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Revista Colombiana de Ciencias Hortícolas

Print version ISSN 2011-2173

rev.colomb.cienc.hortic. vol.16 no.2 Bogotá May/Aug. 2022  Epub Feb 18, 2023

https://doi.org/10.17584/rcch.2022v16i2.13882 

Section of other species

In vitro effect of cocoa leachates ongrowthanddevelopmentof Moniliophthora roreri ([Cif.] H.C. Evans et al.) isolatedfrom Theobroma cacao (L.)

Evaluación in vitro de lixiviados de cacao sobre el crecimiento y desarrollo de Moniliophthoraroreri ([Cif.] H.C. Evans et al.) aislado de Theobroma cacao (L.)

SANDRA VICTORIA GÓMEZ-GUTIÉRREZ1  3 
http://orcid.org/0000-0001-7950-0814

CAMILO RUBÉN BELTRÁN-ACOSTA2 
http://orcid.org/0000-0002-6063-6962

SANDRA GÓMEZ-CARO1 
http://orcid.org/0000-0002-6670-0275

1 Universidad Nacional de Colombia, Facultad de Ciencias Agrarias, Bogota (Colombia).

2 Corporación Colombiana de Investigación Agropecuaria (AGROSAVIA), Centro de Investigación Tibaitatá, Mosquera ( Colombia).


Abstract

The cocoa crop is part of the peasant’s economic activity and agroforestry systems in many regions of Colombia and the world. Its yields are diminished by phytosanitary problems, being the frosty pod rot caused by the fungus Moniliophthora roreri, the most limiting disease with decreases in production of over 90%. In this study, samples of cocoa leachates from commercial producing farms were characterized and the antifungal activity of sterilized, non-sterilized, and filtered cocoa leachates against M. roreri was evaluated under in vitro conditions, at concentrations of 1, 2, 5, 10, and 15%. Monosporic isolates of the pathogen were obtained from diseased fruits collected from cocoa-producing farms in the municipality of Yacopi in Cundinamarca, Colombia. The effect of leachates on M. roreri conidial germination, mycelial growth, and inoculum production was evaluated. It was found that non-sterilized cocoa leachates at all concentrations caused 100% reduction on the three variables evaluated, while sterilized leachates generated the same effect at concentrations of 10 and 15%. Filtered leachates showed no inhibitory effect on the radial growth of the pathogen, but they caused a reduction of conidial germination of 89.9, 90.5 and 95.9% at concentrations of 5, 10, and 15%. The presence of malic, citric, and ascorbic acids, compounds such as NH4, PO4, and NO3, and elements such as Ca, K, Na, Mg, and Cl in the evaluated leachates was identified using high-efficiency liquid chromatography and physicochemical analysis. This research showed the potential of cocoa leachates, even at low concentrations, for the control of M. roreri, which can be attributed to the action of specific compounds such as those found in chromatographic tests.

Additional keywords: fungal mycelialgrowth; conidia germination; frosty pod rot disease; liquid products

Resumen

El cultivo de cacao es parte de la actividad económica campesina y de sistemas de agroforestería en muchas regiones de Colombia y del mundo. Su rendimiento se ve disminuido por problemas fitosanitarios, siendo la monilia causada por el hongo Moniliophthora roreri, la enfermedad más limitante causando disminuciones de producción de más del 90%. En este estudio, se caracterizaron muestras de lixiviados de cacao de fincas comerciales y la actividad antifúngica de estos lixiviados esterilizados, no esterilizados, y filtrados contra M. roreri fue evaluada bajo condiciones in vitro en concentraciones de 1, 2, 5, 10, y 15%. Aislamientos monospóricos del patógeno fueron obtenidos a partir de frutos enfermos colectados en fincas productoras de cacao del municipio de Yacopí en Cundinamarca, Colombia. El efecto de los lixiviados se evaluó sobre la germinación conidial de M. roreri, el crecimiento micelial, y la producción de inóculo. Se encontró que los lixiviados de cacao no esterilizados en todas las concentraciones generaron 100% de reducción de las tres variables evaluadas, mientras que los lixiviados esterilizados generaron el mismo efecto a concentraciones de 10 y 15%. Los lixiviados filtrados no mostraron efecto inhibitorio sobre el crecimiento radial del patógeno, pero una reducción de la germinación conidial de 89,9; 90,5 y 95,9% a las concentraciones de 5, 10, y 15%, respectivamente. La presencia de ácido málico, cítrico, y ascórbico, compuestos como NH4, PO4, y NO3, y elementos como Ca, K, Na, Mg, y Cl fue identificada en los lixiviados evaluados usando cromatografía líquida de alta eficiencia y análisis fisicoquímicos. Esta investigación mostró el potencial de los lixiviados de cacao, aún a bajas concentraciones para el control de M. roreri, el cual puede ser atribuido a la acción de compuestos específicos como los encontrados en las evaluaciones cromatográficas.

Palabras clave adicionales: crecimiento micelial; germinación conidial; monilia; productos líquidos

INTRODUCTION

The cocoa (Theobroma cacao L.) is a tropical species from which chocolate and its derivatives are obtained (Lozada et al., 2012). It is cultivated by 6 million farmers and is the source of income for more than 40 million people around the world (Fromm, 2016). The International Cocoa Organization (ICCO) estimated that more than 4.697 million metric tons of cocoa beans were produced globally between 2019 and 2020. According to this report, Africa was the first largest cocoa-producing continent with 75.7% (3.55 million tons), followed by the Americas with 18.4%, and Asia and Oceania with 5.9% (ICCO, 2020). According to Fedecacao (National Federation of Cocoa Producers), Colombia registered a production of 63,416 t for 2020, showing an increase of 6.1% compared to the production in 2019 (Fedecacao, 2021).

The cocoa crop is affected by limiting diseases, among which are the black pod caused by the oomycete Phytophthora spp., witches’ broom disease (Moniliophthora perniciosa (Stahel) Aime and Phillips-Mora), and frosty pod rot (Moniliophthora roreri (Cif.) H.C. Evans et al., 1978) that can cause significant yield losses (Jaimes et al., 2016; Pérez-Vicente, 2018). Frosty pod rot is the most economically limiting disease in all the Latin American countries where cocoa is cultivated (Phillips-Mora et al., 2005; Sánchez-Mora et al., 2014). The center of origin of the disease is central/north-eastern Colombia where the highest levels of genetic diversity of the pathogen have been found (Phillips-Mora et al., 2006b; Phillips-Mora et al., 2007). M. roreri has progressively expanded from its center of origin in South America northwards through Central America and Mexico and westwards across the Andes and Amazonian forests (Phillips-Mora et al., 2006b). In Colombia, frosty pod rot has generated losses of over 90% (Phillips-Mora et al., 2006a; Phillips-Mora and Wilkinson, 2007; Jaimes and Aranzazu, 2010; Correa et al., 2014).

The pathogen only attacks the fruits at any stage of development causing external and internal damage and total pod loss (Jaimes et al., 2016). Pods of less than 2 months old are the more susceptible (Sánchez and Garcés, 2012). Initial infections are symptomless, except for tissue swelling causing deformations or bumps (Bailey et al., 2018). Subsequently, a brownish spots appears on the fruit’s surface, on which millions of conidia develop, forming a cream-colored powder. These conidia are dispersed by the wind and when they fall on a healthy fruit, under appropriate conditions, they germinate penetrating the cuticle or stomata. The structures colonize tissues intercellularly invading the cortical parenchyma and starting the disease cycle again (Evans et al., 2003; Ramírez, 2013; Correa et al., 2014; Bailey et al., 2018).

Frosty pod rot management consists of sanitary pruning of fruits, planting of improved material, and biological control practices (Krauss et al., 2010; Suárez and Rangel, 2013). The application of systemic fungicides has shown low efficacy and increases production costs (Flood and Murphy, 2004; Bateman et al., 2005). Therefore, it is necessary to look for new alternatives to manage the disease. Liquid products of the decomposition of harvest residues, known as leachates (Weltzien, 1991; Bele et al., 2018) have been reported with the potential to control some plant diseases. The use of banana rachis leachates to control black leaf streak disease (Osorio et al., 2012) has shown the ability to inhibit mycelial growth and germination of Botryodiplodia theobromae, Colletotrichum musae, Fusarium sp., and Musicillium theobromae conidia, pathogens that cause postharvest diseases in banana (Musa acuminata Colla) in Ivory Coast (Bele et al., 2018). This last study showed that leachate concentrations of 5, 15, and 20% exhibited an antifungal activity, with the 20% concentration being the most effective and the one that obtained complete inhibition of mycelial growth and conidial germination of all the fungi evaluated (Bele et al., 2018). The in vitro and in vivo effects of banana rachis leachates have also been demonstrated for the control of southern blight in tomatoes caused by Sclerotium rolfsii in Porto-Novo, Benin (Africa). In that study, leachates inhibited mycelial growth and pathogen development in the field with effectiveness similar to that found for the fungicide Maneb 80 (Sikirou et al., 2010).

Kamel et al. (2014) report the use of fulvic acid extracted from banana rachis to control powdery mildew (Pohosphaera fusca (syn. Sphaerotheca fuliginea)) and downy mildew (Pseudoperonospora cubensis) in cucumber at the Agricultural Research station in Sakha, Egypt. Álvarez et al. (2015) mention that leachates contain a high concentration of potassium that induces resistance to some diseases. These authors also state that applications of 5% fulvic acids from banana leachates reduce the severity of powdery mildew in roses caused by Sphaerotheca pannosa. There are no reports of the use of cocoa leachates for the control of M. roreri, although vegetable extracts of grapefruit, pepper, marjoram, and linden have been evaluated for their in vitro control. All these extracts without sterilization and at a concentration of 25% generated a 100% inhibition of mycelial growth (Arcos-Méndez et al., 2019). In Colombia, leachates from banana rachis have been assessed in vitro and in vivo against Mycosphaerella fijiensis and in vivo for S. pannosa in rose crops (Álvarez et al., 2010; Álvarez et al., 2015). Nevertheless, its use by farmers is still empirical and some leachates have been mainly used as biofertilizers or biofungicides. Cocoa leachates are obtained from the bean fermentation process. The mucilage that covers the seeds is subjected to a fermentation process by the action of microorganisms, forming sugars and then acetic acid. During the first 24 h of this process, cocoa beans leach substances or leachates composed of amino acids, sugars, and other substances (Wacher, 2011). This study sought to (i) characterize cocoa leachate samples from commercial cocoa producing farms and (ii) evaluate, under in vitro conditions, the potential antifungal activity of cocoa leachates against M. roreri at variable concentrations as an alternative for disease management with low impact on the production system, to provide knowledge on the potential use of these leachates.

MATERIALS AND METHODS

Characterization of cocoa leachates from two commercial producing farms in Cundinamarca

Cocoa leachates production and collection

The leachates obtained from the fermentation of cocoa beans were collected in sterile glass containers 24 h after the beginning of the fermentation process and kept refrigerated at 6ºC. This period was selected due to the fact that the highest amount of leachates was produced at this time. To conduct the study, three samples (S) of leachates were obtained from two farms located at the municipality of Yacopi (Cundinamarca, Colombia). Leachates were obtained from the farms La Floresta (5º 31' 30.3'' N, 74º 20' 40.39'' W) (S1 and S3), and Filadelfia (5º 29' 18.3'' N, 74º 20' 3.7'' W) (S2). These farms were selected due to the fact that both were planted with cocoa clones CCN51, ICS95 TSH565, ICS60, EET8, YAC2, and farmers followed a similar fermentation procedure to obtain the cacao leachates.

Physicochemical and chromatographic analysis of cocoa leachates

To determine the compounds that are present in the three leachate samples and their concentration, the physicochemical analysis of cocoa leachates was carried out at the Water and Soils Laboratory of the Faculty of Agricultural Sciences at Universidad Nacional de Colombia. The following variables were evaluated: pH, using the potentiometric method (Tello and Fernández, 2012); OH, CaCO3, and HCO3 by titration with H2SO4 (Roldán and Ramírez, 2008); chlorides by titration with AgNO3 (Carrasquero and Castillo, 2002); sulfates using barium chloride by turbidimetric titration (Aguilera et al., 2010); phosphates and ammonium by colorimetric titration (D’Angelo et al., 2001); Ca, Mg, K and Na using atomic absorption spectrometry (Pohl et al., 2012), and B by potentiometric titration (Peña et al., 2012). The electrical conductivity (EC) was measured by reading with a conductivity meter (Schott, Lab960 and electrode of the same brand) at 25°C and the sodium adsorption ratio (SAR) that consists of the ratio between Na and Ca plus Mg (Peña et al., 2012).

The analysis by high-efficiency liquid chromatography was carried out at the Postharvest Laboratory of the Faculty of Agricultural Sciences at Universidad Nacional de Colombia. The main sugars and organic acids in the compound were determined following the methodology of Zheng et al. (2016). The samples were centrifuged (3,000 rpm, 5 min) to eliminate impurities and the supernatant was stored at 4ºC. Then, 0.5 mL of the leachate sample was taken and completed to a volume of 5 mL with H2SO4 1N solution. This solution was subjected to analysis on an Ultimate 3000 Dionex HPLC chromatograph (Zheng et al., 2016).

In vitro evaluation of the antifungal activity of cocoa leachates against Moniliophthora roreri at variable concentrations

Collection of affected plant material and obtaining of M. roreri isolates

Fruits with symptoms associated with frosty pod rot were collected in the farms Filadelfia (5º 29' 18.3'' N, 74º 20' 3.7'' W) and El Porvenir (5° 31' 2.6'' N, 74° 20' 40.2'' W) located in the municipality of Yacopi, province of Rionegro, at the north of the department of Cundinamarca (Colombia). The conditions of these farms were as follows: an average temperature of 21.1°C (minimum of 18.8°C and maximum of 29°C), average annual rainfall of 2,592 mm, and relative humidity between 81 and 90% (Pinzón et al., 2012; Penagos, 2019). In each farm, 15 trees were randomly selected to collect fruits with the presence of the pathogen. These fruits were processed at the Plant Health Laboratory of the Faculty of Agricultural Sciences at Universidad Nacional de Colombia, Bogotá campus.

Five mm explants were taken from the diseased fruits collected, making deep cuts of the affected tissue at the lesion site. Explants were disinfected using 70% alcohol for 1 min, 2% sodium hypochlorite for 30 s, followed by three washes with sterile distilled water (Barrera and García, 2008). Then, they were seeded in Petri dishes with Potato Dextrose Agar (PDA) medium (Oxoid, Thermo Scientific, USA). The dishes were incubated for 14 d at 25°C until sporulation. Isolates of the pathogen were confirmed by macroscopic and microscopic characterization (Phillips-Mora et al., 2006a; Phillips-Mora et al., 2006b). Finally, monosporic cultures were carried out following the methodology described by Carrera-Sánchez et al. (2014).

Isolates were then cultured on PDA medium (Oxoid, Thermo Scientific, USA), and the diameter of the colony and sporulation were measured in eight isolates obtained (data not shown) for 14 d. The isolate with the highest rate of mycelial growth in time (mm d-1) and the highest conidia production per cm2 of the colony was selected.

Preparation of culture medium with cocoa leachates for in vitro evaluations

Cocoa leachates were centrifuged at 3,000 rpm for 5 min to remove impurities (Sorvall Legend X1, Thermo Scientific, USA). Subsequently, they were added to sterile PDA medium (120°C, 20 min) before solidifying, at concentrations of 1, 2, 5, 10, and 15% v/v in relation to the culture medium, following the agar diffusion method (Chang et al., 2008). Petri dishes with PDA and the growing pathogen were used as controls.

On a second evaluation, a PDA medium was prepared, and the cocoa leachates were added at the same concentrations mentioned above, before the sterilization process. The mixture of culture medium and cocoa leachates was then subjected to autoclave sterilization at 120°C for 45 min (Automatic electromechanical autoclave, Aravell, Colombia). Petri dishes with PDA and the growing pathogen were used as controls.

The third method evaluated consisted in filtering the leachates using sterile 0.20 μm filters (Millipore) after centrifugation (3,000 rpm, 5 min). The filtered leachates were added to the culture medium previously sterilized in an autoclave. The treatments were the same as those of the previous evaluations. Petri dishes with PDA and non-sterilized leachates and Petri dishes with PDA, both with the growing pathogen, were used as controls.

Evaluations of antifungal activity of cocoa leachates on M. roreri

The antifungal activity of cocoa leachates to inhibit the radial growth of the fungus was determined by macroscopic observation, placing an agar/M. roreri mycelium disc (5 mm radius) from monosporic cultures of the 18-d-old pathogen in each of the Petri dishes with cocoa leachates at the evaluated concentrations according to the treatment (Chuah et al., 2010) and controls. Radial growth was determined by measuring the diameter (mm) of colonies for 14 d (time during which the pathogen in the control treatment completed growth in the Petri dishes).

Percentage of inhibition of M. roreri mycelial growth

The toxicity of cocoa leachates on M. roreri was expressed as the percentage of inhibition of mycelial growth (IMG) of M. roreri, according to the formula proposed by Yahyazadeh et al. (2007), after 14 d of growth on PDA culture medium (1).

IMG (%)= [(C-T)/C]×100 (1)

where, C is the diameter of the pathogen colony in the control treatment without cocoa leachates, and T is the diameter of the pathogen colony according to the cocoa leachate concentrations evaluated.

Evaluation of the effect of cocoa leachates on the germination of M. roreri conidia

Cocoa leachates were centrifuged at 3,000 rpm for 5 min to remove impurities (Sorvall Legend X1, Thermo Scientific, USA). Subsequently, they were added to a sterile water agar (WA) culture medium (Oxoid, Thermo Scientific, USA) before solidification at concentrations of 1, 2, 5, 10, and 15 v/v in relation to the culture medium.

For the second evaluation method, the leachates were added to the WA medium before sterilization at the same concentrations. Finally, for filtered leachates, the same concentrations mentioned above were added to the WA medium previously sterilized in an autoclave. To evaluate the effect of cocoa leachates on conidial germination, 200 μL of a 4.5·104 conidia/mL suspension of M. roreri was seeded on WA with the concentrations of leachates to be evaluated (prepared by the three methods previously described). Conidial germination was determined by microscopic counting (Olympus CX31, Olympus, Japan) every 24 h for 96 h. For this purpose, 100 conidia were evaluated and those conidia that showed a germ tube with twice the diameter of the conidia were considered germinated (Marín and Bustillo, 2002). Germination values were calculated as the ratio between germinated and the total number of evaluated conidia and then expressed as percentage.

Evaluation of the effect of cocoa leachates on M. roreri inoculum production

Conidia formed on sterilized and non-sterilized leachate treatments and controls were collected 14 d after incubation by removal with 2 mL of sterile distilled water with Tween 80. The number of conidia produced was determined by quantification in a Hemocytometer (Boeco, Germany) (Petlamul and Prasertsan, 2012). The effect of filtered leachates on inoculum production was not evaluated. Filtration was considered as a complementary analysis to evaluate if the sterilization method may alter leachates effect on mycelial growth and conidia germination of M. roreri.

Determination of EC50 value for mycelial growth and conidia germination inhibition

The effective concentration of cocoa leachates to reduce mycelial growth or conidia germination by 50% (EC50) was calculated by fitting the mycelial growth or conidia germination rate against the log transformed cocoa leachate concentrations using the best fitting model (lLL.4) in the R package “drc'' v3.0.1 (Ritz et al., 2015).

Experimental design and statistical analysis

A completely randomized design was used to evaluate the antifungal activity of cocoa leachates. Five concentrations of leachates (1, 2, 5, 10, and 15% v/v) were evaluated for sterilized, non-sterilized and filtered leachates, for a total of 16 treatments including the control treatment (0%), in which no leachates were added to the culture media. Seven replicates were used for each combination of leachate concentration and sterilization method. Each replicate corresponded to one Petri dish with the PDA medium amended with the cocoa leachate concentration to be assessed. Filtered leachates were assessed in five replicates at each concentration due to contamination of two of the initially established replicates. Additional experiments were conducted to validate the obtained results. The free statistical software R 3.6.2 (R Development Core Team, 2019) (PBC, Boston, USA) and the packages dplyr (Wickham et al., 2021), ggplot2 (Wickham, 2009) and car (Fox and Weisberg, 2019) were used for the analysis of radial growth, conidial germination, and inoculum production data. An ANOVA mean comparison analysis and Tukey's test were performed with a probability value of P≤0.05.

RESULTS

Physicochemical and chromatographic analysis of cocoa leachates evaluated on M. roreri

The analyses showed an acidic pH lower than 3.7 in the three leachate samples from the farms La Floresta (S1 and S3) and Filadelfia (S2) (Tab. 1); for this parameter, the three leachates showed similar values (3.66, 3.64 and 3.49, respectively).

Table 1. Presence and quantity of basic compounds, sugars and main acids in the cocoa leachate samples (S1 and S3 - La Floresta, S2 - Filadelfia), expressed as concentration in mg L-1 of compound and/or elements obtained by physicochemical analysis of water and liquid compounds. 

Parameter Sample 1 (S1) Sample 2 (S2) Sample 3 (S3)
Chromatographic analysis
Fructose 3,982 1,793 6,332
Glucose 4,246 5,318 3,831
Saccharose 2,032 157 1,234
Citric acid 91,677 10,160 132,693
Ascorbic acid 697 143 340
Malic acid 79,783 125,208 138,014
Physicochemical analysis
pH 3.66 3.64 3.49
Cl* 246 215 273
SO4* 240 74.1 134
PO4* 27.0 64.9 172
NO3* 45.5 23.7 28.8
Ca* 232 67.5 108
K* 1,238 1,045 1,148
Mg* 186 151 132
Na* 5.43 2.41 4.29
NH4* 25.3 8.35 30.9
EC 4.3 2.9 3.4
SAR 0.06 0.04 0.07

*: measurements in mg L-1. EC: Electrical conductivity, SAR: Sodium absorption ratio.

S1 and S3: leachates obtained from the farm La Floresta (5º 31' 30.3'' N, 74º 20' 40.39'' W). S2: leachates obtained from the farm Filadelfia (5º 29' 18.3'' N, 74º 20' 3.7'' W). Both farms are located at Yacopi, Cundinamarca. Colombia.

The concentrations of Cl, K, and Mg were close among the three leachate samples. The SAR also showed similar values for the three leachate samples evaluated (Tab. 1). On the other hand, the NH4 concentration for samples S1 and S3 did not show differences between these two samples. However, a lower NH4 concentration was obtained in sample S2 than in samples S1 and S3 (Tab. 1). This result shows close values of NH4 concentration in the leachates from the farm La Floresta (S1 and S3) in contrast to those obtained in the second farm (Filadelfia, S2). In the case of S, leachate sample S1 showed a higher content (240 mg L-1) than that found in samples S2 (74.1 mg L-1) and S3 (134 mg L-1). Sample Sl obtained a Ca concentration of 232 mg L-1 compared to 67.5 mg L-1 and 108 mg L-1 in samples S2 and S3, respectively (Tab. 1). For this parameter, the higher values were observed in the leachates from the farm La Floresta (S1, S3) in contrast to those obtained from the second farm (Filadelfia, S2).

Simple and compound sugars such as fructose, glucose, and sucrose were found at different concentrations in each of the leachates evaluated. Values for fructose of 3,982, 1,793 and 6,332 mg L-1 were determined in the leachates of samples S1, S2, and S3, respectively (Tab. 1). However, the results showed a wide variation in the concentration of this compound between leachates S2 and S3. In the case of glucose, close values were found among the evaluated samples (Tab. 1). Saccharose concentration showed variation between both farms, with close values in the samples S1 and S3 (Floresta) and the lowest values observed in S2 (Filadelfia).

The presence of citric, ascorbic, and malic acids was identified. Citric and malic acids were found at higher concentrations in sample S3. Additionally, the leachates of S2 showed a lower content of citric and ascorbic acids compared to the other two samples evaluated (Tab. 1).

Selection of the M. roreri isolate

Monosporic cultures were obtained from each of the eight isolates, and the growth speed of the colonies in vitro and inoculum production capacity were evaluated for each of them. Based on this information, one isolate from the farm Filadelfia was selected for its higher growth speed (90 mm diameter of the colony 12 d after incubation) and sporulation capacity (9·103 to 1·104 conidia/cm2).

Effect of cocoa leachates on the in vitro growth of M. roreri

Non-sterilized leachates showed a 100% inhibitory effect on the radial growth of M. roreri (P<0.000) from a concentration of 1 to 15% (Fig. 1A and 1B). These results were consistent with additional experiments conducted with other cocoa leachate samples in which 100% inhibitory effect was obtained (data not shown). The control treatment started mycelial growth from 18 to 24 h after seeding on the medium and continued during the 12 d of incubation, showing typical M. roreri colonies with a powdery appearance and beige to brown colors (Phillips-Mora et al., 2006a; Phillips-Mora et al., 2006b).

Figure 1. Radial growth of M. roreri under five cocoa leachate dilutions on PDA culture medium incubated at 25 °C at 2, 4, 6, 8, 10, 12 and 14 days after incubation (DAI) and their effect on the appearance of colonies 12 DAI for non-sterilized and sterilized leachates treatments, and 14 DAI for filtered leachates treatment. A. and B. Non-sterilized leacheates. C and D. Sterilized leachates. E and F. Filtered leachates, control (M. roreri on PDA) and leachate control (M. roreri on PDA with 10% non-sterilized leachates). I). The data represent the mean value of seven Petri dishes (n=7) for non-sterilized and sterilized leachates and five Petri dishes (n=5)for filtered leachates ± standard error per treatment. Letters refer to significant differences between means according to Tukey's test(P≤0.05). Control: CTR. 

In the culture medium prepared with the different dilutions of non-sterilized leachates, the profuse growth of bacterial colonies of similar size was observed, both on the surface of the medium and deep inside. The colonies showed a creamy appearance, individual growth, whitish to cream color without prominent elevation on the culture medium.

Regarding the leachates sterilized by autoclaving, in the 1, 2, and 5% treatments the mycelial growth of M. roreri did not show significant differences compared to the control. In these treatments, the colonies completed the total area of the Petri dish at 12 d of incubation (Fig. 1C). However, an alteration in the morphology of the colony was observed with the treatment of 5%. A change in pigment (hue) in the central axis of the colony was registered, which was of clear color and not beige (due to lower sporulation), with a cottony and dense appearance compared to the control (Fig. 1D). Significant differences were found for the evaluated concentrations of 10 and 15% compared to the control (P<0.0001 and P<0.0001, respectively). The sterilized cocoa leachates at a concentration of 10% inhibited about 80% of the radial growth of the M. roreri colony (Fig. 1C and 1D) and the concentration of 15% showed a 100% inhibitory effect on the mycelial growth of M. roreri (Fig. 1C and 1D). In additional experiments conducted with other cocoa leachate samples, an inhibitory effect of 88% of the radial growth for the concentration of 10%, and an inhibitory effect of 100% for the concentration of 15% were observed (data not shown).

Significant differences were not found in the diameter of the colony between the different concentrations of filtered leachates and the control treatment of the fungus growing on PDA. Significant differences were found in the diameter of the colony between the concentrations of filtered leachates and the treatment of non-sterilized leachates at a concentration of 10% (leachate control) (P<0.0001). The obtained result confirmed the inhibitory effect of non-sterilized leachates on the mycelial growth of the fungus (Fig. 1E and 1F).

Percentage of inhibition of M. roreri mycelial growth

Non-sterilized leachates were the most effective, with 100% inhibition of the mycelial growth of the pathogen (P<0.0000) (Tab. 2). Their inhibitory effect was maintained at all evaluated concentrations and moments of assessment.

Table 2. Percentage of inhibition of M. roreri mycelial growth in vitro on PDA medium amended with cocoa leachates at five concentrations. 

Treatment Concentration
1% 2% 5% 10% 15%
Sterilized leachates by autoclaving -0.830±0.1 c 0.538±1.0 c 0.202±0.4 c 8.029±1.4 b 100±0 a
Non-sterilized leachates 100±0 a 100±0 a 100±0 a 100±0 a 100±0 a
Filtered leachates 2.667±0.3 a -0.734±0.9 a -4.036±0.5 a -4.671±1.4 a -0.621±0 a

The data represent the mean value of seven Petri dishes (n=7) for non-sterilized and sterilized leachates and five Petri dishes (n=5) for filtered leachates. Letters refer to significant differences between rows according to Tukey's test (P≤0.05). Mean values ± standard errors are presented.

Autoclave-sterilized leachates were effective in inhibiting mycelial growth of M. roreri only at the 15% dose with a 100% inhibitory effect (P<0.000), while the 10% dose showed an inhibition percentage of 8.03% (P<0.000). The doses of 1, 2, and 5% did not significantly inhibit the growth of the pathogen (P>0.975).

Filter-sterilized leachates were not effective in inhibiting the mycelial growth of M. roreri (P>0.428) and the doses of 2, 5, 10 and 15% even generated an increase in M. roreri growth.

Effect of cocoa leachates on the germination of M. roreri conidia

Non-sterilized cocoa leachates inhibited the conidial germination of the pathogen at all the concentrations evaluated (P<0.000), while the control showed germination percentages between 6 and 27% (Fig. 2A). These results were consistent with additional experiments conducted with other cocoa leachate samples in which 100% inhibitory effect was obtained on the germination of M. roreri conidia (data not shown).

Sterilized cocoa leachates showed a significant effect on conidial germination at concentrations of 10 and 15% (P<0.001 and P<0.000). At the 10% concentration, conidial germination was between 2 and 12%, while the control showed values between 6 and 37%. At the 15% concentration, conidial germination was less than 2% at 24 h after incubation without germination at 48 h. The lowest concentrations (1, 2, and 5%) did not show differences compared to the control (Fig. 2B). In additional experiments conducted with other cocoa leachate samples, the conidial germination was 15.2% for the concentration of 10%. At the 15% concentration, conidial germination was 0% at 24 h after incubation (data not shown).

Figure 2. Effect of cocoa leachates on the germination of M. roreri conidia 24, 48, 72 and 96 hours after incubation (HAI) under five concentrations of cocoa leachates and three methods of incorporation into the Water Agar culture medium incubated at 25 ºC. A. Non-sterilized cocoa leachates. B. Autoclave-sterilized cocoa leachates, and C. Filtered cocoa leachates. Each bar represents the mean of seven values±standard error (n=7) or five values±standard error (n=5) for autoclave-sterilized and filtered cocoa leachate respectively. Bars followed by different letters indicate significant differences according to Tukey's test (P≤0.05). 

On the other hand, filtered cocoa leachates showed an inhibitory effect on conidial germination with a germination percentage between 3 and 10% at concentrations of 5, 10 and 15% from 24 to 96 h after seeding. These results indicate an inhibitory activity, although at a lower proportion than that evidenced with non-sterilized leachates (Fig. 2C).

Effect of leachates on M. roreri inoculum production

Non-sterilized leachates at all the concentrations evaluated inhibited M. roreri conidia production (P<0.000); in this case, the mycelial inhibition of the pathogen was 100%, then no conidia production was registered. In contrast, the control produced an average of 10,000 conidia/cm2 of the colony. The same results were observed in additional experiments conducted with other cocoa leachate samples (data not shown).

Regarding sterilized leachates, a total inhibition in the production of inoculum was observed from the concentration of 10% (P<0.000). The concentrations of 1, 2 and 5% showed a lower inoculum production compared to the control, with values between 8.2·103 and 8.5·103 conidia/cm2, but without significant differences with the control treatment (1.1·104 conidia/cm2) (P>0.575) (Fig. 3). The absence of sporulation at the highest concentration of sterilized cocoa leachates (15%) was also observed in additional experiments conducted with other cocoa leachate samples. Therefore, the results confirm the effect of these concentrations on the reduction in the production of M. roreri inoculum.

Figure 3. Production of M. roreri inoculum under five concentrations of sterilized leachates on PDA culture medium incubated at 25 °C on day 14 after incubation. The data represent the mean of seven Petri dishes (n=7). Values with different letters indicate significant differences according to Tukey's test (P≤0.05). 

EC50 value for mycelial growth and conidia germination inhibition

The estimation of EC50 showed that the effective cocoa leachates concentration to reduce mycelial growth rate by 50% was 11.25% for the sterilized leachates, 0.974% for the non-sterilized leachates and 2.039% for the filtered leachates. The EC50 obtained for conidia germination inhibition assay was 10.25% for the sterilized leachates, 0.980% for the non-sterilized leachates, and 1.011% for the filtered leachates (Tab. 3).

Table 3. EC50 values (%) estimated using mycelial growth inhibition and conidia germination. 

Leachates Mycelial growth Conidia germination
EC50 SE EC50 SE
Sterilized 11.252 1.09 10.250 41.18
Non-sterilized 0.974 0.54 0.980 1.01
Filtered 2.039 0.46 1.011 0.11

The data represent the effective concentration values of cocoa leachates to reduce mycelial growth or conidia germination by 50% (EC50). EC50 and SE (standard error) values were obtained by fitting the mycelial growth or conidia germination rate against the log transformed cocoa leachate concentrations using the best fitting model (lLL.4).

DISCUSSION

The physicochemical and chromatographic analysis of cocoa leachates showed variation for the different evaluated parameters. In general, glucose and fructose showed higher concentrations in contrast to saccharose. The concentrations of citric and malic acids tended to be higher in comparison to those of ascorbic acid. Cl, NO3, Mg and K tended to show similar values between leachate samples, and PO4 and Ca showed a higher variation. Concerning the origin of the leachates, although variations were found among samples, a tendency to have similar concentrations was observed in the leachates obtained from the same farm at different times. S1 and S3 (Floresta) showed contrast with S2 (Filadelfia) regarding the contents of fructose, saccharose, ascorbic and citric acids, glucose, Na, EC, Cl, SO4, Ca and K; glucose concentration was higher in S2 leachates.

Pacheco-Montealegre et al. (2020) stated that the fermentation process in cacao varies depending on the environmental conditions, fermentation protocol of the farm and genetics of the plant material, among others. Therefore, the content variations observed in the leachates assessed in this study, regardless of the similarities between both farms, may be due to factors found by Pacheco-Montealegre et al. (2020) in their study. Despite the variation observed, according to our results, the effect of the leachates on the in vitro growth of M. roreri seems not to depend on the content variations but on the compounds (fructose, saccharose, glucose, ascorbic and citric acids, glucose, Na, EC, Cl, SO4, Ca and K) present in the liquid products. These compounds were the same in the three leachate samples evaluated in this study. The observed inhibition of M. roreri may be not only related to the presence of the compounds mentioned above but also to the microbiological composition of the leachates. The high percentage (100%) of inhibition of the pathogen obtained with non-sterilized leachates at the five concentrations and the low effect observed with sterilized leachates by autoclaving and filtered leachates indicate that both, chemical and microbiological compositions of the cacao leachates may play a role in the inhibition of M. roreri.

The antifungal activity of some types of leachates has been previously reported by authors such as Özer et al. (2002), who demonstrated that leachates from composted alfalfa and sunflower stalks inhibit the production of pectolytic enzymes and isoenzymes of Aspergillus niger in treated onion seeds. Huang et al. (2012) and Yang et al. (2015), using in vitro analyses, demonstrated that aqueous leachates and volatile compounds produced by Chinese leek (Allium tuberosum) inhibit the growth of Fusarium oxysporum f. sp. cubense race 4 (Foc TR4), conidia proliferation and germination, and the activity of cell wall-degrading enzymes produced by the fungus.

The inhibitory activity of cocoa leachates on the germination of M. roreri propagules observed in this study showed a similar effect to that reported by Mogollón and Castaño-Zapata (2010), who obtained a total inhibition of conidial germination of the pathogen when using banana rachis leachates at concentrations of 90% for the in vitro control of Paracercospora fijiensis (Morelet) Deighton. In this study, non-sterilized cocoa leachates showed an inhibitory effect on conidial germination from a concentration of 1%. This could suggest variable effectiveness of leachate concentrations depending on the plant species these leachates are obtained from and the target pathogen.

Banana rachis leachates have been used in foliar sprays for the control of fungal diseases in plants. Álvarez et al. (2001) mention that applications of 5% fulvic acid from banana leachates have generated a decrease in the severity of powdery mildew in roses caused by Sphaerotheca pannosa. Arenas et al. (2004) report the use of fulvic acid for the control of Mycosphaerella fijensis and Ralstonia solanacearum Race 2 (causal agent of banana moko disease), achieving reductions of 31.6% in the incidence of the disease. In this study, an inhibitory effect on M. roreri of 100% (Tab. 1) was generated from the lowest concentration of non-sterilized cocoa leachates, while an inhibitory effect of 8.0% on the radial growth of M. roreri was observed from the concentration of 10% in the sterilized leachates. This suggests that compounds in cocoa leachates like ascorbic and citric acids may contribute to the inhibition of the pathogen through mechanisms that need to be evaluated in subsequent studies. Recent studies have reported the fungicidal and bactericidal effect of citric acid, which was shown to inhibit growth of bacteria Shigella sp. (In et al., 2013), and phytopathogenic fungi Colletotrichum sp., the causal agent of anthracnose of cucumber and gourds (Kang et al., 2003; Morgunov et al., 2017). Additionally, exogenous applications of ascorbic acid have been found to induce disease resistance in some pathosystems (Boubakri, 2017). The application of ascorbic acid along with jasmonic acid enhanced the accumulation of phytoalexins in rice, and ascorbic acid alone induced resistance against Huanglongbing in citrus plants (Li et al., 2016). The application of derivative compounds of ascorbic acid induced resistance against Turnip mosaic virus in turnip (Fujiwara et al., 2013). Ascorbic acid has also been found to be active against fungal pathogens such as the rice blast fungus Magnaporthe oryzae, which decreased the percentage of normal appressorium formation after treatment with this acid (Egan et al., 2007). Both ascorbic and citric acids were found to be present in the cocoa leachates evaluated, which can suggest a possible effect of these compounds on the inhibition of M. roreri.

The high effectiveness of non-sterilized cocoa leachates that completely inhibited radial growth and conidial germination of M. roreri can be explained based on results of previous studies conducted with leachates from different plant species. In cocoa, microbial communities in the fermentation process are mainly Enterobacteriaceae related bacteria, Lactic Acid Bacteria, Acid Acetic Bacteria and yeasts (Camu et al., 2007; Okiyama et al., 2017; Pacheco-Montealegre et al., 2020). Ceballos et al. (2012) found that during the fermentation processes to obtain leachates from banana rachis, many microorganisms are present in these substances and are responsible for the segregation of numerous secondary metabolites that can act as biocides on other microorganisms. Bacteria involved in fermentation processes such as Bacillus subtilis and B. amyloliquefaciens can produce metabolites (chitinolytic and glucanolytic enzymes) that alter the structure of the mycelium cell wall and fungal ascospores, inhibiting the development of pathogenic microorganisms under in vitro conditions (Ceballos et al., 2012). Ouattara et al. (2011) reported that Bacillus strains are involved in the production of pectinolytic enzymes during cocoa fermentation. They identified six species of Bacillus, including Bacillus subtilis. Cocoa fermentation microbiota also vary according to the geographic area, but most of the Bacillus strains have been reported as constituents of cocoa fermentation microbiota in Brazil (Schwan et al., 1986), Trinidad (Ostovar and Keeney, 1973) and Ghana (Carr et al., 1979; Nielsen et al., 2007). This could suggest that the combined action of microorganisms and substances (citric and ascorbic acids found in our samples) present in non-sterilized cocoa leachates increases the effectiveness of the compound to inhibit M. roreri compared to sterilized cocoa leachates. Nevertheless, bacterial species with antifungal effects that are present in the cocoa fermentation process have to be determined in further studies.

In addition to the above, authors such as Garcia-Armisen et al. (2010) detected bacteria of the genera Tatumella, Pantoea, and Erwinia during the fermentation process. Although some of these genera may be plant pathogens, these authors think they may contribute to citrate consumption since they are microorganisms that compete against other plant pathogens for space and nutrients. The analysis conducted by Pacheco-Montealegre et al. (2020) also showed that bacteria of these genera may be present in the cacao fermentation process. Additionally, Viesser et al. (2021) reported three major microbial groups in the cocoa fermentation process: lactic acid bacteria, acetic acid bacteria, and yeasts. These authors found that B. subtilis strains present in the cocoa fermentation process were associated with the production of pectinase and secondary metabolites such as lactic and acetic acids. Although we did not measure the acetic acid in our leachate samples, this compound has been reported as a key component for an efficient fermentation of cocoa beans (Soumahoro et al.,2020). Also, acetic acid is recognized for its antifungal and antibacterial properties, and has been applied for control of plant pathogens, such as seed-borne fungi (Dorna et al., 2021). This could explain the greater inhibitory effect of non-sterilized cocoa leachates on M. roreri, which can result from the combined action of microorganisms and compounds typically found in the leachates such as acetic acid.

The inhibitory effect of the filtered leachates on M. roreri was not observed during the test. From the 2% concentration, the leachates even contributed to the growth of the fungus at percentages between 0.6 and 4.7%. This could be due to the elimination of microorganisms that compete with the pathogen for space and nutrients, thus limiting its growth. Filter sterilization can eliminate microorganisms producing compounds with the potential to control M. roreri, reducing the control effect of leachates. On the other hand, an inhibitory effect of the filtered leachates was not observed at concentrations of 10 and 15%, as observed in the sterilized leachates. Although the heating at high temperatures of certain substances in the leachates eliminates important microorganisms, it may also generate some chemical reaction in their compounds that contributes to maintaining their capacity to control M. roreri. The degradation or oxidation of products such as ascorbic acid at heating temperatures of 100ºC was reported to produce compounds such as furfural, 2-furoic acid, and 3-hydroxy-2-pyrone (Yin et al., 2022). Among these products, furfural is the main degradation product of ascorbic acid. This compound is reported as a very effective fungicide and it was found that as little as 0.5% furfural is sufficient to entirely prevent the growth of the mold Penicillium. Furfural was observed to be particularly effective in inhibiting the growth of wheat smut (Tilletisfoetens) (Zeitsch, 2000). Similarly, furfural from pine needle extract was shown to inhibit the growth of Alternaria mali the causal agent of Alternaria blotch of apple. The authors of that study mention that although furfural itself can not be completely substituted for an antifungal agrochemical, a partial mixture of furfural and antifungal agrochemical is effective as a fungicide (Jung et al., 2007).

Studies conducted to evaluate the microbial composition associated to the cocoa fermentation in different cocoa production areas in Asia, Africa, South America (Ecuador and Colombia) and Central America (Mexico) have reported bacteria in the families Enterobacteriaceae, Lactobacillaceae and Acetobacteraceae and yeast as such as Hanseniaspora opuntiae, Picha sp., Pichia kudriavzevi, and Wickerhamomyces pijperi (Ardhana and Fleet, 2003; Garcia-Armisen et al., 2010; Papalexandratou et al., 2011; Papalexandratou et al., 2013; Arana-Sánchez et al., 2015; Pereira et al., 2016; Pacheco-Montealegre et al., 2020). Therefore, it is highly probable that the bacteria and yeast present in the cacao leachates used in this study belong to these taxonomic groups.

Pacheco-Montealegre et al. (2020) stated that the dynamics of microbial fermentation in cacao vary between farms, protocols used and time of the process that changes the bacterial composition during fermentation. Nevertheless, our study evaluated cacao leachates at 24 h of the addition of fresh harvested seeds of similar genetic plant material. Additionally, the fermentation process was conducted following similar procedures at the farm level and under comparable environmental conditions. In this sense, the obtained results in terms of the effects of the leachates on the in vitro growth of M. roreri seem to be more influenced by the leachates condition (filtered, sterile or non-sterile) than by their source of origin. This, despite the variation observed in the chemical composition of the leachates between farms. Our results may be explained by the findings reported by Pacheco-Montealegre et al. (2020) who showed that, although there is heterogeneity in the microbial transitions in the cacao fermentation process from a general perspective, the functional groups present over time may be predictable. Those microorganisms potentially involved in the in vitro control of M. roreri may belong to these groups.

Banana leachates have been reported to be a mixture of humic and non-humic substances. Within the non-humic substances, we can find compounds such as sugars, amino acids, polysaccharides, and proteins, whereas the mixture of different macromolecular complexes is reported within the humic substances (Arenas et al., 2004; Álvarez et al., 2015). Additionally, the use of plant leachates involves the action of microorganisms in charge of microbial decomposition and the production of natural compounds that act as factors inhibiting the pathogen, since they prevent the germination of conidia and the penetration of potential fungal pathogens (Arenas et al., 2004; Özer and Köycü, 2006). The inhibitory effect of leachates can be attributed to the action of biochemical compounds with antimicrobial effects such as phenolic acids, saponins, essential oils, naphthoquinones, and terpenoids. It can also be attributed to direct antagonism due to antibiosis, parasitism, or competition (for space or nutrients) (Mainer, 2009; Bubici et al., 2019). This suggests that certain acids present in leachates, such as citric acid and ascorbic acid, that were found in cocoa leachates during this study, may exert a control activity on fungal pathogens as previously demonstrated in research analysis conducted on some pathosystems. Therefore, future studies should analyze the control potential of this type of compound.

The use of cocoa leachates as a method to control M. roreri could be a great advantage for the farmer since it is a product generated naturally by the transformation processes of cocoa beans on the farm. Additionally, leachates, especially without sterilization, are natural products that exert effective control of the pathogen from low concentrations. However, it is necessary to carry out more studies to confirm that the microorganisms present in leachates do not represent a risk for human consumption and can be safely applied to cocoa fruits. It is important to note that this is the first study to evaluate the activity of cocoa leachates for the in vitro control of M. roreri. For this reason, the results obtained were contrasted and discussed with studies carried out with leachates from other vegetable species. Therefore, further studies must deepen in the compounds and microbiological composition of cacao leachates that may be involved in the inhibition of M. roreri. Additionally, it is necessary to conduct research that confirms the effect on the pathogen found, but using cacao leachates obtained under variable fermentation procedures at the farm level.

CONCLUSIONS

The cocoa leachates showed variation for the different evaluated parameters. The effect of the leachates on the in vitro growth of M. roreri seems not to depend on the content variations but on the compounds present in the liquid products. The highest inhibition of M. roreri radial growth and conidial germination was obtained with non-sterilized leachates at all concentrations evaluated, and with autoclave-sterilized leachates at concentrations of 10 and 15%. The antifungal ability of non-sterilized cocoa leachates from low concentrations can be attributed to the combined action of the compounds and microorganisms present in the substance. The inhibitory effect on M. roreri of sterilized cocoa leachates is possibly attributed to specific compounds such as citric and ascorbic acids. The antifungal activity of these acids has been reported in the literature and these compounds were found in the cocoa leachates using chromatographic tests. The filtered leachates proved not to be an efficient method for the in vitro control of M. roreri in comparison with the other two leachates evaluated. The results obtained in this study show the control potential of cocoa leachates on M. roreri in vitro, which is a limiting pathogen of the crop. This suggests that further studies are required to clarify the microbiological and chemical effects and composition of the cocoa leachates. Additionally, in vivo evaluation needs to be conducted to confirm cocoa leachates as an alternative for commercial cacao crops.

Acknowledgments

The authors would like to thank Universidad Nacional de Colombia for providing the equipment and resources, and funding the research through the project “Mejoramiento de la tecnología de producción de cacao en las provincias de Rionegro y Alto Magdalena, Cundinamarca” within the frame of “Corredor Tecnológico Agroindustrial - Bogotá Cundinamarca. Derivado 2”. They are also grateful to “Federación Nacional de Cacaoteros - FEDECACAO” for supporting the researchers in the study area, and all the farmers from the municipality of Yacopi for their cooperation.

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Received: March 01, 2022; Revised: April 20, 2022; Accepted: August 19, 2022

3 Corresponding author. svgomezg@unal.edu.co

Author’s contributions

All authors contributed to the study conceptualization. Material preparation and methodology design were performed by SVGG, SGC and CBA. Data collection and analysis was conducted by SVGG. The first draft of the manuscript was written by SVGG and all authors commented on previous versions of the manuscript approving its final version. Funding of this research was acquired by SGC and CBA.

Conflict of interest: On behalf of all authors, the corresponding author states that there is no conflict of interest.

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