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Antimicrobial Agents and Chemotherapy, May 2004, p. 1534-1540, Vol. 48, No. 5
0066-4804/04/$08.00+0     DOI: 10.1128/AAC.48.5.1534-1540.2004
Copyright © 2004, American Society for Microbiology. All Rights Reserved.

Fungus-Elicited Metabolites from Plants as an Enriched Source for New Leishmanicidal Agents: Antifungal Phenyl-Phenalenone Phytoalexins from the Banana Plant (Musa acuminata) Target Mitochondria of Leishmania donovani Promastigotes

Centro de Investigaciones Biológicas, E-28040 Madrid,¹ Departamento de Parasitología, Facultad de Farmacia, Universidad de La Laguna, E-38206 La Laguna-Tenerife,² Instituto de Bio-Orgánica A.G. González, E-38206 La Laguna-Tenerife, Spain³

Received 31 July 2003/ Returned for modification 25 November 2003/ Accepted 30 January 2004

	ABSTRACT

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Two antifungal phenyl-phenalenone phytoalexins isolated from the banana plant (Musa acuminata) elicited with the fungus Fusarium oxysporum, together with a methoxy derivative of one of them and two epoxide precursors of their chemical synthesis, were tested for leishmanicidal activity on Leishmania donovani promastigotes and L. infantum amastigotes. Drugs inhibited proliferation of both forms of the parasite with a 50% lethal concentration range between 10.3 and 68.7 µg/ml. Their lethal mechanism was found linked to the respiratory chain by a systematic approach, including electron microscopy, measurement of the oxygen consumption rate on digitonin-permeabilized promastigotes, and enzymatic assays on a mitochondrial enriched fraction. Whereas the whole set of compounds inhibited the activity of fumarate reductase in the mitochondrial fraction (50% effective concentration [EC₅₀] between 33.3 and 78.8 µg/ml) and on purified enzyme (EC₅₀ = 53.3 to 115 µg/ml), inhibition for succinate dehydrogenase was only observed for the two phytoalexins with the highest leishmanicidal activity: anigorufone and its natural analogue 2-methoxy-9-phenyl-phenalen-1-one (EC₅₀ = 33.5 and 59.6 µg/ml, respectively). These results provided a new structural motif, phenyl-phenalenone, as a new lead for leishmanicidal activity, and support the use of plant extracts enriched in antifungal phytoalexins, synthesized under fungal challenge, as a more rational and effective strategy to screen for new plant leishmanicidal drugs.

	INTRODUCTION

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The human protozoan parasite Leishmania is the causative agent of leishmaniasis, a disease with a wide variety of clinical manifestations, ranging from self-healing cutaneous lesions (mostly species from Leishmania tropica and L. mexicana complexes) to life-threatening visceral infections caused by different species of the donovani complex (L. donovani, L. infantum, and L. chagasi). Leishmania threatens 350 million people worldwide with an annual incidence of 2 million cases and more than 12 million people infected (http://www.who.int/emc/diseases/leish/leisdis1.html). Due to the lack of a reliable human vaccine, together with the daunting control of parasite vectors and reservoirs, treatment relies exclusively on chemotherapy, with organic pentavalent antimonials as the first-line drugs (17). Nevertheless, their efficacy is impaired by the growing incidence of parasite resistance and their frequent and severe side effects (19). Alternative treatments, based on amphotericin B, paramomycin, allopurinol, and more recently, miltefosine, are also available (17), although most of these treatments have secondary effects (10). Thus, there is a pressing need for new leishmanicidal drugs.

One of the main sources for new leishmanicidal reagents is the isolation of secondary metabolites from plants (8, 15, 21). The biosynthesis of these molecules is carried out either in a constitutive, pathogen-independent manner (phytoanticipins) or is induced as a part of the plant defensive response against infection by bacteria, fungi, or nematodes (phytoalexins) (16). As expected from this functional classification, the structural diversity for both groups is extremely large, and structures such as flavanones, isoflavones, aurones, stilbenes, or phenalenones are gathered under the common name of phytoalexins (13, 16, 18, 25). A survey of the literature addressing the microbicidal activity of phytoalexins on human pathogens revealed an unexpectedly scarce number of works; these reports mainly focused on in vitro assays for bactericidal and fungicidal activities (7) and, to our knowledge, none of these studies examined the use of phytoalexins as antiprotozoal agents.

Anigorufone is an antifungal phenyl-phenalenone phytoalexin, isolated from the banana plant (Musa acuminata). Its synthesis is triggered by infection with the fungus Fusarium oxysporum, a saprophytic pathogenic fungus that causes Panama's disease in the banana plant (25). We tested anigorufone and reference 20 (REF20), another phytoalexin from the same origin, and reference 5 (REF5), a methoxy derivative of anigorufone, together with epoxide 5 (EP5) and epoxide 6 (EP6), two precursors of their chemical synthesis, on L. donovani promastigotes and L. infantum axenic amastigotes. All of these compounds demonstrated leishmanicidal activity. In a further step, definition of their targets was undertaken. Mitochondrial respiratory chain, the essential source for ATP production in Leishmania spp. (1, 38), was found to be one of the main targets for these compounds.

	MATERIALS AND METHODS

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Reagents. Anigorufone and 2-methoxy-9-phenyl-phenalen-1-one (REF20) were isolated from rhizomes of M. acuminata (AAA) infected with the fungus F. oxysporum (25). 2-Hydroxy-9-(p-methoxyphenyl)phenalen-1-one (REF5), was synthesized as previously reported (24). 2,3-Epoxy-9-(p-methoxyphenyl)phenalen-1-one (EP5) (24) and 2,3-epoxy-9-phenyl-phenalen-1-one (EP6) (25) were prepared as part of a general synthetic route to phenyl-phenalenone-type phytoalexins. Their structures and molecular weight are shown in Fig. 1.

View larger version (18K): [in this window] [in a new window]   FIG. 1. Chemical structures of the compounds assayed for leishmanicidal activity: anigorufone, 2-hydroxy-9-phenyl-phenalen-1-one (molecular weight = 272.31); REF5, 2-hydroxy-9-(p-methoxyphenyl)- phenalen-1-one (molecular weight = 302.33); REF20, 2-methoxy-9-phenyl-phenalen-1-one (molecular weight = 286.33); EP5, 2,3-epoxy-9-(p-methoxyphenyl)phenalen-1-one (molecular weight = 302.33); and EP6, 2,3-epoxy-9-phenyl-phenalen-1-one (molecular weight = 272.31).

Parasites. Promastigotes from the L. donovani strain MHOM/SD/00/1S-2D were grown in RPMI 1640 medium (Gibco, Paisley, United Kingdom), supplemented with 10% heat-inactivated fetal calf serum (HIFCS), 24 mM NaHCO₃, 25 mM HEPES, 2 mM L-glutamine, 100 U of uniciline/ml, and 48 µg of gentamicin/ml at pH 7.2 (RPMI+HIFCS) at 25°C. Its derived 3-Luc L. donovani strain was obtained by transfection with the expression vector pX63NEO-3Luc, which encodes for a Photinus pyralis luciferase form mutated in its C-terminal tripeptide as described previously (27). Parasites were grown under identical conditions in the medium described above but supplemented with 30 µg of Geneticin/ml (G418; Gibco). L. infantum axenic amastigotes (MCAN/ES/89/IPZ229/1/89) were grown at 37°C as described previously (2).

Cell proliferation measurements. Parasites were harvested at late exponential phase, washed twice in Hanks buffer supplemented with 10 mM D-glucose (pH 7.2; Hanks+Glc) at 4°C, and resuspended in the same buffer at 2 x 10⁷ cells/ml. Unless stated otherwise, these conditions were maintained for the rest of the experiments. Parasites (20 µl) were incubated with the drugs for 2 h at 25 or 37°C for promastigotes and amastigotes, respectively, washed with 1 ml of Hanks+Glc in order to remove unbound reagent, and resuspended in 100 µl of their respective culture medium devoid of phenol red. Parasites were then transferred into a 96-well microplate for a 48-h proliferation period according to their respective growth conditions. Finally, 100 µl of a 1-mg/ml MTT solution in Hanks+Glc was added, and substrate reduction was allowed to proceed for 2 h. The resulting formazan was solubilized by addition of 100 µl of 10% (wt/vol) sodium dodecyl sulfate solution and read in a 450 Bio-Rad microplate enzyme-linked immunosorbent assay (ELISA) reader, equipped with a 600-nm filter (23).

Assay for cytotoxic activity against mammalian cells. Murine macrophages of the J-774 (ATCC TIB-67) cell line were grown in RPMI+HIFCS and maintained at 37°C in 5% CO₂ and 90% humidity. Macrophages were resuspended in growth medium at a final concentration of 10⁵ cells/ml, placed in a 96-well culture microplate (100 µl/well), and incubated with the test drugs for 48 h. Cytotoxicity was assessed by using the colorimetric MTT reduction assay (6) and expressed as percentage of MTT reduction relative to control cells.

Bioluminescence assays. The substrate for luciferase, DMNPE-luciferin, was prepared as a 5 mM stock solution in dimethyl sulfoxide. It was added to the 3-Luc promastigote suspension (2 x 10⁷ cells/ml) in Hanks+Glc at a final concentration of 25 µM, and aliquots of this suspension were immediately distributed into a 96-well microplate (100 µl/well). Drugs were added once the luminescence reached a plateau. This point was considered as time zero, and its luminescence was taken as 100%. Changes in luminescence were recorded in a Polarstar Galaxy microplate reader (BMG Labotechnologies, Offenburg, Germany) fitted with luminescence optics, with measurements averaged every 4 s. Inhibition of in vitro luminescence with purified luciferase (Sigma) was carried out as described previously (27).

Promastigote membrane permeabilization. The procedure described by Thevissen et al. (34) was adapted to Leishmania promastigotes. Briefly, parasites (2 x 10⁷ cells/ml) were incubated with SYTOX green in Hanks+Glc (1 µM, final concentration) for 5 min in darkness, and 100-µl aliquots from this suspension were transferred into a 96-well microplate. After fluorescence stabilization, drugs were added at their respective 50% lethal concentration (LC₅₀). Maximal permeabilization was considered as that achieved by 0.1% Triton X-100. The fluorescence increase, due to binding of the dye to intracellular nucleic acids, was measured in a Polarstar Galaxy microplate reader equipped with 485- and 520-nm filters for excitation and emission wavelengths, respectively.

Electron microscopy. After incubation with drugs for 1 h, promastigotes were washed twice in phosphate-buffered saline (PBS), fixed in 5% (wt/vol) glutaraldehyde in PBS, included with 2.5% (wt/vol) OsO₄ for 1 h, gradually dehydrated in ethanol (30, 50, 70, 90, and 100% [vol/vol]; 30 min each) and propylene oxide (1 h), embedded in Epon 812 resin, and observed in a JEOL-1230 electron microscope.

Oxygen consumption rates. Oxygen consumption rates were measured in a Clark oxygen electrode (Hansatech, KingsLynn, United Kingdom) at 25°C by using 1 ml of a parasite suspension (10⁸ cells/ml) permeabilized with 60 µM digitonin and supplemented with 100 µM ADP as described previously (1). After drug addition and once a steady rate was reached, a selective set of substrates and inhibitors of the respiratory chain was assayed at final concentrations of 6.7 mM -glycerophosphate, 0.1 mM tetramethyl-p-phenylenediamine plus 1.7 mM ascorbate (TMPD-ascorbate), 2 mM malonate, 1.9 µM antimycin A, and 10 mM KCN.

Obtention of mitochondrial fraction. The protocol described previously by Chen et al. was used (8). Promastigotes were washed twice in Hanks buffer and resuspended in hypo-osmotic 5 mM Tris-HCl (pH 7.4) for 10 min at 25°C. This suspension was homogenized in a Potter-Elvehjem homogenizer on ice and then centrifuged at 1,000 x g for 10 min to remove cellular debris. The supernatant was next centrifuged for 20 min at 13,000 x g. The pellet, containing the mitochondrial fraction, was resuspended in isotonic phosphate saline buffer (50 mM sodium phosphate [pH 7.2], 90 mM NaCl, 5 mM KCl) at a protein concentration of 0.5 mg/ml. Aliquots (100 µl/well) of this mitochondrial fraction were distributed into a 96-well microplate and incubated for 1 h at 25°C with the respective drugs. These conditions were maintained for the rest of the enzymatic assays with the mitochondrial fractions.

SDH activity. The succinate dehydrogenase (SDH) activity was measured spectrophotometrically at 600 nm in a 450 Bio-Rad microplate ELISA reader in the presence of 3 mM succinate, 0.5 mM 2,6-dichlorophenol indophenol (DCPIP), and 0.1 mM phenazine methosulfate (8).

Succinate- and NADH-cytochrome c reductase activities. Succinate- and NADH-cytochrome c reductase activities were measured as changes in 550-nm absorption of a solution containing 20 µM cytochrome c and 5 mM succinate or 0.2 mM NADH, respectively, in a 450 Bio-Rad microplate ELISA reader with a 550-nm filter (8).

FRD activity. Fumarate reductase (FRD) activity was assessed as the rate of NADH oxidation (100 µM) upon 1 mM fumarate addition. The decrease of NADH fluorescence was monitored in a Polarstar Galaxy microplate reader equipped with 340- and 470-nm filters for excitation and emission wavelengths, respectively.

Purification of NADH-FRD. FRD activity was purified according to the protocol described by Chen et al. (8). The promastigote mitochondrial fraction was resuspended in a high-ionic-strength buffer (50 mM sodium phosphate [pH 7.2], 90 mM NaCl, and 150 mM KCl), incubated for 30 min in ice, and spun down (100,000 x g, 40 min, 4°C). The FRD activity, present in the supernatant, was purified by an initial concentration on HiTrap QFF column (Amersham Biosciences, Barcelona, Spain), followed by size exclusion chromatography on a HiPrep 16/60 Sephacryl S-200HR column (Amersham Biosciences), and finally fractionated on an HPLC Mono-Q HR 5/5 (Pharmacia, Uppsala, Sweden) through a 0.05 to 1 M NaCl gradient, with a purification factor between 90 and 120, similar to that previously reported (8).

Statistical analysis. Data represent the mean of triplicates ± the standard deviation. Experiments were repeated at least twice. The 50% effective concentration (EC₅₀) and the LC₅₀ values were calculated by the Litchfield and Wilcoxon procedure, and their 95% confidence interval is included in parentheses in Table 1.

	RESULTS

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None of the phenyl-phenalenones caused a decrease in J774 cell proliferation beyond 10% at a concentration fivefold their respective LC₅₀ for Leishmania amastigotes.

Inhibition of luminescence. In vivo real-time monitoring of intracellular ATP levels can be easily performed with the 3-Luc L. donovani strain (27). In order to bypass the poor membrane permeability of D-luciferin at neutral pH, it was substituted by its free membrane-permeable caged analogue DMNPE-luciferin. The luminescence was inhibited in a dose-dependent manner for the whole set of compounds, as illustrated for anigorufone (Fig. 2, inset). To compare the inhibition of promastigote luminescence for the five compounds, they were assayed at their corresponding LC₅₀s. The results are represented in Fig. 2. Except for EP6, all of them caused 40 to 60% inhibition relative to the initial value. Anigorufone displayed a steady decline extended for 60 min, whereas the pattern for the rest of compounds followed an exponential decay with a fast initial step lasting for 10 min. None of the drugs inhibited in vitro purified luciferase activity at their highest concentration beyond 5% (data not shown).

View larger version (26K): [in this window] [in a new window]   FIG. 2. In vivo variation of the luminescence of 3-Luc L. donovani parasites after drug addition at their respective LC50. Parasites (2 x 107 cells/ml) were incubated with 25 µM DMNPE-luciferin. When luminescence reached a plateau, drug was added (t = 0) and luminescence was monitored as described in Materials and Methods. Drugs were administered as follows: 12 µg of anigorufone/ml (•), 24 µg of REF5/ml (), 10 µg of REF20/ml (), 38 µg of EP5/ml (), and 69 µg of EP6/ml (). The inset shows the dose-dependent variation of luminescence with anigorufone at 2.5 µg/ml (), 5 µg/ml (), 10 µg/ml (), 15 µg/ml (), and 20 µg/ml (•). The results were normalized relative to the luminescence variation in control parasites.

Electron microscopy. In order to gain insight into the damage caused to the parasite by the drugs, electron microscopy of treated parasites was carried out. Figure 3 shows the promastigotes treated with the different drugs at their LC₅₀s. Swelling of mitochondria was observed in more than 50% of the parasites for the whole set of phenyl-phenalenones and was particularly evident for EP5 and EP6 (Fig. 3E and F), whereas the plasma membrane integrity appeared unharmed. Furthermore, a more dramatic effect was observed for anigorufone and REF20 since they caused extensive intracellular damage with strong disorganization of cytoplasmic organelles (Fig. 3B and D). At lower concentrations the extent and percentage of injured cells was lower (data not shown).

View larger version (121K): [in this window] [in a new window]   FIG. 3. Electron microscopy of L. donovani promastigotes treated with phenyl-phenalenones at their respective LC50s. (A) Control parasites; (B) anigorufone; (C) REF5; (D) REF20; (E) EP5. (F) EP6. k, kinetoplast. Bar, 0.5 µm.

Inhibition of mitochondrial enzymatic activities. We next set out to further define the Leishmania target for phenyl-phenalenones. We proceeded by testing in the promastigote mitochondrial fraction of the inhibitory activity on the enzymatic activities associated with complex II. At their LC₅₀ for promastigotes, none of the drugs inhibited more than 3% succinate- or NADH-cytochrome c reductase activities (data not shown), which are involved in the electron transfers from complex II to III and from complex I to III, respectively. FRD activity was inhibited by the whole set of drugs in a dose-dependent manner (Fig. 4). EP6 caused the highest inhibition (EC₅₀ = 33.3 µg/ml), whereas REF5 showed the lowest activity (EC₅₀ = 78.8 µg/ml) (Table 1). In contrast, SDH activity (32.9 nmol/min/mg of protein) was only inhibited by anigorufone and REF20 and at concentrations higher than their LC₅₀ values (Fig. 5). When compared on purified FRD, all of the drugs inhibited the enzyme (Table 1), although with EC₅₀s consistently higher (2-fold) relative to those obtained on mitochondrial fraction; a similar situation was previously reported for licochalcone A and was attributed to changes in the physiological conditions (8).

View larger version (20K): [in this window] [in a new window]   FIG. 4. Inhibition of FRD activity in the mitochondrial fraction of L. donovani promastigotes, with different phenyl-phenalenones. The results for anigorufone (•), REF5 (), REF20 (), EP5 (), and EP6 () are given. The data represent the average of at least two different experiments.

View larger version (19K): [in this window] [in a new window]   FIG. 5. Inhibition of SDH activity in the mitochondrial fraction of L. donovani promastigotes. SDH was assayed by determining the reduction of DCPIP as described in Materials and Methods. The results for anigorufone (•), REF5 (), REF20 (), EP5 (), and EP6 () are shown. Maximal inhibition (100%) was considered to be that caused by 12 mM malonate.

	DISCUSSION

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The second option, inhibition of ATP synthesis, was supported by the consistent observation in treated parasites of swollen mitochondria, only identified by the presence of the electron-dense kinetoplast. In parasites treated with REF5, EP5, or EP6, this was the main structural observation; a similar effect was reported for licochalcone A, a leishmanicidal drug targeting the mitochondria (39). In contrast, in promastigotes treated with anigorufone or REF20, a more extensive intracellular damage, not limited to mitochondria, was evidenced. However, alteration of plasma membrane was not observed for any drug.

We addressed the aforementioned possibility by searching the phenyl-phenalenone targets on the respiratory chain, since oxidative phosphorylation is the major source for energy generation in Leishmania (1, 38). In digitonin-permeabilized parasites, phenyl-phenalenones inhibited the oxygen consumption rate by using succinate as the substrate. Since this was partially restored by addition of TMPD-ascorbate, which donates electrons to cytochrome c, the putative phytoalexins targets were restricted upstream cytochrome c. The addition of -glycerophosphate partially restored oxygen consumption; thus, complex II was considered to be the more likely target for phenyl-phenalenones (28). In a step beyond, it was found that SDH and FRD, associated with the mitochondrial fraction, were inhibited by anigorufone and REF20 or by the whole set of phenyl-phenalenones, respectively. An unspecific effect was ruled out, since neither succinate- nor NADH-cytochrome c reductase was inhibited by any phenyl-phenalenone, but all of them inhibited the purified FRD and preserved the same pattern of inhibitory activity obtained in the mitochondrial fraction. Nevertheless, at a given concentration of any of these drugs, the inhibition of FRD was consistently lower in the purified enzyme than in the mitochondrial fraction. This effect was also reported for licochalcone A, another inhibitor of FRD in Leishmania (8). This is most likely due to the loss of modulation of the FRD-soluble catalytic portion by its membrane hydrophobic domain, which is absent in the purified enzyme. In fact, for other organisms, it has been reported that the hydrophobic portion is involved in electron transfer to the catalytic subunits (37). Accordingly, from a physiological perspective, the results obtained for mitochondrial fraction are more relevant than those obtained for the purified enzyme, as noted when the EC₅₀s for both forms of the enzyme (membrane-bound and purified) were compared to their respective LC₅₀ values.

Despite some controversies concerning the bioenergetic metabolism of Leishmania (4, 5, 8, 33, 38), FRD is likely an important target for the leishmanicidal activity of phenyl-phenalenones since (i) it is the only enzymatic activity from the panel assayed that is inhibited by the five compounds, (ii) inhibition of this enzyme is enough to account for the leishmanicidal effect of new drugs such as licochalcone A, aurones, or 2-mercaptopyridine-N-oxide (8, 22, 36), and (iii) FRD is an enzyme absent in mammalian cells (8, 37).

The large divergences inherent in the three experimental approaches used to assess phenyl-phenalenone activity (the use of live parasites, an enriched mitochondrial fraction, and purified FRD) may account for the quantitative differences among the inhibition of these parameters by phenyl-phenalenones. Furthermore, at present we cannot discard additional alternative targets for these drugs, as exemplified by anigorufone and REF20, the two compounds with the highest leishmanicidal effect, since they inhibited FRD and SDH activities simultaneously. Likewise, other sites of action, apart from the respiratory chain, cannot be excluded.

Natural plant products such as licochalcone A, plumbagin, and 2-substituted quinolones are new promising leishmanicidal drugs and have provided important leads for chemotherapy (8, 10). Unexpectedly, medical applications for phytoalexins, rather than to their antimicrobial activities (7), were related to cardiovascular or cancer prevention as reported for resveratrol (20, 32, 35), genistein (14), or brassinin (29). To the best of our knowledge, leishmanicidal activity has not yet been described for any compound explicitly defined as phytoalexin. Nevertheless, given that pathogen elicitation in plants is continuous under natural conditions, the odds for the unsuspected presence of phytoalexins in extracts or compounds with previously reported leishmanicidal activity are quite high.

In the present study we have demonstrated the leishmanicidal activity of five molecules based on a phenyl-phenalenone skeleton, a new lead structure for future development of leishmanicidal drugs. Their inhibition of SDH and FRD activities pinpoints these enzymes as their more likely targets. Two of them were originally isolated from the banana plant (M. acuminata) elicited with the fungus F. oxysporum (25). Thus, a new approach to define leishmanicidal agents will profit from this higher probability of finding new leishmanicidal compounds in plants previously challenged with fungi. This elicitation will induce antifungal phytoalexins that, in the best scenario, will share some of their antifungal targets with Leishmania. In a step beyond, this rationale might be further optimized by plant infection with a much closer evolutionary organism such as Phytomonas, a plant trypanosomatid. The feasibility of this new experimental approach will require additional investigation.

	ACKNOWLEDGMENTS

 
This study was supported by grants from C.A.M. (08.2/0054/2001.02) and the Plan Estratégico de Grupos en Biotecnología (EU grants QLK2-CT-2001-01404 and CICyT BIO2003-09056-CO2-02) to L.R. C.I.B. belongs to the Red Española de Investigación en Patología Infecciosa, supported by the Fondo de Investigaciones Sanitarias (grant C03/14). Work at the Instituto de Bio-Orgánica A. G. González was funded by the Spanish Ministry of Science and Technology (grant BQU2001-3721). L.R.I. thanks the Spanish Ministry of Science and Technology for a doctoral fellowship. The Departamento de Parasitología was supported by grant 1802380102 from La Laguna University.

L. infantum axenic amastigotes (MCAN/ES/89/IPZ229/1/89) were kindly provided by María Colmenares (C.I.B.-C.S.I.C). The technical assistance of María Dolores Guirao Rey (C.I.B.-C.S.I.C) with the electron microscopy and critical reading of the manuscript by Victoria Herrán Coombs (Universidade Da Coruña) are greatly appreciated.

	FOOTNOTES

 
* Corresponding author. Mailing address: Centro de Investigaciones Biológicas, Ramiro de Maeztu 9, E-28040, Madrid, Spain. Phone: 34-918373112, ext. 4234. Fax: 34-915627518. E-mail: luis_rivas{at}cib.csic.es.

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