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Synthesis, SAR, and Docking Studies Disclose 2-Arylfuran-1,4-naphthoquinones as In Vitro Antiplasmodial Hits.

1. Introduction

Malaria, a tropical disease caused by protozoa Plasmodium spp., is still a serious public health problem, affecting mostly Africa (88%) [1]. P. falciparum is the main agent responsible for mortality and morbidity in endemic tropical regions. Drug-resistance to available agents, including artemisinin (1, Figure 1), is a serious limitation to chemotherapeutics [2], the main strategy for combating malaria. Aiming to control selection of artemisinin resistant parasites, ACT (Artemisinin-Based Combination Therapy) was developed and is the first-line treatment recommended by WHO [3].

Lapachol (2, Figure 1), a prenylnaphthoquinone occurring in Central and South American species of Handroanthus spp. (synon. Tabebuia, Bignoniaceae family) [4] and first isolated from Tabebuia avellanedae, in 1882 by Paterno [5], was used as an antiplasmodial drug during World War II, when there was a shortage of quinine, the only available antimalarial agent at that time [6]. Since the pioneering work of Wendel (1946), who demonstrated that lapachol (2, Figure 1) was active against P. vivax [7], numerous publications reported on the antiplasmodial activity of naphthoquinones leading to the development of atovaquone (3, Figure 1), a totally synthetic hydroxy-1,4-naphthoquinone [4]. Atovaquone, in combination with proguanil (4, Figure 1) (Malarone[R]), is a recommended regimen for prophylaxis in areas of chloroquine resistance and for treatment of uncomplicated falciparum malaria [8].

Previous studies demonstrated that atovaquone (3, Figure 1) is a potent and specific inhibitor of the mitochondrial electron transport at the level of cytochrome bc1 complex (Pfcyt bcl) [9-12]. This inhibition results in the collapse of the mitochondrial membrane potential that causes shutdown of mitochondrial metabolism and blockage of the dihydroorotate dehydrogenase (Pf DHOD) enzyme, which participates in the fourth step of the de novo pyrimidine biosynthesis, which is essential to parasite nucleic acids synthesis, resulting in parasite death [12, 13].

Atovaquone has a broad spectrum of activity against various apicomplexan parasites and mutations in the Pfcyt bcl gene were shown to be associated with resistance to atovaquone in various organisms, such as TM90C2B P. falciparum strain, Toxoplasma, and Pneumocystis jirovecii [12-15]. Therefore, atovaquone resistant P. falciparum strains represent limitations to its clinical use in malaria endemic areas and are a motivation for the synthesis of atovaquone analogs [16, 17].

In addition to lapachol (2, Figure 1), different structural types of naphthoquinones, such as pyran and furanonaphthoquinones, are found in Bignoniaceae [18, 19] and disclose abroad spectrum of biological activities, including antitumor [20-23], trypanocidal [24], anti-inflammatory [7], antifungal [25], and antiparasitic activities [26-33]. Prior studies have reported that furanonaphthoquinones (FNQs) containing alkyl groups linked to the furan ring have proven to be efficient in in vitro antiplasmodial evaluations [27, 28, 34]. Furthermore, it has been demonstrated that the incorporation of a basic amino group into naphthoquinones led to new chemical entities with increased in vitro antiplasmodial activity, including lapachol derivatives [35-37].

The present paper reports the results of an work aiming to investigate the in vitro antiplasmodial activity against the resistant strain of P. falciparum W2 and the cytotoxicity to Hep G2A16 cell cultures of naphthoquinones with different scaffolds, including ortho- and para-derivatives represented by ortho-FNQs (7) para-FNQs (8) supporting alkyl and aryl groups at the furan ring that were synthesized from HNQs (6) obtained from lawsone (5), as shown in the retrosynthetic scheme (Figure 2). Nine aryl derivatives (6, 7, 8f-h) were designed as atovaquone analogs. Another group of naphthoquinones, the aminopropoxynaphthoquinones (ANQs) 12a-c, derived from 5 (Figure 2), was synthesized aiming to evaluate the influence of the amino group in the antiplasmodial activity of simple naphthoquinones.

The proposed synthetic work was carried out leading to 28 naphthoquinones of four different scaffolds that were assayed for in vitro antiplasmodial activity against chloroquineresistant P. falciparum (W2) and for cytotoxicity to Hep G2A16 cells. Molecular docking simulations for interaction of the synthesized compounds were performed aiming to evaluate the correlation of binding energies with structure activity relationship (SAR) data. Besides P. falciparum cytochrome bc1 complex (Pfcyt bc1) that has been proven to be the target for atovaquone [9, 11, 12], docking simulations were also performed against P. falciparum dihydroorotate dehydrogenase enzyme (PfDHOD) that is considered an attractive antimalarial chemotherapeutic target [16].

2. Materials and Methods

Melting points were determined using a MQAPF-307 melting point apparatus (Microquimica, Brazil) and remained uncorrected. The progress of the reactions was monitored by thin layer chromatography (TLC) in silica gel plates. Column chromatography was performed over silica gel (60-230 mesh). Infrared spectra were recorded on a Spectra One Perkin-Elmer spectrophotometer, fitted with a Paragon ATR accessory. Mass spectra (HRMS) were recorded on a Shimadzu GC MS-QP5050A instrument using direct insertion together with the electrospray ionization method and a quadrupole analyzer. The [sup.1]H, [sup.13]C, and DEPT 135 nuclear magnetic resonance (NMR) spectra and two dimensional NMR spectra--correlations spectroscopy (COSY), heteronuclear single-quantum correlation (HSQC), and heteronuclear multiple bound correlation (HMBC)--were recorded on a Bruker Avance DPX 200 and a DPX 400 spectrometer at 200 and 400 MHz using CD[Cl.sub.3] and DMSO[d.sub.6] as the solvent and Tetramethylsylane (TMS) as the internal standard, unless otherwise stated. The NMR data are presented as follows: chemical shift in ppm, multiplicity, number of protons, / in Hz, and proton assignments. Multiplicities are indicated by the following abbreviations: s (singlet), d (doublet), dd (double doublet), t (triplet), q (quartet), m (multiplet), qn (quintet), st (sextet), ht (heptet), and bs (broad singlet).

2.1. General Procedures of Synthesis

2.1.1. 2-Hydroxy-3-(1'-alkenyl)-1,4-naphthoquinones: HNQs (6a-h). The appropriated aldehyde (86mmol) was added to a solution of lawsone (17 mmol) in glacial acetic acid (20 mL), followed by concentrated HCL (15 mL). The reaction mixture was kept under magnetic stirring and reflux for 40 min, at which time the TLC showed the consumption of lawsone. Subsequently, water was added to the reaction mixture (50 mL), followed by extraction with dichloromethane. The organic layer was extracted with aqueous sodium carbonate (2.5%), and the water layers were combined, neutralized with HCl 2N, and extracted with dichloromethane. The organic layer was dried with anhydrous [Na.sub.2]S[O.sub.4] and then filtered. The solvent was removed under lower pressure, and the residue was fractionated in a silica gel column chromatography. Fractions eluted with a mixture of hexane/dichloromethane (7:3) afforded 2-hydroxy-3-(1'-alkenyl)-1,4- naphthoquinones (6a-h, Scheme 1).

2.1.2. Furanonaphthoquinones: FNQs (7a-h and 8a-h). Hg[(OAc).sub.2] (4 mmol) in glacial acetic acid (15 mL) was added to a solution of HNQ (2 mmol) in glacial acetic acid (15 mL). The reaction mixture was kept under magnetic stirring at room temperature for 30 min and at 80[degrees]C for 15 min. Subsequently, diethyl ether was added to the reaction mixture. The solid was separated by filtration, and the solution solvent was removed, resulting in a crude product. To obtain the ortho-FNQs 7a-h, the crude product was dissolved in ethanol (20 mL), and HCl 2N (20 mL) was added. The mixture was kept under magnetic stirring and reflux for 15 min. Subsequently, water (30 mL) was added to the reaction mixture, followed by extraction with ethyl acetate. The organic layer was extracted with aqueous sodium bicarbonate, rinsed with water, and dried with anhydrous [Na.sub.2]S[O.sub.4]. The solvent was removed, and the residue was chromatographed through a silica gel column. Elution with a mixture of hexane/dichloromethane (8: 2) led to the ortho- furanonaphthoquinones (7a-h, Scheme 1). To obtain the para-FNQs 8a-h, the crude product was dissolved in ethanol (20 mL), and concentrated HCl (20 mL) was added in this solution. The mixture was kept under magnetic stirring and reflux for 3h. Water (30 mL) was then added to the reaction mixture, followed by extraction with ethyl acetate. The organic layer was extracted using an aqueous sodium bicarbonate, rinsed with water, and dried with anhydrous [Na.sub.2]S[O.sub.4]. The solvent was removed, and the residue was fractionated in a silica gel column chromatography. Elution with a mixture of hexane/dichloromethane (9:1) led to the para-FNQs 8a-h (Scheme 1).,4-dione (9). Lawsone (6 mmol) was added to a round bottom flask containing sodium hydride (11 mmol) and dimethylformamide (5mL). The reaction mixture was kept under stirring at room temperature for 30 min, after which time epichlorohydrin (30 mmol) was added to the mixture, which was kept under stirring and reflux for 3 h, when TLC showed the consumption of lawsone. Ethyl acetate (50 mL) was added to the reaction mixture, followed by the extraction with a solution of NaCl. The organic layer was dried with anhydrous [Na.sub.2]S[O.sub.4]. The solvent was removed, and the residue was purified by silica gel column chromatography. The product was eluted with a mixture of hexane/ethyl acetate (9: 1), leading to compound 9 (Scheme 2).

2.1.4. Aminopropoxynaphthoquinones: ANQS (10a-c). An appropriatedamine(0.2 mol)wasaddedtoaroundbottomflask containing compound 9 (4 mmol) and MeOH. The reaction solution was kept under stirring and reflux for 3 h, when TLC showed the consumption of starting materials. Ethyl acetate (20 mL) was then added to the mixture, followed by extraction with HCl 2N. The water layer was neutralized with NaOH 2N and extracted with ethyl acetate. The organic layer was dried with anhydrous [Na.sub.2]S[O.sub.4]. The solvent was removed and the residue was chromatographed through a silica gel column chromatography. The product was eluted with a mixture of hexane/ethyl acetate (9.5:0.5), leading to the ANQs 10a-c (Scheme 2).

2.2. Biological Assays

2.2.1. In Vitro Antiplasmodial Activity. There are several in vitro methods commonly used for the assessment of parasite growth inhibition [38]. The parasite protein lactate dehydrogenase (pLDH) method [39, 40] was chosen to evaluate the in vitro antiplasmodial activity of HNQs 6a-h, ortho-FNQs 7a-h, 8a-h, 9, and ANQs 10a-c.

P. falciparum (W2 strain) was maintained in a continuous culture, as described by Trager and Jensen (1976) [41]. Ring-stage parasites in sorbitol-synchronized blood cultures were added to 96-well culture plates, at 2% parasitemia and 1% hematocrit. Stock solutions at 50 mg x [mL.sup.-1] of each compound in DMSO were diluted in a complete medium, in serial concentrations of 2: 1 to final concentrations of 0.002% (v/v), and 20 [micro]l of each one was added to the 96-well culture plates containing the parasite culture. After 48 h incubation, the plates were frozen (-20[degrees]C for 24 h) and thawed before starting the pLDH assay [40].

The hemolyzed cultures were transferred to another 96-well culture plate to which Malstat[R] and NBT/PES reagents were added. After 1h of incubation at 37[degrees]C in the dark, absorbance was read at 540 nm in a spectrophotometer (Infinite[R]200 PRO, Tecan). The experiment was performed three times, each one in triplicate. The results were evaluated by the Microcal Origin 8.5 software to determine the doseresponse curves plotted with sigmoidal fit. The [IC.sub.50] was determined by comparison with controls for standard drug and without drugs.

2.2.2. Cytotoxicity to Hep G2A16 Cells. Cytotoxicity determination was carried out in human hepatoma cell culture (Hep G2A16), which was kept at 37[degrees]C in RPMI medium supplemented with 5% fetal calf serum (complete medium) in a 5% C[O.sub.2] environment. Cells from confluent monolayers were trypsinized, washed, counted, diluted in complete medium, distributed in 96-well microtiter plates (4 x [10.sup.5] cells/well), and then incubated for 18 h at 37[degrees]C. The compounds to be tested were diluted in DMSO (final concentration of 0.02%). After 24 h incubation at 37[degrees]C, 28 [micro]L of MTT solution (2 mg x [mL.sup.-1] in PBS) was added to each well. After 1.5 h of incubation at 37[degrees]C, the supernatant was removed and 130 [micro]L of DMSO was added to each well [40, 42]. The experiment was performed three times, each one in triplicate. The culture plates were read by a spectrophotometer with a 510 nm [42]. The selective indexes (SI = C[C.sub.50]/[IC.sub.50]) of compounds 6a-h, 7a-h, and 8a-h were calculated.

2.3. Computational Methods: Molecular Docking. Initially, the molecular targets were obtained from a Protein Data Bank (PDB) [43] under codes 4PD4 (P. falciparum cytochrome bc1 complex) [8] and 5FI8 (P. falciparum dihydroorotate dehydrogenase) [44]. Next, the molecular target structures were represented according to the Swiss Model software [45] for building the missing loops, and the resulting structures were submitted to H++3.0 [46], a program that automates the key steps in the preparation of biomolecular structures for molecular modeling and simulations, as well as by the MGLTools software [47] to assign the protonate state of histidines. In addition, a grid box was generated with dimensions of 20, 20, and 20 [Angstrom] for both molecular targets. The coordinates of the grid box were centered on crystallographic ligands, 198.619, -25.603, and 81.313 [Angstrom] for %, y, and z, respectively, for 4PD4, and -38.861, 102.656, and -15.221, for 5FI8, using the MGLTools software [47]. Subsequently, the HNQs and the FNQs structures were generated by the MarvinSketch program [48]. The protonation states and the tautomers, when possible, were adjusted according to pH 7.4 [49]. Next, all compound structures were refined by the Octopus software [50]. Octopus is an automated workflow management tool that integrates MOPAC2016, MGLTools, PyMOL, and AutoDock Vina to perform molecular docking through a user-friendly interface [45, 51-55]. HNQs and FNQs were refined by the parametric method 7 (PM7) [56] and the Eigenvector Following (EF) [56] routine implemented in MOPAC2016 [52] by the Octopus Run_mopac routine, which automatically assigns the total molecular charge for each ligand and checks for errors in the structures. The AutoDock Vina methodology was evaluated by redocking, and its exhaustiveness parameter was set to 24 to achieve more accurate results [57]. The figures were generated by academic versions of the Discovery Studio 4.5 program [58].

3. Results and Discussion

3.1. Chemistry

3.1.1. Synthesis. Three series of naphthoquinones--HNQs, ortho- and para-FNQs--were synthesized, affording 24 compounds, 20 of which had been previously described [20, 29, 34], while the other 4 compounds (6h, 7g, 7h, and 8h) represent new chemical entities (Scheme 1).

The HNQs (6a-h) were synthesized by aldol condensation between commercial lawsone (5) (Sigma-Aldrich) and appropriate aldehydes, according to a methodology adapted from Hooker [59] with yields ranging from 32% to 91% (Scheme 1). The FNQs 7a-h and 8a-h were prepared by oxidative cyclization of the corresponding HNQs with Hg[(OAc).sub.2] [20, 34, 60], as outlined in Scheme 1. When the reaction mixtures were diluted with HCl 2N for 15 min, ortho-FNQs (kinetic products) were the major products, while when concentrated HCl (12N) was used with 3 h of reaction, para-FNQs (thermodynamic products) were obtained [60]. The ortho- and para-FNQs were obtained with yields ranging from 20% to 92% (Scheme 1). In presence of concentrated sulfuric acid, ortho-FNQs can be converted into para-FNQs, a process called isomerization, previously described by Hooker in 1986 [59]; however, this method was not used in the present work.

Some of the HNQs, ortho- and para-FNQs described in this work, had also been synthesized by our research group in prior studies, but these were only evaluated against Toxoplasma gondii [30-32].

A fourth series of naphthoquinones, the ANQs (10a-c), was prepared from lawsone (5) by etherification with epichlorohydrin to produce compound 9 (58% yield), followed by a nucleophilic opening of the epoxide ring with appropriated amines affording 10a-c with low yields (20% to 30%), Scheme 2. All compounds of this series represent new chemical entities.

3.1.2. Spectroscopic Characterization of Compounds. All the synthesized compounds were chemically characterized by their spectra in the IR (infrared), [sup.1]H NMR, and [sup.13]C NMR and some of them by HRMS and two dimensional NMR spectra. Spectra for the new chemical entities are shown in the Supplementary Data in Supplementary Material available online at

3.2. Biological Evaluation. Initially, the percentage of parasite growth inhibition was determined for each compound in two different concentrations (50 and 25 [micro]g x [mL.sup.-1]), in triplicate, and the results are shown in Table 1. Compounds showing a parasitemia reduction greater than 50% at 25 [micro]g x [mL.sup.-1] were classified as active.

All of the HNQs (6a-h), ortho-FNQs (7a-h), and para-FNQs (8a-h) were classified as in vitro antiplasmodial active compounds (parasitemia reduction > 50% at 25 [micro]g x [mL.sup.-1]), and their [IC.sub.50] values were experimentally determined by the pLDH methodology (Table 2) [40, 42]. Lawsone glycidyl ether (9) and ANQs (10a-c) were inactive, with parasitemia reduction ranging from 9% to 34% at 25 [micro]g x [mL.sup.-1] (Table 1); therefore, their [IC.sub.50] and C[C.sub.50] were not determined. It is important to highlight that the in vitro assays were performed in 48 h, because that is the duration of the asexual erythrocytic stage of P. falciparum, and it is within the time range recommended by Makler and collaborators (1998) [39] whose methodology was followed in the present in vitro antiplasmodial evaluations.

All of the naphthoquinones of the first three series, namely, HNQs (6a-h), ortho-FNQs (7a-h), and paraFNQs (8a-h), were more active than lapachol ([IC.sub.50] 206.38 [micro]mol x [L.sup.-1]) (Table 2). The HNQs series (6a-h) was the least effective, with only 6f and 6h disclosing moderate activity ([IC.sub.50] < 50 [micro]mol x [L.sup.-1]) (Table 2). In general, ortho-FNQs (7a-h) and para-FNQs (8a-h) showed higher activity (lower [IC.sub.50]) than HNQs. In total, twelve FNQs showed [IC.sub.50] < 30 [micro]mol x [L.sup.-1]: six ortho-FNQs (7a, 7b, 7c, 7e, 7f, and 7h) and six para-FNQs (8a, 8b, 8c, 8d, 8f, and 8g), highlighting 8c ([IC.sub.50] 11.65 [micro]mol x [L.sup.-1]), 8f ([IC.sub.50] 18.78 [micro]mol x [L.sup.-1]), and 7h ([IC.sub.50] 19.91 [micro]mol x [L.sup.-1]), which were the most active. Another interesting aspect to be noted is related to compound pairs with a phenyl and a chlorophenyl substituent in each of these three structural series. The presence of a chlorine atom was planned by analogy with atovaquone, and a surprising result was observed. For the HNQs 6g and 6h and the ortho-FNQs 7g and 7h, the chlorinated derivatives were about three times more active in HNQs and two times more active in ortho-FNQs, while for the para-FNQs series, 8g and 8h, an inverse effect was observed, which could, possibly, be related to the low solubility of these compounds in the conditions of the biological assays.

To investigate the selectivity of the active compounds, C[C.sub.50] against Hep G2A16 cells was determined, and the SI values (SI = C[C.sub.50] / [IC.sub.50]) were calculated (Table 2).

Six of the 13 less cytotoxic compounds (C[C.sub.50] > 90 [micro]mol x [L.sup.-1]) are HNQs (6a, 6b, 6c, 6e, 6g, and 6h), while seven are para-FNQs (8a, 8c, 8d, 8e, 8f, 8g, and 8h). As expected, ortho-FNQs were more cytotoxic because they can be easier reduced and, therefore, more reactive oxygen species (ROS) are generated, increasing thus cell damage [61].

Nine compounds showed SI > 5: four HNQs (6a, 6e, 6g, and 6h) and five para-FNQs (8a, 8c, 8d, 8f, and 8g). Compounds 8c and 8f are highlighted here because they exhibit the best [IC.sub.50] values (8c 11.65 [micro]mol x [L.sup.- 1]; 8f 18.78 [micro]mol x [L.sup.-1]), presented low cytotoxicity (8c 115.90 [micro]mol x [L.sup.-1]; 8f 97.89 [micro]mol x [L.sup.-1]), and showed SI > 5 (8c 9.94 and 8f 5.21). Despite disclosing a moderate activity, compound 8a ([IC.sub.50] 26.57 [micro]mol x [L.sup.-1]) showed low cytotoxicity (C[C.sub.50] 869.10 [micro]mol x [L.sup.-1]), resulting in the highest SI value (32.71), and might be highlighted as a lead compound, when its SI is considered; that is, 8a can be selected for in vivo antimalarial efficacy evaluation and early safety and toxicity studies. Finally, compounds 6h, 8a, 8c, 8d, 8f, and 8g showing moderate antiplasmodial activity ([IC.sub.50] < 40 [micro]mol x [L.sup.-1]) against the chloroquine-resistant P. falciparum W2 strain, low cytotoxicity (C[C.sub.50] > 90 [micro]mol x [L.sup.-1]), and SI > 5 are thus selective to resistant parasite and deserve also further investigations.

The in vitro antiplasmodial activity of some naphthoquinones described in this work was previously described [27, 28] as causing completely growth inhibition of an unidentified strain of P. falciparum. Recently, Duran-Lengua et al. (2015) [34] reported enhanced effects of 6, 7, 8-a, 6, 7, 8-b, and 6, 7, 8-d against sensitive and moderately resistant strains of P. falciparum, 3D7, and Dd2, respectively. With respect to the [IC.sub.50] values, it should be taken into account that, in the present case, the higher [IC.sub.50] values might be explained by the fact that the in vitro assays were performed upon P. falciparum W2, a chloroquine-resistant strain, which represents a challenge to the discovery of new antiplasmodial drugs.

3.3. Computational Methods: Molecular Docking. Intermolecular interactions between HNQs and FNQs against the molecular targets 4PD4 (Pfcyt bc1) and 5FI8 (PfDHOD) were simulated by the AutoDock Vina software [8, 37]. The methodology was evaluated by redocking, which consists of the docking of crystallographic structures onto the targets binding sites. This simulation can show if the docking parameters and the methodology are adequately adjusted to the system. As a result, the root mean square deviation (RMSD) of atovaquone (2) and DSM422 (Figure 3) redocking were 0.75 [Angstrom] and 0.86 [Angstrom], respectively. These results were below the threshold value of 2.0 [Angstrom] [52] and binding energies of -11.3 Kcal x [mol.sup.-1] to atovaquone with 4PD4 and -12.1 Kcal x [mol.sup.-1] to DSM422 with 5FI8 (Figure 3). These data suggest that the AutoDock Vina methodology is appropriate for simulating the intermolecular interaction and predicting the binding energy of HNQs and FNQs to targets (4PD4 and 5FI8).

Binding energies of docking simulations ranged from -8.2 Kcal x [mol.sup.-1] to -10.6 Kcal x [mol.sup.-1] for 4PD4 and from -8.2 Kcal x [mol.sup.-1] to -11.5 Kcal x [mol.sup.-1] for 5FI8 (Table 2). These values are relevant in the interpretation of docking results for the HNQs and FNQs, as active compounds are expected to disclose binding energies close to the models (atovaquone and DMS422) and should promote good activities.

Molecular docking simulations disclosed favorable binding energies (BE [less than or equal to] -10 Kcal x [mol.sup.-1]) for interactions of twelve compounds with the targets 4PD4 (6g, 6h, 7g, 7h, 8g, 8h) and 5FI8 (6f, 6g, 7f, 8f, 8g, 8h) which are coherent with SI > 5 for 6g, 6h, 8f, and 8g, highlighting FNQs.

For HNQ 6d, one of the less active compounds (SI 0.24), a weak correlation with the binding energies (4PD4 -8.5 and 5FI8 -9.0 Kcal x [mol.sup.-1]) for both of the targets (Table 2), was observed. On the other hand, for the HNQ 6h (SI = 8.49), the binding energy is -10.6 Kcal x [mol.sup.-1] for 4PD4, while the value of BE forpara-FNQ 8f (SI = 5.21) is -11.5 Kcal x [mol.sup.-1] for 5FI8 (Table 2); these are the most active compounds of these series and their complexed structures into the hydrophobic cavities of the targets, as shown in Figure 4.

Figure 5(a) shows that HNQ 6h represents van der Waals intermolecular interactions with 4PD4 through amino acids Met139, Gly143, Val146, Trp142, Ile269, Pro271, Leu275, and Phe278. Similarly, for compound 8f, van der Waals interactions are depicted with Leu34, Cys37, Leu38, Leu59, Cys46, Phe89, Ile99, Leu363, and Leu364 amino acids of 5FI8 (Figure 5(b)). In addition, the molecular recognition for compound 8f is improved by two weak noncovalent intermolecular interactions: His47 and the furan oxygen with a distance of 2.69 [Angstrom] and a [pi]-sulfur interaction between Cys95 and the benzenoid ring in the naphthoquinone moiety with a distance of 2.47 [Angstrom]. These intermolecular interactions might certainly contribute for the biological activity of compounds 6h and 8f.

Previous studies have shown the inhibition of Pf cyt bc1 and PfDHOD by naphthoquinones [8, 10, 11], and the molecular docking results described here are in accordance with this mode of action, although further enzymatic assays are necessary for confirmation.

4. Conclusions

The present study reported on the synthesis of 28 compounds belonging to four structural series--HNQs, ortho-FNQs, para-FNQs, and ANQs--eight of which represented new chemical entities. All of the HNQs (6a-h) and FNQs (7a-h and 8a-h) were classified as active compounds with in vitro parasitemia reduction ranging from 45% to 90% at 25 [micro]g x [mL.sup.-1] and proved to be more potent than lapachol ([IC.sub.50] 206.38 [micro]mol x [L.sup.-1]) against the chloroquine-resistant P. falciparum W2 strain. The insertion of a furan ring in the naphthoquinone moiety increased the biological activity, and the FNQs were, in general, more active than the HNQs. As expected, ortho-FNQs (7a-h) were more cytotoxic to Hep G2A16 cells and less selective to the parasite (SI < 5). The ortho-FNQs might be highlighted for their potential antitumoral rather than antiplasmodial effect. On the other hand, ANQs, although containing an amino group in their structures, disclosed low biological activity and were classified as inactive compounds (parasitemia reduction < 50% at 25 [micro]g x [mL.sup.-1]). Considering the experimental values of IC50 < 40 [micro]g x [mL.sup.-1], C[C.sub.50] > 90 [micro]g x [mL.sup.-1], and SI > 5, the para-FNQ 8a is highlighted for its high value of SI (32.71). However, the following naphthoquinones 6h, 8c, 8d, 8f, and 8g deserve also further investigations. Molecular docking simulations disclosed most favorable binding energies (< -10 Kcal x [mol.sup.-1]) for 6h and 8f, disclosing good correlations with the present biological data for naphthoquinones that support aryl moieties. This study points out to arylnaphthoquinones as new potential inhibitors of the Pf cyt bc1 and PfDHOD enzymes since, for both of these targets, favorable binding energies were calculated. However enzymatic assays are necessary for confirming this hypothesis.

Conflicts of Interest

The authors declare no conflicts of interest.


The authors wish to thank FAPEMIG (Fundacao de Amparo a Pesquisa do Estado de Minas Gerais) and CNPq (Conselho Nacional de Desenvolvimento Cientifico e Tecnologico) for their financial support to Alaide Braga de Oliveira through PRONEX Rede Malaria, Protocols nos. APQ-01129-10 and 555655/2009-1, respectively. Fellowships to Alaide Braga de Oliveira, Maria Fernanda Alves do Nascimento, Tatiane Freitas Borgati, and Juma Fortunato Bernardino are fully acknowledged.


[1] World Health Organization, "World Malaria Report," 2015,

[2] J. Y. Wang, W. C. Cao, C. Q. Shan et al., "Naphthoquine phosphate and its combination with artemisinine," Acta Tropica, vol. 89, no. 3, pp. 375-381, 2004.

[3] D. J. Krogstad, B. L. Herwaldt, and P. H. Schlesinger, "Antimalarial agents: specific treatment regimens.," Antimicrobial Agents and Chemotherapy, vol. 32, no. 7, pp. 957-961, 1988.

[4] M. Schlitzer, "Malaria chemotherapeutics part i: history of antimalarial drug development, currently used therapeutics, and drugs in clinical development," ChemMedChem, vol. 2, no. 7, pp. 944-986, 2007.

[5] H. Hussain, K. Krohn, V. U. Ahmad et al., "Lapachol: an overview," Special Issue Reviews and Accounts ARKIVOC, vol. 2, pp. 145-171, 2007.

[6] M. F. C. Cardoso, I. M. C. B. da Silva, H. M. dos Santos Junior et al., "A new approach for the synthesis of 3-substituted cytotoxic nor-[beta]-lapachones," Journal of the Brazilian Chemical Society, vol. 24, no. 1, pp. 12-16, 2013.

[7] D.-O. Moon, Y. H. Choi, N.-D. Kim et al., "Anti-inflammatory effects of [beta]-lapachone in lipopolysaccharide-stimulated BV2 microglia," International Immunopharmacology, vol. 7, no. 4, pp. 506-514, 2007.

[8] D. Birth, W. C. Kao, and C. Hunte, "Structural analysis of atovaquone--inhibited cytochrome bc1 complex reveals the molecular basis of antimalarial drug action," Nature Communications, vol. 4, no. 5, pp. 1-11, 2014.

[9] M. Fry and M. Pudney, "Site of action of the antimalarial hydroxynaphthoquinone, 2-[trans-4-(4'-chlorophenyl) cyclo-hexyl]-3- hydroxy-1,4-naphthoquinone (566C80)," Biochemical Pharmacology, vol. 43, no. 7, pp. 1545-1553, 1992.

[10] A. B. Vaidya, M. S. Lashgari, L. G. Pologe, and J. Morrisey, "Structural features of Plasmodium cytochrome b that may underlie susceptibility to 8-aminoquinolines and hydroxynaphthoquinones," Molecular and Biochemical Parasitology, vol. 58, no. 1, pp. 33-42, 1993.

[11] I. K. Srivastava, H. Rottenberg, and A. B. Vaidya, "Atovaquone, a broad spectrum antiparasitic drug, collapses mitochondrial membrane potential in a malarial parasite," Journal of Biological Chemistry, vol. 272, no. 7, pp. 3961-3966, 1997.

[12] J. E. Siregar, G. Kurisi, T. Kobayashi et al., "Direct evidence for the atovaquone action on the Plasmodium cytochrome bc1 complex," Parasitology Internationalvol, vol. 63, no. 3, pp. 295-300, 2014.

[13] R. Khositnithikul, P. Tan-ariya, and M. Mungthin, "In vitro atovaquone/proguanil susceptibility and characterization of the cytochrome b gene of Plasmodium falciparum from different endemic regions of Thailand," Malaria Journal, vol. 7, no. 23, pp. 1-5, 2008.

[14] N. Fisher, R. A. Majid, T. Antoine et al., "Cytochrome bmutation Y268S conferring atovaquone resistance phenotype in malaria parasite results in reduced parasite bc1 catalytic turnover and protein expression," The Journal of Biological Chemistry, vol. 287, no. 13, pp. 9731-9741, 2012.

[15] M. Korsinczky, N. Chen, B. Kotecka, A. Saul, K. Rieckmann, and Q. Cheng, "Mutations in Plasmodium falciparum cytochrome b that are associated with atovaquone resistance are located at a putative drug-binding site," Antimicrobial Agents and Chemotherapy, vol. 44, no. 8, pp. 2100-2108, 2000.

[16] V. Patel, M. Booker, M. Krame et al., "Identification and characterization of small molecule inhibitors of Plasmodium falciparum dihydroorotate dehydrogenase," The Journal of Biological Chemistry, vol. 283, no. 50, pp. 35078-35085, 2008.

[17] V. Barton, N. Fisher, G. A. Biagini et al., "Inhibiting Plasmodium cytochrome bc1: a complex issue," Current Opinion in Chemical Biology, vol. 14, no. 4, pp. 440-446, 2010.

[18] S. K. Morais, S. G. Silva, C. N. Portela et al., "Bioactive dihydroxyfuranonaphthoquinones from the bark of Tabebuia incana A.H. Gentry (Bignoniaceae) and HPLC analysis of commercial pau d'arco and certified T.incana bark infusions," Acta Amazonica, vol. 37, no. 1, pp. 99-102, 2007.

[19] A. M. P. Silva, S. R. Paiva, M. R. Figueiredo, and M. A. C. Kaplan, "Atividade Biologica de Naftoquinonas de Especies de Bignoniaceae," Revista Fitos, vol. 7, no. 4, pp. 207-215, 2012.

[20] J. M. M. del Corral, M. A. Castro, A. B. Oliveira et al., "New cytotoxic furoquinones obtained from terpenyl-1, 4-naphthoquinones and 1, 4-anthracenediones," Bioorganic & Medicinal Chemistry, vol. 14, no. 21, pp. 7231-7240, 2006.

[21] J. M. M. del Corral, M. A. Castro, M. Gordaliza et al., "Synthesis and Biological Evaluation of Cytotoxic 6(7)-Alkyl-2-hydroxy-1, 4-naphthoqmnones," Archiv der Pharmazie, vol. 335, no. 9, pp. 427-437, 2002.

[22] H. Rutner, "Analogues of lapachol as antitumor agents," U.S. Patent 3,655,699, 1972.

[23] J. E. Carvalho, C. A. Camara, M. D. Vargas et al., "Naftoquinonas naturais e semi-sintoeticas parcialmente hidrogenadas derivadas do lapachol com atividade citotoxica e antitumoral," Br. Patent PI 0502766-7, 2005.

[24] E. N. da Silva Junior, T. T. Guimaraes, R. F. Menna-Barreto, and eyal, "The evaluation of quinonoid compounds against Trypanosoma cruzi: Synthesis of imidazolic anthraquinones, nor-[beta]-lapachone derivatives and [beta]-lapachone-based 1,2,3-triazoles," Bioorganic & Medicinal Chemistry, vol. 18, no. 9, pp. 3224-3230, 2010.

[25] S. Gafner, J. Wolfender, M. Nianga et al., "Antifungal and antibacterial naphthoquinones from Newbouldia laevis roots," Phytochemistry, vol. 42, no. 5, pp. 1315-1320, 1996.

[26] N. M. F. Lima, C. S. Correia, L. L. Leon et al., "Antiieishmanial activity of lapachol analogues," Memorias do Instituto Oswaldo Cruz, vol. 99, no. 7, pp. 757-761, 2004.

[27] L. H. Carvalho, Quimioterapia experimental antimalarica com extratos brutos de plantas e compostos quimicamente definidos [Master's Degree in Parasitology], Instituto de Ciencias Bioloogicas, Universidade Federal de Minas Gerais, Minas Gerais, Brazil.

[28] L. H. Carvalho, E. M. Rocha, D. S. Raslan et al., "In vitro activity of natural and synthetic naphthoquinones against erythrocytic stages of Plasmodium falciparum" Brazilian Journal of Medical and Biological Research, vol. 21, no. 3, pp. 485-487, 1988.

[29] S. A. Gualberto, Sintese e atividades antiparasitaria e antitumoral de naftoquinonas [Doctorate in Science], Faculdade de Farmaocia, Universidade Federal de Minas Gerais, 2001.

[30] R. Ferreira, A. Oliveira, S. Gualberto, and R. Vitor, "Activity of natural and synthetic naphthoquinones against Toxoplasma gondii, in vitro and in murine models of infection," Parasite, vol. 9, no. 3, pp. 261-269, 2002.

[31] R. A. Ferreira, A. B. Oliveira, M. F. Ribeiro et al., "Toxoplasma gondii: in vitro and in vivo activities of the hydroxynaphthoquinone 2-hydroxy-3-(1'-propen-3-phenyl)-1,4-naphthoquinone alone or combined with sulfadiazine," Experimental Parasitology, vol. 113, no. 2, pp. 125-129, 2006.

[32] R. A. Ferreira, A. B. de Oliveira, S. A. Gualberto et al., "New naphthoquinones and an alkaloid with in vitro activity against Toxoplasma gondii RH and EGS strains," Experimental Parasitology, vol. 132, no. 4, pp. 450-457, 2012.

[33] E. Perez-Sacau, A. Estavez-Braun, A. G. Ravelo et al., "Antiplasmodial activity of naphthoquinones related to lapachol and [beta]-lapachone," Chemistry & Biodiversity, vol. 2, no. 2, pp. 264-274, 2005.

[34] M. Duran-Lengua, A. N. Kamali, A. J. Cano et al., "Synthetic alkyl substituted quinones oxidize membrane proteins and arrest Plasmodium falciparum growth in vitro," African Journal of Pharmacy and Pharmacology, vol. 9, no. 23, pp. 595-602, 2015.

[35] A. Baramee, A. Coppin, M. Mortuaire et al., "Synthesis and in vitro activities of ferrocenic aminohydroxynaphthoquinones against Toxoplasma gondii and Plasmodium falciparum" Bioorganic Medicinal Chemistry, vol. 14, no. 5, pp. 1294-1302, 2006.

[36] M. T. Leffler and R. J. Hathaway, "Naphthoquinone antimalarials; 2-hydroxy-3-substituted-aminoethyl derivatives by the Mannich reaction," Journal of the American Chemical Society, vol. 70, no. 10, pp. 3222-3223, 1948.

[37] G. J. Kapadia, M. A. Azuine, V. Balasubramanian, and R. Sridhar, "Aminonaphthoquinones--a novel class of compounds with potent antimalarial activity against plasmodium falciparum " Pharmacological Research, vol. 43, no. 4, pp. 363-367, 2001.

[38] F. Nogueira and V. E. Rosario, "Methods for assessment of antimalarial activity in the different phases of the Plasmodium life cycle," Revista Pan-Amazonica de Saude, vol. 1, no. 3, pp. 109-124, 2010.

[39] M. T. Makler, R. C. Piper, and W. K. Milhous, "Lactate dehydrogenase and the diagnosis of malaria," Parasitology Today, vol. 14, no. 9, pp. 376-377, 1998.

[40] T. Borgati, G. Pereira, G. Brandao et al., "Synthesis by click reactions and antiplasmodial activity of lupeol 1,2,3-triazole derivatives," Journal of the Brazilian Chemical Society, vol. 28, no. 10, pp. 1850-1856, 2017.

[41] W. Trager and J. B. Jensen, "Human malaria parasites in continuous culture," Science, vol. 193, no. 4254, pp. 673-675, 1976.

[42] F. P. Varotti, A. C. C. Botelho, A. A. Andrade et al., "Synthesis, antimalarial activity, and intracellular targets of MEFAS, a new hybrid compound derived from mefloquine and artesunate," Antimicrobial Agents and Chemotherapy, vol. 52, no. 11, pp. 3868-3874, 2008.

[43] H. M. Berman, G. J. Kleywegt, H. Nakamura, and J. L. Markley, "The Protein Data Bank archive as an open data resource," Journal of Computer-Aided Molecular Design, vol. 28, no. 10, pp. 1009-1014, 2014.

[44] S. Kokkonda, X. Deng, K. L. White et al., "Tetrahydro-2-naphthyl and 2-Indanyl triazolopyrimidines targeting Plasmodium falciparum dihydroorotate dehydrogenase display potent and selective antimalarial activity," Journal of Medicinal Chemistry, vol. 59, no. 11, pp. 5416-5431, 2016.

[45] L. Bordoli, F. Kiefer, K. Arnold et al., "Protein structure homology modeling using SWISS-MODEL workspace," Nature Protocols, vol. 4, no. 1, pp. 1-13, 2009.

[46] R. Anandakrishnan, B. Aguilar, and A. V. Onufriev, "H++ 3.0: automating pK prediction and the preparation of biomolecular structures for atomistic molecular modeling and simulations," Nucleic Acids Research, vol. 40, no. W1, pp. W537-W541, 2012.

[47] G. M. Morris, H. Ruth, W. Lindstrom et al., "AutoDock4 and AutoDockTools4: automated docking with selective receptor flexibility," Journal of Computational Chemistry, vol. 30, no. 16, pp. 2785-2791, 2009.

[48] ChemAxon, Chemicalize,

[49] E. Glaab, "Building a virtual ligand screening pipeline using free software: a survey," Briefings in Bioinformatics, vol. 17, no. 2, pp. 352-366, 2016.

[50] A. P. Carregal, F. V Maciel, J. B. Carregal et al., "Docking-based virtual screening of Brazilian natural compounds using the OOMT as the pharmacological target database," Journal of Molecular Modeling, vol. 23, no. 111, pp. 1-9, 2017.

[51] O. Trott and A. J. Olson, "AutoDock Vina: improving the speed and accuracy of docking with a new scoring function, efficient optimization and multithreading," Journal of Computational Chemistry, vol. 31, no. 2, pp. 455-461, 2010.

[52] J. J. P. Stewart, MOPAC2016, Stewart Computational Chemistry, Colorado Springs, Colo, USA, 2016,

[53] The PyMOL Molecular Graphics System, Version 1.8 Schrodinger, LLC,

[54] E. Yuriev and P. A. Ramsland, "Latest developments in molecular docking: 2010-2011 in review," Journal of Molecular Recognition, vol. 26, no. 5, pp. 215-239, 2013.

[55] J. J. P. Stewart, "Optimization of parameters for semiempirical methods VI: more modifications to the NDDO approximations and re-optimization of parameters," Journal of Molecular Modeling, vol. 19, no. 1, pp. 1-32, 2013.

[56] J. Baker, "An algorithm for the location of transition states," Journal of Computational Chemistry, vol. 7, no. 4, pp. 385-395, 1986.

[57] S. Forli, M. E. Piche, M. F. Sanner et al., "Computational protein-ligand docking and virtual drug screening with the AutoDock suite," Nature Protocols, vol. 11, no. 5, pp. 905-919, 2016.

[58] Dassault Systemes BIOVIA, Discovery Studio Modeling Environment, Release 2017, Dassault Systemes, San Diego, Calif, USA, 2016.

[59] S. C. Hooker, "The constitution of lapachol and its derivatives. Part III. The structure of the amylene chain," Journal of the Chemical Society, vol. 69, pp. 1355-1381,1896.

[60] K. H. Dudley and H. W. Miller, "Mercuric acetate oxidation of isolapachol," The Journal of Organic Chemistry, vol. 32, no. 7, pp. 2341-2344, 1967.

[61] J. Tonholo, L. R. Freitas, and F. C. Abreu, "Electrochemical properties of piological active heterocyclic naphthoquinones," Journal of the Brazilian Chemical Society, vol. 9, no. 2, pp. 163-169, 1998.

Tatiane Freitas Borgati, (1) Maria Fernanda Alves do Nascimento, (1) Juma Fortunato Bernardino, (1) Lunamaura Claudia Oliveira Martins, (1) Alex Gutterres Taranto, (2) and Alaide Braga de Oliveira (1)

(1) Departamento de Produtos Farmaceuticos, Faculdade de Farmacia, UFMG, Campus Pampulha, Av. Antonio Carlos 6627, 31270-901 Belo Horizonte, MG, Brazil

(2) Faculdade de Farmacia, UFSJ, Campus Divinopolis, Rua Sebastiao Goncalves Coelho 400, Chanadour, 35501-296 Divinopolis, MG, Brazil

Correspondence should be addressed to Alaide Braga de Oliveira;

Received 16 June 2017; Revised 11 August 2017; Accepted 27 August 2017; Published 31 October 2017

Academic Editor: Marcel Tanner

Caption: Figure 1: Chemical structures of artemisinin (1), lapachol (2), atovaquone (3), and proguanil (4).

Caption: Figure 2: Retrosynthetic scheme of HNQs 6a-h, ortho-FNQs 7a-h andpara- FNQs 8a-h, 2-(oxiran-2- ylmethoxy)naphthalene-1,4-dione (9), and ANQs 10a-c, starting from lawsone (5).

Caption: Figure 3: Values of the root mean square deviation (RMSD) of redocking and binding energy (BE) for the interaction of 4PD4 with atovaquone (a) and of 5FI8 with DSM422 (b).

Caption: Figure 4: (a) Compound 6h complexed into the hydrophobic surface of 4PD4. (b) Compound 8f complexed into the hydrophobic surface of 5FI8.

Caption: Figure 5: 2D diagram of intermolecular interaction between 6h and 4PD4 (a) and between 8f and 5FI8 (b).
Table 1: Percentages of Plasmodium falciparum (W2) parasitemia
reduction at 50 [micro]g x [mL.sup.-1] and 25 [micro]g x [mL.sup.-1]
for naphthoquinones 6a-h, 7a-h, 8a-h, 9, and 10a-c.

Compound     % reduction at    % reduction at
             50 [micro]g x     25 [micro]g x
               [mL.sup.-1]       [mL.sup.-1]

6a                 75                53
6b                 73                80
6c                 64                50
6d                 91                81
6e                 71                53
6f                 64                54
6g                 78                73
6h                 83                58
7a                 98                98
7b                 90                81
7c                 94                91
7d                 81                81
7e                 94                88
7f                 81                75
7g                 79                18
7h                 95                89
8a                 83                75
8b                 85                78
8c                 92                86
8d                 71                70
8e                 83                76
8f                 87                85
8g                 80                78
8h                 62                24
9                  61                34
10a                21                 9
10b                22                16
10c                15                12

Table 2: In vitro antiplasmodial activity ([IC.sub.50]) against
Plasmodium falciparum (W2), cytotoxicity (C[C.sub.50], Hep G2A16
cells), selectivity index (SI), and binding energy values of
docking simulations for 4PD4 and 5FI8 with naphthoquinones 6a-h,
7a-h, and 8a-h.

Compound          [IC.sub.50]                C[C.sub.50]
                 ([micro]mol x              ([micro]mol x
                [L.sup.-1]) (b)            [L.sup.-1]) (c)

6a            99.85 [+ or -] 8.46       970.00 [+ or -] 42.60
6b            59.24 [+ or -] 10.27      138.97 [+ or -] 15.14
6c            52.65 [+ or -] 3.71       146.80 [+ or -] 29.10
6d            90.17 [+ or -] 10.43       21.55 [+ or -] 9.44
6e            72.21 [+ or -] 2.98     1,127.00 [+ or -] 39.67
6f            45.76 [+ or -] 2.55        19.51 [+ or -] 4.03
6g           110.34 [+ or -] 6.64       940.30 [+ or -] 40.10
6h            39.55 [+ or -] 8.98       335.90 [+ or -] 26.70
7a            23.22 [+ or -] 5.09         4.68 [+ or -] 0.70
7b            25.10 [+ or -] 2.64        11.91 [+ or -] 4.65
7c            24.70 [+ or -] 2.25        11.53 [+ or -] 2.97
7d            50.22 [+ or -] 2.90        12.99 [+ or -] 2.01
7e            26.41 [+ or -] 3.12        21.33 [+ or -] 3.15
7f            23.44 [+ or -] 6.39        13.68 [+ or -] 4.46
7g            40.72 [+ or -] 7.82         6.10 [+ or -] 0.84
7h            19.91 [+ or -] 4.35        68.68 [+ or -] 14.79
8a            26.57 [+ or -] 3.25       869.10 [+ or -] 32.71
8b            28.86 [+ or -] 3.66        12.51 [+ or -] 2.18
8c            11.65 [+ or -] 2.50       115.90 [+ or -] 21.90
8d            23.77 [+ or -] 2.41       119.20 [+ or -] 23.70
8e            30.55 [+ or -] 3.81       143.27 [+ or -] 12.24
8f            18.78 [+ or -] 0.83        97.89 [+ or -] 13.22
8g            21.80 [+ or -] 2.64       120.84 [+ or -] 6.05
8h           140.70 [+ or -] 7.80     1,048.90 [+ or -] 32.90
2            206.38 [+ or -] 3.64      1567.96 [+ or -] 7.44
(a) CQ        0.280 [+ or -] 0.01       361.84 [+ or -] 10.64

Compound      SI (d)      Binding energy 4PD4     Binding energy 5FI8
                              (e) (Kcal x             (f) (Kcal x
                             [mol.sup.-1])           [mol.sup.-1])

6a             9.72              -8.2                    -8.2
6b             2.34              -8.5                    -8.5
6c             2.79              -8.5                    -8.7
6d             0.24              -8.5                    -9.0
6e             15.61             -8.9                    -9.0
6f             0.43              -9.4                    -10.2
6g             8.52              -10.3                   -10.7
6h             8.49              -10.6                   -9.1
7a             0.20              -8.6                    -9.1
7b             0.47              -8.6                    -9.1
7c             0.47              -8.5                    -9.2
7d             0.26              -8.6                    -9.3
7e             0.80              -9.2                    -9.3
7f             0.58              -9.9                    -10.2
7g             0.15              -10.2                   -9.9
7h             3.45              -10.0                   -9.8
8a             32.71             -8.2                    -8.9
8b             0.43              -8.4                    -9.0
8c             9.94              -8.3                    -9.1
8d             5.01              -8.4                    -9.5
8e             4.69              -8.9                    -9.4
8f             5.21              -9.90                   -11.5
8g             5.54              -10.0                   -11.3
8h             2.40              -10.3                   -10.5
2               7.6               ND                      ND
(a) CQ       1,292.30             ND                      ND

(a) CQ: chloroquine; (b) [IC.sub.50] : concentration ([micro]mol x
[L.sup.-1]) that kills 50% of P. falciparum, determined by the pLDH
method; (c) C[C.sub.50]: concentration that kills 50% of Hep G2A16
cells 24 h after incubation with the compounds, determined by the
MTT method; (d) SI (selectivity index): C[C.sub.50]/[IC.sub.50];
(e) 4PD4: cytochrome bc1 complex subunit 1; (f) 5FI8:
dihydroorotate dehydrogenase; ND: not determined.

Scheme 1: Synthesis of naphthoquinones 6a-h, 7a-h,
and 8a-h and their yields.


Compound        Yield%

6a                37
6b                40
6c                50
6d                32
6e                60
6f                40
6g                45
6h                91


 Compound       Yield%

    7a            54
    7b            41
    7c            73
    7d            92
    7e            66
    7f            77
    7g            30
    7h            20


 Compound       Yield%

    8a            43
    8b            49
    8c            72
    8d            92
    8e            82
    8f            30
    8g            30
    8h            20

Scheme 2: Synthesis of naphthoquinones 9 and 10a-c and their yields.

Compound      Yield%

9               58
10a             20
10b             30
10c             25
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Title Annotation:Research Article
Author:Borgati, Tatiane Freitas; do Nascimento, Maria Fernanda Alves; Bernardino, Juma Fortunato; Martins,
Publication:Journal of Tropical Medicine
Article Type:Report
Geographic Code:3BRAZ
Date:Jan 1, 2017
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