Enhancing methyl parathion degradation by the immobilization of Burkholderia sp. isolated from agricultural soils

Abstract Organophosphate pesticides are of great interest for research because they are currently the most commonly used pesticides. In this study, a bacterial strain capable of completely degrading methyl parathion (MP) was isolated from agricultural soils in central Mexico. This strain was designated strain S5‐2 and was identified as Burkholderia cenocepacia. To increase degradation yields, cells were immobilized on three different supports: powdered zeolite and Opuntia sp. and Agave sp. fibers. The results indicated a significant increase in MP hydrolysis and p‐nitrophenol (PNP) degradation with immobilized cells compared to free cell cultures. Furthermore, immobilized cells were capable of withstanding and degrading higher concentrations of PNP compared to cell suspension cultures. The cell viability in the free cell cultures, as well as PNP degradation, was affected at concentrations greater than 25 mg/L. In contrast, cells immobilized on Opuntia sp. and Agave sp. fibers completely degraded PNP at concentrations of 100 mg/L. To verify that MP solution toxicity was decreased by B. cenocepacia strain S5‐2 via pesticide degradation, we measured the acetylcholinesterase activity, both before and after treatment with bacteria. The results demonstrate that the activity of acetylcholinesterase was unaffected after MP degradation by bacteria.

these methods remain inefficient. For this reason, the use of microorganisms isolated from contaminated sites that can degrade the OPs has gained greater acceptance, particularly due to microorganisms' ability to perform complete mineralization of the pesticide without causing environmental damage.
Methyl parathion (O,O-dimethyl-O-4-p-nitrophenyl phosphorothioate) is an OP. In Mexico, MP is one of the most commonly used pesticides and has been used extensively for insect control with crops, including avocados, rice, onions, peaches, spinach, and strawberries. Although the use of MP is legal, its trade has recently been restricted (Torres, Ramos, Avila, & Ortiz, 2012), and it can be found in soil and water, as well as in waste. It is considered extremely dangerous and is included in the Ia Category of the World Health Organization (WHO, 2009). This pesticide poorly inhibits acetylcholinesterase activity; however, it is metabolically activated by cytochrome P 450 to produce oxons that are very potent inhibitors of this enzyme (Sultatos, 2006). Initially, interaction between the pesticide and enzyme is reversible, but over time, a process called "aging" occurs, which results in the formation of a covalent bond that is much more stable. This process results from the elimination of one of the alkyl side chains of the phosphate group, leaving the hydroxyl group, which avoids regeneration of the active site of the enzyme (Wilson, Colman, & Sutton, 2001).
The first report of a microorganism capable of degrading an organophosphorus compound dates from 1973, when the strain Flavobacterium sp. was isolated from a rice field in the Philippines (Sethunathan & Yoshida, 1973). This bacterium was subsequently reclassified as Sphingobium fuliginis by Kawahara, Tanaka, Yoon, and Yokota (2010). Although the hydrolytic activity of these bacteria on MP is high, their ability to degrade the PNP generated after MP hydrolysis is limited (Adhya, Barik, & Sethunathan, 1981). PNP is less toxic to animals than MP; however, it is resistant to degradation and is toxic to many microorganisms. There are multiple reports of microorganisms that can hydrolyze MP; however, PNP generated during the hydrolysis of MP may be a limiting factor in the development of biotechnological tools for pesticide degradation.
Therefore, a bacterium that can hydrolyze MP and simultaneously degrade PNP is a valuable tool for the biological treatment of MP waste and/or for the remediation of sites contaminated with this pesticide.
In this study, a bacterial strain that can completely degrade MP was isolated from agricultural soils. The cells were immobilized on Opuntia sp., Agave, and zeolite. These three supports are waste materials that are abundant in the region and can be used for biotechnological purposes. The results obtained using cells in suspension and immobilized in three different supports are reported. We also conducted different analyses to test the toxicity of the resulting solutions after treatment with the isolated bacteria.

| Isolation and selection of the strain
Soil samples were taken from a commercial cornfield in central Mexico (latitude 18° 58′26″ N and longitude 99° 07′05″ W). The soil was a vertisol type and was collected at 10 cm below the soil surface. Sterile Erlenmeyer flasks were used to store and transport samples at 4°C until isolation of the bacteria. After reaching the laboratory, soil samples were enriched with MP by adding aliquots every week for 30 days, reaching a concentration of 200 mg/L. The enriched soil samples were incubated in the dark at 30°C (Goda, Elsayed, Khodair, El-Sayed, & Mohamed, 2010). Subsequently, 1 g of each sample was collected and inoculated into 50 ml of MSM supplemented with MP (50 mg/L) and incubated for 7 days at 30°C at 140 rpm. An aliquot of the culture medium was used to inoculate another flask of fresh MSM with MP (50 mg/L), leaving it to grow for 7 days under the same conditions. After three subsequent repetitions, an aliquot of 100 μl was taken and seeded in Petri dishes with tryptone soy agar supplemented with 50 mg/L of the pesticide.
These were incubated at 30°C for the necessary time until bacterial colonies were visible.
The colonies that showed yellow halos around of them (indicative of MP hydrolysis to PNP) were selected. The selected strains were cultured in MSM supplemented with MP, and the production of PNP and its subsequent degradation was monitored spectrophotometrically at 410 nm. Those strains that could perform both processes (MP hydrolysis and PNP degradation) were selected. The strain that showed the greatest efficiency degradation of both MP and PNP was selected and this colony was labeled as S5-2.

| Characterization of the selected strain
The isolate was identified by biochemical tests (Voges-Proskauer, methyl red, motility-indole-ornithine, citrate Simons, catalase, and Gram stain) and 16S rRNA gene analysis. Genomic DNA extraction was performed using a kit from Axygen and this was used as substrate for the amplification of the 16S rRNA gene using the universal oligonucleotides L1041 5′-CGGTGTGTACAAGACCC-3′ and PROK63FW 5′-CAGGCCTAACACATGCAAGTC-3′ (Felske, Engelen, Nübel, & Backhaus, 1996). The amplification products were purified using the High Pure PCR Product Purification (Roche) kit, and they were subsequently sequenced and compared with GenBank sequences.

| Inoculum
The selected strain was inoculated into the tryptone soy broth supplemented with MP to a final concentration of 50 mg/L for 18 hr at 30°C with agitation at 120 rpm. Subsequently, the biomass was collected by centrifugation and washed twice with a sterile solution of 0.8% NaCl (w/v) and resuspended in the same solution. This suspension was adjusted to an optical density of approximately 0.5 at 600 nm and the resulting suspension was used as an inoculum for MP degradation tests. In all experiments, 1% v/v inoculum was added to the culture medium and MP to a concentration of 50 mg/L.

| Growth and degradation kinetics using free cells
For free cell cultures, growth and degradation kinetics were assessed.
Sterile Erlenmeyer flasks of 125 ml were supplemented with MSM and MP at a final concentration of 50 mg/L. A 1% (v/v) inoculum with biomass prepared as described above was added. All flasks were incubated on a shaking platform for 24 hr at 120 rpm and 30°C. The removal of MP, generation and subsequent PNP degradation, and the growth of bacteria by viable count were measured immediately after inoculation and at different time intervals. MSM with MP and without inoculum and MSM with inoculum and without MP were used as controls. All treatments were performed in triplicate.

| Material used as a support for cell immobilization
For cell immobilization, the following materials were used as supports:

| Opuntia sp. fibers
Opuntia sp. is a genus belonging to the Cactaceae family, growing in fields throughout central and northern Mexico and the southwestern United States. The plant material was collected in the central region of Mexico and was left to dry after collection. A porous, strong structure that makes it favorable for cell immobilization is then formed. These dry leaves of Opuntia sp. were cut into small pieces (approximately 2 cm 2 ), washed with water, and dried in the oven at 50°C. The composition (%) of the Opuntia sp. fibers is as follows: structural carbohydrates, 36.3 ± 1.1; cellulose, 13.1 ± 0.7; hemicellulose, 18.5 ± 0.7; lignin, 12.3 ± 1.1; protein, 7.4 ± 0.3; extractives, 25 ± 0.9; and ash, 23.7 ± 0.1 (Yang et al., 2015).

| Agave sp. fibers
Agave sp. is a plant widely used in Mexico for tequila production. During tequila production, the leaves of the plant are discarded and large amounts of waste-like fibers are generated. These fibers are highly resistant and can be used for cell immobilization. Agave sp. fibers were autoclaved at 121°C for 15 min. Next, the fibers were macerated to separate the fibers and washed with water. The fibers were left overnight in acetone, washed with water, and allowed to dry in an oven at 50°C. The composition (%) of Agave sp. fibers is as follows: structural carbohydrates, 43.8 ± 1.3; cellulose, 26.0 ± 1.2; hemicellulose, 22.8 ± 1.2; lignin 13.8 ± 1.3; protein, 2.4 ± 0.1; extractives, 29.0 ± 1.2; and ash, 6.0 ± 0.1 (Yang et al., 2015).

| Powdered zeolite
Zeolites are microporous crystalline solids with well-defined structures and shape-selective properties. They are widely used in molecular adsorption (Datta, Christena, & Rajaram, 2012) as well as in adsorption and separation processes, environmental pollution control, petrochemical processes, fine chemical synthesis, biochemistry for the synthesis of nanocomposite materials, and cell immobilization (Tope, Srinivas, Kulkarni, & Jamil, 2001). Among a wide range of adsorbents available, the unique physical and chemical properties of natural zeolites, particularly their high porosity and large surface area, have made them useful for the immobilization of microorganisms (Shindo, Takata, Taguchi, & Yoshimura, 2001).
The zeolite used in this study is the waste of an industrial process in which it is used as a carrier for the manufacture of food supplements. This material is ground and sieved in a 500 mesh, resulting in particles with a size of approximately 25 microns, which provides a large surface area. The X-ray analysis revealed the following elemental composition (%): C,9.23;O,44.87;Na,3.48;Al,6.15;Si,32.18;and Cl,4.09. Before being introduced into the flasks for cell immobilization, the zeolite was washed with abundant distilled water.

| Growth and degradation kinetics using immobilized cells
Supports were added at 2% (w/v) to tryptone soy broth medium and sterilized by autoclaving for 15 min at 121°C twice with an intermediate repose of 24 hr. Next, the media was inoculated with the S5-2 strain and incubated for 24 hr at 30°C and 100 rpm to allow colonization of the bacteria on the supports. We next proceeded to wash the supports twice with 0.8% NaCl solution (w/v) to eliminate free cells by centrifugation at low speed (1250 g for 5 min). The mineral medium described above supplemented with MP as a carbon source was added to the supports. To measure the MP and PNP concentrations, samples at regular intervals were taken and analyzed by HPLC.
To evaluate bacterial survival immobilized on the supports, the viable count was determined for each treatment, collecting samples weekly for 21 days. The results are reported as CFU/g support . We also report the percentage of survival of bacteria, which was calculated from the CFU/g support values obtained at the end of the kinetics, with respect to the initial values.
To desorb the pesticide adsorbed by the zeolite, Opuntia sp., and Agave sp., the uninoculated controls (MSM with MP) were used.
After 24 hr incubation, the MSM was removed and the supports were washed twice with 0.8% NaCl solution (w/v). After that, ethyl acetate was added to the supports and they were shaken at 250 rpm for 1 hr.
Then, they were sonicated for 30 min and 1 ml of the supernatant was removed and dried. Samples were suspended in a methanol-water mixture and analyzed by HPLC.

| Toxicity tests
Toxicity tests were performed in two ways to evaluate distinct aspects of PNP effects at different levels. It has been reported that PNP causes acute toxicity to biological systems (Bhushan, Chauhan, Samanta, & Jain, 2000), so we decided to test its effect on the growth of the strain at several PNP concentrations using free and immobilized cells. It is also well documented that organophosphate pesticides inhibit the activity of acetylcholinesterase, and for this reason, we measured the activity of this enzyme before and after treatment of media containing MP.

| Toxicity test of PNP on the isolated strain
To measure the PNP effect on the isolated strain, the same methodology described in the previous section was followed; however, the MP was replaced by PNP and different concentrations were tested (25, 50, 100, 200, and 300 mg/L). Viability was measured by counting viable cells and PNP concentration measurement at the initial time and 24 hr after incubation.

| Acetylcholinesterase inhibition by MP added to the culture media before and after treatment with the isolated strain
To determine whether treatment with the bacterial strain reduces acetylcholinesterase inhibition by methyl parathion, we measured the acetylcholinesterase activity both before and after pesticide treatment. This measurement was performed according to the methodology developed by Ellman, Courtney, Andres, and Featherstone (1961) with several modifications. The S9 fraction of rat liver was added to the reaction mixture to oxidize the MP by cytochrome P 450 and thus become the oxon derivative active on acetylcholinesterase (Sultatos, 2006). To use this fraction, a primarily S9 mixture was prepared as follows: distilled water, 375 μl; phosphate buffer 0.2 mol/L, 500 μl; glucose-6-phosphate 1 M, 5 μl; NADP 0.1 mol/L, 40 μl; KCl 1.65 mol/L, 20 μl; MgCl 2 0.4 mol/L, 20 μl; and S9 fraction of rat liver, 40 μl (Ames, McCann, & Yamasaki, 1975).
A volume of 475 μl of MSM with pesticide, before and after each treatment, was mixed with 15 μl of an acetylcholinesterase solution (5 U/ml) and 500 μl of S9 mixture. Next, the mixture was incubated at

| Analytical methods
To quantify the MP and PNP concentration, 1 ml of sample from each flask was collected at different time intervals and extracted with 1 ml of ethyl acetate. The organic phase was recovered and filtered through a glass funnel packed with glass wool and anhydrous sodium sulfate.
The extract was collected in amber vials and the procedure was repeated three times by adding 1 ml of ethyl acetate each time, then mixing and recovering the organic phase (Ortiz-Hernández & Sánchez-Salinas, 2010). Finally, the contents of the vials were allowed to dry and 1 ml of 50% HPLC grade methanol was added. Samples were analyzed by HPLC on a C18 column (3.5 μm; 4.6 × 100 mm, Waters, Model XTerra ® MS), with a flow rate of 0.8 ml/min in a 60:40 methanol-water system, at 30°C, and readings were recorded at 270 nm.

| Preparation of immobilizing material for observation in a scanning electron microscope
Cell immobilization was confirmed by scanning electron microscopy field emission (Hitachi S-5500). The material used for immobilization was dried for 48 hr at 70°C. Samples were observed directly on the microscope.

| Statistical analysis
The final concentrations of removed MP were transformed using an angular transformation (arcsine) and were analyzed using the general linear models procedure (SAS, PROC GLM) as an analysis of variance.
Post hoc analysis of differences in means was conducted with the Tukey's test (α = 0.05).

| Isolation and identification of S5-2 strain
In this study, it was possible to isolate a strain, designated S5-2, that was capable of hydrolyzing MP, and using PNP as a sole carbon source for growth in the mineral medium. This strain is a Gram-negative bacillus, with responses in the biochemical tests that were negative for methyl

| Growth kinetics and pesticide degradation in suspension cultures
Growth kinetics and pesticide degradation in suspension cultures showed that MP was completely hydrolyzed during the first 6 hr of culture ( Figure 1). The PNP concentration in the culture medium increased while MP hydrolysis occurred, and its higher concentration occurred when the entire MP added to the medium was hydrolyzed.
Subsequently, the newly formed PNP concentration decreased to zero.
Biomass growth was associated with the degradation of PNP, suggesting that cells used this compound as a source of carbon and energy.

| Pesticide degradation kinetics with immobilized cells
At the beginning of the degradation tests with immobilized cells, the biomass was 600 × 10 6 CFU/g support for Opuntia sp., 730 × 10 6 CFU/g support for Agave sp., and 99 × 10 6 CFU/g support for zeolite. Each treatment with immobilized cells showed similar behavior in the degradation process and they were superior to suspension cultures. Complete removal of MP was achieved in less than 1 hr, and the PNP degradation generated during the hydrolysis occurred in less time compared to cell-free cultures. By contrast, when the MP was in contact with the materials used as a support, without immobilized cells, the MP concentration in the culture medium decreased, likely due to a MP adsorption process on the fibers used ( Figure 2).
Our results show that after the MP is added to the culture medium with the respective fibers used, this compound is adsorbed into the fibers between 50% and 70% and the remainder of the MP remains in the culture medium, which is hydrolyzed by bacteria. It is necessary to clarify that in this experiment, the PNP was not added to the culture medium; therefore, this compound is not generated due to the absence of the strain (Figure 2). To verify the MP desorption of the fibers, however, we found that the adsorbed amount corresponds to 12.4% and 29.1% of the pesticide with respect to its initial concentration in supports Opuntia and Agave, respectively. Although not all the pesticide was desorbed by the method proposed, the results show that PNP is not generated, indicating no abiotic degradation of the pesticide. Therefore, the removal of the MP in the culture medium occurs via a combined action between its adsorption on the supports and degradation in the culture medium by the strain.
To evaluate strain stability, viability for each treatment was determined for 21 days. The results showed a significant decrease in survival for the cells immobilized on powdered zeolite. For Opuntia sp. and Agave sp. fibers, there was no significant loss of viability (Figure 3).

| Evidence of immobilization by scanning electron microscopy
The bacterial ability for biofilm formation on surfaces is a very useful tool for biotechnology. To confirm that the Burkholderia sp. strain S5-2 can support colonization, scanning electron microscopy of the three supports used in this paper was performed. The results showed that bacteria are trapped on the surface of Opuntia sp. and Agave sp. fibers after incubation for 24 hr. In zeolite, unimmobilized cells on the surface were observed (Figure 4).  fibers with the immobilized cells were incubated with different concentrations of PNP, a decrease between 60% and 80% of immobilized cells was observed compared to values reported at the beginning of the experiment ( Figure 5c); however, all the PNP is degraded at a concentration of 100 mg/L. The amount of immobilized cells on zeolite was lower compared to supports of vegetable origin, but the PNP was degraded up to a concentration of 50 mg/L; concentrations above this limit cause a decrease in viability and degradation (Figure 5d).

| Acetylcholinesterase inhibition by culture media before and after treatment with the isolated strain
To assess the MP toxicity before and after treatment with the isolated strain, the acetylcholinesterase residual activity was measured at different time intervals. Free or immobilized cells of the strain were cultured in MSM and MP, and after the treatment (see below), the culture medium was used to test its capacity to inhibit acetylcholinesterase activity at different time intervals. The results obtained using a control mixture of acetylcholinesterase, S9 mix, and phosphate buffer, pH 8, showed that in 30 min, the enzyme had no significant loss of activity by abiotic factors (data not shown). This incubation time was sufficient to achieve significant enzyme inhibition by the pesticide.
This result led to the selection of this time as the most suitable for this trial.
The results showed that after 24 hr of culture with the isolated strain in MP, the resulting medium lost its capacity to inhibit the acetylcholinesterase activity, indicating that the MP was completely transformed. Therefore, this treatment is promising for detoxifying F I G U R E 3 Survival of the Burkholderia sp. strain S5-2 immobilized on Opuntia sp., Agave sp., and zeolite. Percentage survival of bacteria was calculated from the CFU/g support values of at the end of the kinetics, with respect to the initial values. The same letters are not significantly different (α = 0.05). All supports were added at 2% w/v to the culture medium  (e) and (f), but using zeolite. In controls without cells (b, d, and f), PNP was not detected because the MP hydrolysis did not occur via abiotic factors (PNP was not added to the culture media). All supports were added at 2% w/v to the culture medium solutions containing MP ( Figure 6). In addition, control media with supports only do not have negative effects on the activity of acetylcholinesterase. There were differences in the MSM with MP treatment without bacteria, demonstrating that the acetylcholinesterase activity remained low (α=0.05). In contrast, the acetylcholinesterase assays using the culture media before and after each treatment with free and immobilized cells with MSM and without MP (control) showed that the acetylcholinesterase activity was not lost during the incubation time ( Figure 6).

| DISCUSSION
A bacterial strain with ability to hydrolyze MP, and mineralized PNP, was isolated from contaminated soil. Biochemical and molecular tests allowed for the inclusion of this strain in the B. cepacia complex. There are reports of the genus Burkholderia that have genes involved in the degradation of organophosphorus pesticides (Chino-Flores et al., 2012); however, the ability of this particular strain to degrade PNP, which is toxic to microorganisms, makes it a useful tool in biotechnology for bioremediation purposes. Nitroaromatic compounds are released into the environment because they have wide use as dyes, pesticides, plasticizers, explosives, and solvents (Spain & Gibson, 1991). Aromatic compounds are relatively resistant to biomineralization due to enhanced stability caused by the resonance energy of the aromatic ring (Ismail & Gescher, 2012). The Burkholderia sp.
strain S5-2 can degrade an aromatic compound such as PNP, however, which begs the question: what other aromatic pollutants will this strain be able to mineralize?
There is a report in B. cepacia of the mpd gene coding for methyl parathion hydrolase, which is responsible for the hydrolysis of MP (Ekkhunnatham, Jongsareejit, Yamkunthong, & Wichitwechkarn, 2012). Vikram et al. (2012) found in the Burkholderia strain SJ98 genes encoding monooxygenases responsible for the degradation of aromatic compounds. However, we do not have any report of B. cenocepacia that can hydrolyze the MP and degrade PNP. We do not know the molecular mechanisms by which the B. cenocepacia strain S5-2 hydrolyzes the MP and degrades the PNP, however, opening the doors for future investigations to solve this question.
PNP and other nitroaromatics have been reported to be highly toxic to most microorganisms, thus limiting its degradation at high concentrations (Samuel, Sivaramakrishna, & Mehta, 2014). It has been reported, however, that some bacteria such as Pseudomonas, Arthrobacter, Flavobacterium, Nocardia, and Moraxella More recently, attention has turned to the isolation of bacteria capable of degrading PNP at high concentrations (in the order of 100 mg/L) that are toxic to previously studied strains (Ray, Oubelli, & Löser, 1999).
In this work, when the degradation tests were performed using suspended cells, a slight delay in B. cenocepacia strain S5-2 growth was , Agave sp., and zeolite, respectively. The PNP (▪) and UFC/ml of Burkholderia cenocepacia S5-2 strain ( ) was determined after 24 hr of treatment in mineral medium supplemented with PNP and inoculated with strain S5-2. As a control, the same medium is used uninoculated ( ). Different letters indicate significant differences (α = 0.05). All supports were added at 2% w/v to the culture medium observed during the first 12 hr, which is associated with the toxic effect of PNP. The gap between the PNP decrease and biomass growth may occur because PNP must be transformed by one of the two oxidative pathways described in previous reports, hydroquinone and hydroxyquinol (Kadiyala & Spain, 1998;Kitagawa, Kimura, & Kamagata, 2004;Spain & Gibson, 1991;Zhang et al., 2012). Both pathways transform the PNP into β-ketoadipate, which enters the tricarboxylic acid cycle, allowing for the production of energy and growth. Thereafter, the bacterial growth was exponential.
There are few reports of isolates that can perform both MP hydrolysis and PNP degradation. Burkholderia sp. strain S5-2 can perform both processes, however, suggesting a total mineralization of MP, although their growth is initially limited by PNP toxicity. The toxic effect of PNP was evident when the strain was grown with different concentrations of this compound, which made it necessary to establish new strategies to overcome this drawback using cell immobilization.
Cell immobilization offers many advantages addressed earlier in this study; however, an appropriate material for this process, including characteristics such as being economical, inert, and affordable, is difficult to find. The different supports proposed in this study comply with these characteristics. Thus far, we have not found reports for the supports used in this study for the biological removal of organophosphate pesticides, although related studies were available. For example, zeolite was studied to immobilize the Pseudomonas sp. strain ADP for atrazine degradation (Stelting, Burns, Sunna, Visnovsky, & Bunt, 2012).
This research showed that this bacterial species remained viable for 10 weeks at 25°C. Another study reported that Agave sp. fiber was used to immobilize fungi (Trametes versicolor and Pleurotus ostreatus) to study the degradation of the dye triphenylmethane basic green 4.
Immobilized fungal cultures on Agave fiber without addition of cosubstrate was selected as the best option, resulting in decoloration efficiencies of 99.3% (Castillo, 2010).
There are multiple reports showing that the immobilization of cells promotes xenobiotic degradation processes. Tallur, Mulla, Megadi, Talwar, and Ninnekar (2015)  also has a negative effect on the ability of bacteria to adhere to this support, as even at the lowest concentration tested we only found 20%-40% of the cells adhered compared to the control without PNP.
Strain immobilization on the three supports was evaluated by scanning electron microscopy. Immobilized cells on the proposed supports were very efficient in the degradation of MP and no differences were found in the times of degradation. In these treatments, however, the degradation was higher than in free cell cultures. The amount of immobilized cells on zeolite was less than Opuntia sp. and Agave sp., likely because this support is pulverized and the cells are much more exposed to the environment and turbulence generated during agitation, preventing biofilm formation on the surface of the support. This is likely why immobilized cells were not observed in zeolite by scanning electron microscopy. In addition, the available surface area for immobilization on zeolite is minor compared to supports of vegetable origin. Although the amount of immobilized cells for each treatment differs significantly, the time required to hydrolyze MP and degrade PNP is not different, and this may be because the system reached the maximum degradation rate for the concentration of pesticide used in our experiments.
For the Opuntia sp. and Agave sp. supports, the amount of adsorbed pesticide was superior to zeolite. The rapid hydrolysis of MP and PNP degradation make it difficult to determine the extent to which the sorption phenomenon affects the degradation process.
Nevertheless, the adsorption of the pesticide by the supports may promote the degradation process. As an example, there is a report in  Increasing the PNP concentration prolonged the acclimation period and reduced the PNP disappearance rate. Saez, Aparicio, Amoroso, and Benimeli (2015) evaluated the influence of acclimation on a free or immobilized Streptomyces consortium on lindane degradation in liquid and slurry systems. After the acclimation period, the survival of all members was confirmed, thus demonstrating the consortium stability. Acclimated cultures reached a higher biomass (0.56-0.65 g/L) and lindane removal (40%-97%) than the consortium without acclimation (0.37-0.44 g/L; 33%-87%) when they were cultured in a liquid medium with 20 and 50 mg/L of lindane.
There are no recent reports that provide information on the use of Agave sp. and Opuntia sp. fibers for pesticides degradation; therefore, the results found in this study propose an opportunity to degrade For the purposes of bioremediation, we suggest studying genes and enzymes responsible for this degradation pathway and expressing them in another vector that offers greater security against such risks.
Toxicological tests, however, showed that the effect of the parental material (MP) on acetylcholinesterase is removed by strain S5-2, but fails to demonstrate the possibility of the media remaining toxic due to other metabolites derived from MP degradation. Considering this possibility, a test to detect metabolites coming from MP degradation was conducted but none of the reported metabolites were found (data not shown), suggesting total MP degradation. These results encourage the safe use of immobilized Burkholderia sp. strain S5-2 as a system for MP degradation under controlled conditions, for example, in a reactor.
A strain belonging to the genus Burkholderia sp. that can completely degrade MP was isolated from agricultural soil in central Mexico. The degradation process was compared between free and immobilized cells on Opuntia sp. and Agave sp. fibers, as well as powdered zeolite.
The results showed that the degradation process is superior with immobilized cells because cells remain viable for longer periods, and the strain can withstand higher concentrations of PNP when immobilized.
Toxicity tests for acetylcholinesterase activity demonstrated complete detoxification of the pesticide.