Hongos filamentosos eliminan hidrocarburos intemperizados de suelos tropicales mexicanos

Beatriz PÉREZ–ARMENDÁRIZ^1,2*, Daniel MARTÍNEZ–CARRERA³, María CALIXTO–MOSQUEDA^1,4, Joel ALBA ¹ and Refugio RODRÍGUEZ–VÁZQUEZ¹

¹ Laboratorio de Compuestos Xenobióticos, Departamento de Biotecnología y Bioingeniería, Centro de Investigación y de Estudios Avanzados, Instituto Politécnico Nacional, Av. Instituto Politécnico Nacional 2508, San Pedro Zacatenco, Delegación Gustavo A. Madero, México, D. F. 07360.

² Centro Interdisciplinario de Posgrados, Investigación y Consultoría, Universidad Popular Autónoma del Estado de Puebla, 21 Sur 1103 Col. Santiago. CP 72160, Puebla, México. (+52) 222–229 94 00 ext 7527. beatriz_pereztij@yahoo.com.mx.

³ Biotecnología de Hongos Comestibles, Colegio de Postgraduados en Ciencias Agrícolas (COLPOS), Campus Puebla, Apartado Postal 701, Puebla 72001, Puebla, Mexico.

⁴ Departamento de Bioprocesos, Unidad Profesional Interdisciplinaria de Biotecnología, Instituto Politécnico Nacional, Av. Acueducto s/n, México, D.F. 07340.

Recibido junio 2009
Aceptado enero 2010

ABSTRACT

Weathered hydrocarbons from worldwide petrolic activities become more recalcitrant over time. The removal of petroleum hydrocarbons from a polluted soil [65,000 mg total petroleum hydrocarbons (TPH)/kg soil], which had been exposed to tropical environmental conditions for more than 20 years in southeast Mexico, was studied using filamentous fungi. Experiments were carried out in batch reactors (60 mL) containing a substrate consisting of polluted soil and sugar cane bagasse pith as bulk agent (80:20, w/w). Sterile and non–sterile batch reactors were inoculated with spore suspensions from Aspergillus niger, Penicillium glabrum, and Cladosporium cladosporioides. The TPH were determined at the beginning and at the end of the experiments, and the CO₂ production and accumulation were monitored by gas chromatography. All fungal species studied were associated to the removal of TPH, either on sterile or non–sterile treatments. A bioaugmentation process was observed due to the synergistic effect of C. cladosporioides and well–adapted indigenous microbial populations from the contaminated soil, as the highest removal of TPH (78.5%) and CO₂ accumulation (14.3%) were recorded in this non–sterile treatment. By contrast, the lowest TPH removal was recorded in the same species, but in the sterile treatment (62.3%) showing that the absence of adapted indigenous microbiota significantly reduced fungal metabolism (CO₂ accumulation: 9.1%), as well as the removal of TPH. Patterns of CO₂ accumulation and TPH removal in other treatments suggested interspecific competence between fungal species and the adapted indigenous microbiota.

Key words: Aspergillus, bioaugmentation, Cladosporium, filamentous fungi, Penicillium, total petroleum hydrocarbons (TPH) removal, tropical Mexico.

RESUMEN

Palabras clave: Aspergillus, bioaumentación, Cladosporium, hongos filamentosos, Penicillium, remoción de hidrocarburos totales del petroleo (HTP), trópico mexicano.

INTRODUCTION

Petrolic activities have generated extensive pollution of soils worldwide, mainly in those regions where petroleum is explored, extracted, and refined. The composition of hydrocarbons on polluted soil varies according to environmental conditions and natural degradation processes. Weathered hydrocarbons, which are predominantly saturated and aromatic, become more recalcitrant if polluted soils are not remediated, affecting underground water, food chains, and diverse human activities (e.g., agriculture, cattle raising, silviculture) (Atlas and Bartha 1998).

Bacteria and fungi have been used for degradation and removal of hydrocarbons, as they are capable of producing significant amounts of efficient enzymes (Saraswathy and Hallberg 2002, Chávez–Gómez et al. 2003, Moody et al. 2004, Genovese et al. 2008). Filamentous fungi, commonly found on lignocellulosic substrates, produce extracellular enzymes of low specificity, which can degrade differing recalcitrant compounds, such as hydrocarbons, resins and asphaltens (Tortella et al. 2005). Important enzymes used for bioremediation are lignin peroxidase, manganese–dependent peroxidase, and laccase (Evans and Hedger 2001).

Most fungal research work on bioremediation has been focused on the degradation of specific hydrocarbons using a variety of substrates, showing different levels of pollutant removal (Hammel et al. 1986, Gramss et al. 1999, Novotny et al. 1999, Cortés–Espinosa et al. 2006, Leonardi et al. 2007, Genovese et al. 2008). Mineralization rates by fungal enzymes ranging from 25–93% have been reported for polycyclic aromatic hydrocarbons (PAH) during a period of 8–15 weeks. In a previous research work, it was shown that the removal of weathered hydrocarbons from polluted soil can be improved synergistically by microorganisms from sugar cane bagasse pith, reaching up to 60% removal of total petroleum hydrocarbons (TPH) (Pérez–Armendáriz et al. 2004). In this study, it was assessed the effect of bioaugmentation using three species of filamentous fungi on the removal of hydrocarbons from real polluted soil exposed to tropical environmental conditions for more than 20 years in the State of Tabasco, southeast México.

MATERIALS AND METHODS

Fungal strains

Batch reactors

A soil sample was obtained from a petroleum well located in the tropical State of Tabasco, southeast of México. The soil sample (ca. 20 kg) was placed in a dark glass container and kept at 4 °C for transportation. In the laboratory, the soil was exposed to the sun for a few hours, homogenized manually for 15 min, and characterized as loamy sand (silt 4 %, sand 96 %) having a moisture content of 2 %, an organic matter content of 8.3 %, and a pH of 7.3. The concentration of total petroleum hydrocarbons (TPH) in the polluted soil was of 65 000 mg/kg, as the well from which the sample was taken had been exposed to diesel contamination for more than 20 years. Sugar cane bagasse pith (a lignocellulosic byproduct from the local sugar industry) was sterilized at 121 °C for 20 min and it was used as solid support and carbon source in all experiments. This pith was characterized as follows: pH 4.5, density 0.8 g/cm³, moisture content 80 %, total sugars 2.23 mg glucose/g (Rodríguez–Vázquez et al. 1999). Six different treatments were carried out as shown in table I. A non–sterile soil sample was used directly for part of the experiment, whereas the soil sample used in the other experimental part was autoclaved three times (every 24 h) at 121 °C for 15 min, according to previous research (Pérez–Armendáriz et al. 2004, Cortés–Espinosa et al. 2006). Two controls, involving either sterile or non–sterile soil, were included. The batch reactors were glass serum bottles (60 ml) containing 16 g of soil, either sterile or non sterile, and 4 g of sterile sugar cane bagasse pith. The moisture content was adjusted to 60 %, using sterile distilled water. The C/N/P ratio was 100/10/1 using a sterile water solution of 1 N NH₄SO₄ (Sigma–Aldrich, USA) and 1 N K₂HPO₄ (Sigma–Aldrich, USA) as nitrogen and phosphorus sources. Fungal inocula from strains studied were prepared on PDA plates. Spores were harvested adding 2.5 ml of tween 80 (Sigma–Aldrich, USA) in order to obtain a sterile solution at a standardized concentration. Every reactor was inoculated with 1 mL of the spore suspension (inoculum at 2 x 10⁷ spores/mL). Each bottle was capped with a Teflon septum. The atmosphere of reactors was exchanged every two days, injecting an air flow through a sterile filter (millipore 0.2 mm) for 15 min. All experiments were carried out in triplicate. Residual TPH were determined after 25 days of incubation at 25 °C (Chávez–Gómez et al. 2003, Pérez–Armendáriz et al. 2004, Cortés–Espinosa et al. 2006).

Sample analysis

Microbial activity. It was monitored every two days, before each atmosphere exchange, taking an air sample of 5 µL from the headspace of batch reactors using a sterile syringe, which was injected into the gas chromatograph (Gow–Mac 580, USA) having a thermal conductivity detector. Data were expressed as percent of CO₂ produced and accumulated (Rodríguez–Vázquez et al. 1999).

Total petroleum hydrocarbons (TPH). The content of TPHs was determined in three samples at the beginning and at the end of the experiments, as previously described (Pérez–Armendáriz et al. 2004). Samples were taken for analysis at day 0 (initial soil sample) and at day 25. The total content of each batch reactor was homogenized by thorough manual mixing for 10 min. A sample (2 g) was taken from the mix, and dried at room temperature for 24 h. Hydrocarbons were extracted for 8 h with 80 mL of dichloromethane (Merck, USA) using Soxhlet. Dichloromethane phase was performed in a rotary evaporator, adding 2 g of anhydrous Na₂SO₄ (Sigma–Aldrich, USA). Dry samples were dissolved in 10 mL of dichloromethane, taking an aliquot of 500 µL to be dried at room temperature and dissolved in 5 mL of CCl₄ (Merck, USA). Residual hydrocarbons were determined following the modified EPA 418.1 method (USEPA 1979). Total petroleum hydrocarbons were assessed by infrared spectroscopy (Buck Scientific, model HC–404, USA), using 2930 cm^–1 absorbance, specific for C–H bonds. Samples were analyzed by interpolation in a calibration plot.

Statistical analysis

Data were expressed as means ± standard deviations. One way analysis of variance and F test, at a level of significance of P<0.05, were carried out in order to determine significant differences among the means. Multiple comparisons among treatment means were made using the Tukey's test. All data were analyzed on Minitab Ltd. statistic software.

RESULTS AND DISCUSSION

Very low levels of CO₂ production and accumulation (1.5 %), as well as TPH removal (16.0 %), in the sterile control T8 may be associated to the presence of reproductive structures from adapted indigenous microbiota capable of resisting sterilization processes, which also affect substrate (polluted soil + sugar cane bagasse pith) structure and composition (Sylvia et al. 1999).

The comparison of sterilized and non–sterilized treatments showed variation according to each species (Table II, Fig. 1). In the case of Aspergillus niger, the CO₂ accumulation (T2, 9.9 %) and the TPH removal (T2, 76.3 %) on the sterile treatment were higher than those on the non–sterile treatment containing adapted indigenous microbiota (T1: CO₂, 3.4 %; TPH, 64.6 %). Similar results were obtained in Penicillium glabrum for CO₂ accumulation and TPHs removal, which were higher on the sterile treatment (T4: CO₂, 8.9 %; TPH, 72.5 %). Higher values for CO₂ accumulation and TPH removal on sterile treatments suggested some degree of interspecific competence between filamentous fungi studied (A. niger, P. glabrum) and adapted indigenous microbiota. Competence has also been reported for Phanerochaete chrysosporium and indigenous microorganisms (Fernández–Sánchez et al. 2001). By contrast, the removal of TPHs on the non–sterile treatment containing Cladosporium cladosporioides and adapted indigenous microbiota (T5, 78.5 %) was higher than that on the sterile treatment (T6, 62.3 %). In this case, the CO₂ production and accumulation were also higher on the non–sterile treatment (T5, 14.3 %) than on the sterile treatment (T6, 9.1 %), which indicated the presence of interspecific co–metabolism between the filamentous fungus and adapted indigenous microbiota. Previous research has shown that a closely related species, Cladosporium sphaerospermum, which was isolated from aged soil of a gas manufacturing plant, was capable of degrading several PAH in four weeks using a non–sterile soil model (Potin et al. 2004). This ability to degrade hydrocarbons is due to the concerted action of extracellular and metabolic enzymes produced during Cladosporium growth.

An advantage of using experimental models based on real polluted soil is that the efficiency of a fungal species, such as A. niger, P. glabrum and C. cladosporioides, is directly tested against well–adapted indigenous microbial populations. This is in contrast with those species which are useful for bioremediation under laboratory conditions, but not efficient and poorly competitive under natural conditions where population development is affected by many factors, e.g., Phanerochaete chrysosporium (Lindley and Heydeman 1985, Meulenberg et al. 1997, Fernández–Sánchez et al. 2001, Potin et al. 2004). This research showed that A. niger, P. glabrum and C. cladosporioides are filamentous fungi with good potential for bioremediation processes in tropical regions of Latin America. They are capable of removing and degrading recalcitrant hydrocarbons through bioaugmentation and biostimulation, using sugar cane bagasse pith as bulking agent. However, they show differing responses when confronted with indigenous microbiota. Further studies are needed to understand the biological interactions between filamentous fungi and indigenous microbiota.

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