale-up fermentation, the A. versicolor 170217 was grown under static conditions at 25 • C in 85 × 1 L Erlenmeyer flasks, each containing 200 g oatmeal agar, including 100 g of oatmeal, 15% sea salt, and 120 mL of distilled H 2 O.After 30 days, the fermentation product was extracted, in triplicate, using 95% ethanol.Then, the organic solvent was combined and concentrated to a small volume.The latter was then extracted, in triplicate, using ethyl acetate.Finally, the solvent was removed under vacuum to provide the crude extract (153 g).

Theoretical Calculations
Conformational analysis was first performed via random searching in the stochastic algorithm using the MMFF94 force field, with an energy cutoff of 7.0 kcal/mol and an RMSD threshold of 0.5 Å.The predominant conformers were relocated and confirmed at the B3LYP/6-31G(d) level.The theoretical ECD spectra were calculated using the timedependent density functional theory (TD-DFT) in methanol.The ECD spectrum was obtained by averaging each conformer using the Boltzmann distribution theory.NMR calculation and conformational optimization were performed under the HF/6-31G(d) level; then NMR was calculated at the mPW1PW91/6-311G (2d, p) level.For ORD calculation, the conformations of the compounds were optimized at the B3LYP/6-31G(d) level to obtain the energy-minimized conformers.Then, the optimized conformers were subjected to the calculations of specific rotation value using the B3LYPspAug-cc-pVDZ level (λ = 589.3nm).The calculated specific rotations were later obtained according to the Boltzmann weighting of each conformer.

Anti-Food Allergic Bioassay
The in vitro anti-food allergic assay was conducted following our previous protocol [51,52].Briefly, the rat basophilic leukemia 2H3 (RBL-2H3) cells were incubated with dinitrophenyl (DNP)-immunoglobulin E (IgE) overnight.Then, the IgE-sensitized RBL-2H3 cells were pretreated with the tested compounds and stimulated with DNP-bovine serum albumin (BSA).The bioactivity was quantified by measuring the fluorescence intensity of the hydrolyzed substrate in a fluorometer.Loratadine, a commercially available anti-allergy medicine, was used as a positive control.

Antibacterial Bioassay
The antibacterial assay (MICs) was evaluated by a broth microdilution in 96-well plates, and two bacterial strains, MRSA and Vibrio parahemolyticus, were used as the test targets, following the methods included in the literature [53].The tested compounds were prepared in 20% DMSO to obtain the mother solution with the initial concentration of 20 mM, and then were diluted 40-fold with PBS.The compound solution was subsequently diluted using the 2× dilution method in series to reach eight concentrations from 512 µM to 4 µM.The bacteria are diluted into 5 × 10 5 CFU/mL and added into the 96-well plates, and equal volumes of the compound solutions were added into each well.After culturing for 24 h at 37 • C, the plates were observed by the naked eye.Each experiment was repeated three times.An equal amount of DMSO was used as a negative control.

Conclusions
In the present study, the chemical investigation of the deep-sea-derived fungus A. versicolor 170217 led to the isolation of six new (1-6) and 45 known (7-51) compounds, enriching the diversity of secondary metabolites from the deep-sea-derived Aspergillus.The structures, including absolute configurations of new compounds, were elucidated by the analysis of comprehensive spectroscopic data, quantum chemical calculations, and biogenetic considerations.Biologically, compounds 32 and 17 showed remarkable anti-food allergic activity, with IC 50 values of 7.9 ± 3.0 µM and 13.4 ± 1.2 µM, respectively, while displaying no

Figure 4 .
Figure 4.The calculated and the experimental ECD spectra of compound 1.Compound 2 was isolated as a yellow amorphous solid and assigned the molecular formula C 24 H 29 NO 6 on the basis of the [M − H] − ionic peak at m/z 426.1996 in its negative HRESIMS spectrum, suggestive of a homologue of 1.Comparison of NMR data of 2

Figure 4 .
Figure 4.The calculated and the experimental ECD spectra of compound 1.Compound 2 was isolated as a yellow amorphous solid and assigned the molecular formula C24H29NO6 on the basis of the [M − H] − ionic peak at m/z 426.1996 in its negative HRESIMS spectrum, suggestive of a homologue of 1.Comparison of NMR data of 2 (Figures S8-S13, Table1) and 1 revealed a high degree of similarity, including resonances accounting for the isoquinocitrinin substructure, namely fragment B of 1.The primary differences were attributed to the presence of an aromatic proton (δH 6.30, s; H-9), as well as the shielding of C-2 (ΔδC -5.5).HMBC correlations from H-1″ to C-6/7/8, H-9 to C-5/C-7, together with signals observed from H3-11 to C-4 and COSY correlations of H3-10/H-2/H-3/-H3-11, inferred the penta-substituted benzene fragment A. Considering the molecular formula, the planar structure of 2 was assigned as shown in Figure5.

Figure 4 .
Figure 4.The calculated and the experimental ECD spectra of compound 1.Compound 2 was isolated as a yellow amorphous solid and assigned the molecular formula C24H29NO6 on the basis of the [M − H] − ionic peak at m/z 426.1996 in its negative HRESIMS spectrum, suggestive of a homologue of 1.Comparison of NMR data of 2 (Figures S8-S13, Table1) and 1 revealed a high degree of similarity, including resonances accounting for the isoquinocitrinin substructure, namely fragment B of 1.The primary differences were attributed to the presence of an aromatic proton (δH 6.30, s; H-9), as well as the shielding of C-2 (ΔδC -5.5).HMBC correlations from H-1″ to C-6/7/8, H-9 to C-5/C-7, together with signals observed from H3-11 to C-4 and COSY correlations of H3-10/H-2/H-3/-H3-11, inferred the penta-substituted benzene fragment A. Considering the molecular formula, the planar structure of 2 was assigned as shown in Figure5.

Figure 4 .
Figure 4.The calculated and the experimental ECD spectra of compound 1.Compound 2 was isolated as a yellow amorphous solid and assigned the molecular formula C24H29NO6 on the basis of the [M − H] − ionic peak at m/z 426.1996 in its negative HRESIMS spectrum, suggestive of a homologue of 1.Comparison of NMR data of 2 (Figures S8-S13, Table1) and 1 revealed a high degree of similarity, including resonances accounting for the isoquinocitrinin substructure, namely fragment B of 1.The primary differences were attributed to the presence of an aromatic proton (δH 6.30, s; H-9), as well as the shielding of C-2 (ΔδC -5.5).HMBC correlations from H-1″ to C-6/7/8, H-9 to C-5/C-7, together with signals observed from H3-11 to C-4 and COSY correlations of H3-10/H-2/H-3/-H3-11, inferred the penta-substituted benzene fragment A. Considering the molecular formula, the planar structure of 2 was assigned as shown in Figure5.

Figure 8 .
Figure 8.The calculated and the experimental ECD spectra of compounds 3 and 4.
Recorded in CD 3 OD.
a Recorded in CD 3 OD; b Recorded in CDCl 3. Mar.Drugs 2023, 21, x FOR PEER REVIEW 9 of 15

Table 4 .
The calculated and experimental specific rotation values of compound 6.

Table 4 .
The calculated and experimental specific rotation values of compound 6.

Table 4 .
The calculated and experimental specific rotation values of compound 6.

Table 4 .
The calculated and experimental specific rotation values of compound 6.

Table 4 .
The calculated and experimental specific rotation values of compound 6.