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Magnetic Cross-Linked Enzyme Aggregates (mCLEAs) of Candida antarctica Lipase: An Efficient and Stable Biocatalyst for Biodiesel Synthesis

  • Álvaro Cruz-Izquierdo,

    Current address: Department of Chemistry, University of Bath, Bath, United Kingdom

    Affiliation Department of Biochemistry and Molecular Biology, University of the Basque Country (UPV/EHU), Bilbao, Spain

  • Enrique A. Picó,

    Affiliation Department of Biochemistry and Molecular Biology, University of the Basque Country (UPV/EHU), Bilbao, Spain

  • Carmen López ,

    carmen.lopez@ehu.es

    Current address: Department of Chemistry and Food Technology, Universidad Politécnica de Madrid, Madrid, Spain

    Affiliations Department of Biochemistry and Molecular Biology, University of the Basque Country (UPV/EHU), Bilbao, Spain, IKERBASQUE, Basque Foundation for Science, Bilbao, Spain

  • Juan L. Serra,

    Affiliation Department of Biochemistry and Molecular Biology, University of the Basque Country (UPV/EHU), Bilbao, Spain

  • María J. Llama

    Affiliation Department of Biochemistry and Molecular Biology, University of the Basque Country (UPV/EHU), Bilbao, Spain

Abstract

Enzyme-catalyzed production of biodiesel is the object of extensive research due to the global shortage of fossil fuels and increased environmental concerns. Herein we report the preparation and main characteristics of a novel biocatalyst consisting of Cross-Linked Enzyme Aggregates (CLEAs) of Candida antarctica lipase B (CALB) which are covalently bound to magnetic nanoparticles, and tackle its use for the synthesis of biodiesel from non-edible vegetable and waste frying oils. For this purpose, insolubilized CALB was covalently cross-linked to magnetic nanoparticles of magnetite which the surface was functionalized with –NH2 groups. The resulting biocatalyst combines the relevant catalytic properties of CLEAs (as great stability and feasibility for their reutilization) and the magnetic character, and thus the final product (mCLEAs) are superparamagnetic particles of a robust catalyst which is more stable than the free enzyme, easily recoverable from the reaction medium and reusable for new catalytic cycles. We have studied the main properties of this biocatalyst and we have assessed its utility to catalyze transesterification reactions to obtain biodiesel from non-edible vegetable oils including unrefined soybean, jatropha and cameline, as well as waste frying oil. Using 1% mCLEAs (w/w of oil) conversions near 80% were routinely obtained at 30°C after 24 h of reaction, this value rising to 92% after 72 h. Moreover, the magnetic biocatalyst can be easily recovered from the reaction mixture and reused for at least ten consecutive cycles of 24 h without apparent loss of activity. The obtained results suggest that mCLEAs prepared from CALB can become a powerful biocatalyst for application at industrial scale with better performance than those currently available.

Introduction

Due to the global shortage of fossil fuels, a consequent excessive rise in the price of crude oil and increased environmental concerns, a rapid growth in biodiesel production has being observed [1]. Biodiesel is a clean-burning diesel fuel composed of a mixture of alkyl esters of long-chain fatty acids which is typically produced from nontoxic, renewable biological resources such as vegetable oils, animal fats, or even used cooking oils [2]. Nowadays, the alkali-catalyzed transesterification of triglycerides present in oils or fats is the most common way to produce biodiesel at industrial scale due to its high conversion and kinetics. However, when these raw materials contain an elevated percentage of water or free fatty acids, undesirable reactions drastically reduce the yield and quality of the resulting biodiesel [2]. Thus, enzyme-catalyzed production of biodiesel by lipases is more advantageous over the chemical counterpart since it is chemically selective, reaction is carried out at lower temperature and under milder conditions and downstream processes are more environmentally friendly [3].

Lipases constitute a group of versatile enzymes that catalyze the hydrolysis of lipids in aqueous media, but in organic media they can catalyze synthetic reactions, including interesterifications between triglycerides and alcohols to produce glycerin and alkyl-esters of long chain fatty acids, i.e., biodiesel. However, free lipases are easily inactivated in organic solvents and difficult to recover for reuse [4]. Candida antarctica lipase B (CALB) is an extracellular monomeric globular (33.5 kDa) enzyme which is not as efficient as other lipases in hydrolyzing triglycerides, but it is highly stereospecific towards both ester hydrolysis and synthesis. Due to its efficiency and high selectivity this lipase has been immobilized by several methods (especially by covalent attachment to silica gel, celite or activated nanoparticles) and it is being used in a wide range of applications replacing industrial synthetic processes [5].

Many strategies have been recently applied to immobilize CALB. One of the most successful consists of covalent linking of the enzyme to the surface of iron oxide magnetic nanoparticles (MNPs) [6], [7]. The high specific surface of MNPs favors the binding efficiency of the enzyme, and the superparamagnetic behavior of the support permits the easy and selective recovery of the biocatalyst using a magnet and its subsequent reuse in more catalytic cycles [8], [9]. On the other hand, the support-free methodology consisting of the formation of cross-linking enzyme aggregates (CLEAs) of lipase with glutaraldehyde [10], [11] is a simple technique which does not require the use of highly pure enzymes. It has a broad scope and affords robust, recyclable catalysts that exhibit high activity retention, enhanced thermal stability, better tolerance to organic solvents, and enhanced resistance to autoproteolysis due to the rigidification of the tertiary structure of the enzyme [12][15]. Due to the large size of the aggregates, CLEAs can be recovered from the reaction medium by centrifugation or filtration, although this process leads to the increase of CLEAs size and formation of clusters (clumping) resulting in internal mass-transfer limitations [16], [17].

In recent years, lipases immobilized on MNPs or in CLEAs have been successfully used to obtain biodiesel. Xie and Ma [18], [19] reported 90% conversion to biodiesel using covalently immobilized Thermomyces lanuginosus lipase on amino-functionalized MNPs. Also Burkholderia cepacia lipase immobilized to MNPs of Fe3O4 yielded complete conversion to biodiesel [20]. In addition biodiesel was obtained from olive oil using CLEAs of crude preparations from Photobacterium lipolyticum lipase M37 [21]. Lai et al. [22] also reported 85.7% conversion to biodiesel from microalgal oil using an ionic liquid (1-butyl-3-methylimidazolium hexafluorophosphate) as a solvent and CLEAs obtained from crude preparations of Penicillium expansum.

Recently, our group has developed a method for the preparation of magnetic cross-linked enzyme aggregates (mCLEAs) of CALB. This method consists of the cross-linking of insolubilized lipase to aminated MNPs by glutaraldehyde [23]. The resulting mCLEAs fulfill the main benefits of magnetic biocatalysts and CLEAs, as they show improved thermal and storage stabilities, and can be reused after their recovery from the reaction mixture with a magnet. Also mCLEAs of α-amylase from Bacillus sp. [16] and lipase from Aspergillus niger [24] were successfully prepared and used to hydrolyze starch and to obtain glycerol carbonate, respectively.

In this paper, the main magnetic properties of mCLEAs were assessed as well as the utility of this robust biocatalyst to obtain biodiesel from several non-edible vegetable oils. Finally, the enhanced stability of our mCLEAs of CALB was ascertained by reusing the magnetic enzyme to catalyze the production of biodiesel in consecutive 24 h batch reactions. A similar procedure to that detailed here to prepare mCLEAs of CALB can be easily expanded to prepare mCLEAs of other enzymes of interest.

Materials and Methods

Materials

CALB L, the lipase B of Candida antarctica (CALB, EC 3.1.1.3, 19.1 U/mg protein; 7.50 mg protein/ml) was kindly provided by Novozymes (Bagsvaerd, Denmark). HyperLadder I markers were purchased from Bioline (Randolph, MA, USA). Tween 20 and Tween 80 were obtained from Panreac (Barcelona, Spain). 3-Aminopropyltriethoxysilane (APTS), NaBH4, FeCl2, FeCl3, dimethylsulfoxide (DMSO), sodium dodecyl sulphate (SDS), p-nitrophenyl acetate (pNPA), bovine serum albumin, and Triton X-100 were purchased form Sigma-Aldrich (St. Luis, MO, USA). Coomassie Blue was obtained from GE Healthcare (Uppsala, Sweden). All other chemicals were supplied by Merck (Darmstadt, Germany). Non-edible oils (unrefined soybean, jatropha and cameline) were obtained from Bunge Ibérica, S.A. (Zierbena, Spain), Jatropha Hispania, S.L. (Toledo, Spain) and Camelina Company (Madrid, Spain), respectively. Olive oil used as a control was purchased from Carbonell (Madrid, Spain) and waste frying oil was obtained from local restaurants.

Synthesis and functionalization of magnetic nanoparticles (MNPs)

Magnetic nanoparticles of magnetite (Fe3O4) were synthesized by coprecipitation of iron salts in alkaline medium [25]. An aqueous solution, 50 ml, containing 0.36 M FeCl2 and 0.72 M FeCl3 was pumped at 5.0 ml/min (LKB Pump P-1, Pharmacia, Uppsala, Sweden) into 450 ml of 1 M NH4OH solution under continuous mechanic stirring at room temperature (S1 Video). The obtained black precipitate was separated from the liquid phase using a magnetic field, and then magnetically washed thrice with ultrapure water (MilliQ, Millipore Co., Bedford, MA, USA) and twice with phosphate buffered saline (PBS, 100 mM sodium phosphate, 150 mM NaCl, pH 7.4). All solutions used for the synthesis of MNPs were prepared using MilliQ water. Moreover, a N2 gas stream was continuously bubbled through all solutions during the process. The resulting magnetic nanoparticles contained –OH groups on their surface [26], [27]. In order to functionalize them with –NH2 groups, MNPs (300 mg, dry weight) were incubated with 30 ml of 2% (v/v) APTS at 70°C with orbital shaking (200 rpm). After 24 h, they were washed thrice with PBS and maintained in the same buffer at 4°C until use.

Characterization of MNPs

Phase identification was done by X-ray diffraction studies (XRD, Philips diffractometer PW1710, Almelo, The Netherlands). The crystallite size was calculated from the X-ray line broadening using Scherrer's and Warren's equation:where K takes the value of 0.89 considering spherical particles; λ is the wavelength of X radiation used (0.54 nm); θ is the Bragg angle; β is the net diffraction peak broadening in radians being determined from:

where βobs is the observed broadening (experimental) and βins the instrumental broadening.

The particle size and morphology were determined by transmission electron microscopy (TEM, JEOL 1010, Peabody, MA, USA). The density of –NH2 groups on the nanoparticles surface was determined by a colorimetric assay using p-nitrobenzaldehyde [28]. The magnetic characteristics were measured using different devices: for the calculation of magnetic saturation (Ms) 2 K hysteresis loops were performed using a vibrating sample magnetometer (VSM) in a superconducting magnet (14 T) cooled by a closed circuit of He (CFMS, Cryogenic Ltd., London, UK). To calculate coercivity (Hc) and remanence (Mr) an electromagnet was used at room temperature and moderate fields (0.9 T). The average size of magnetic particles was calculated from the magnetization data according to Langevin's equations adjusted for non-interacting superparamagnetic model. MNPs dry weight and concentration were analyzed using a vacuum concentrator (Savant SpeedVac concentrator, Thermo Scientific, Waltham, MA, USA).

Preparation of magnetic CLEAs from CALB

In order to obtain magnetic CLEAs, 10 mg (dry weight) of MNP–NH2 were incubated with different concentrations of CALB (from 0.025 to 1.2 mg protein/mg MNP–NH2) in the presence of precipitant agents and detergents in a final volume of 15 ml. The precipitant agents used were 80% (v/v) ethanol, 80% (v/v) 2-propanol, 80% (v/v) acetone in water at 4°C, or ammonium sulphate at concentration in the range of 12.5 to 125 mmol/mg protein at 25°C. The detergent concentrations used were 0–5 mM Triton X-100, 0–0.1 mM Tween 20, 0–0.1 mM Tween 80 or 0–25 mM SDS. In all cases, the samples were mixed continuously at 30 rpm using an Intelli-Mixer RM-2, Elmi Ltd. (Riga, Latvia). After 5 min, a 2.5 M glutaraldehyde solution was added (final concentration from 0 to 500 mM) and the suspension was maintained in agitation for 1 to 24 h. After this time, the mCLEAs were removed from the liquid phase using magnetic field, and mCLEAs were washed thrice with PBS. Both the Schiff's bases and the unreacted aldehyde groups were reduced for 2 h at room temperature with rotational mixing with NaBH4 (0.75 mg/mg MNP–NH2) dissolved in 100 mM carbonate/bicarbonate buffer, pH 10.0. In order to minimize non-specific interactions mCLEAs were then magnetically washed for 10 min firstly with 2 M NaCl in PBS and then with 1% (v/v) Triton X-100 in PBS as reported by Mateo et al. (2000) [29]. After each step, the excess of reagents and possible unretained enzyme were removed by washing thrice with PBS for 10 min. At the end of the immobilization process, the final concentration was 2 mg mCLEAs/ml. The magnetic catalyst was stored at 4°C in PBS for future use.

Magnetic biocatalysts at different formation steps were incubated at 100°C for 5 min, and then, the liquid phase was collected and analyzed by sodium dodecyl sulphate polyacrylamide gel electrophoresis (SDS-PAGE) [30] using homogeneous 8% acrylamide gels revealed with silver (Bio-Rad, Hercules, PA, USA). The amount of immobilized lipase was calculated by measuring the protein remaining in solution at 595 nm (Bio-Rad protein Assay kit, Hercules, PA, USA).

Enzyme assays

Esterase activity with pNPA.

The activity of soluble and immobilized CALB was assayed with p-nitrophenyl acetate (pNPA) as a substrate according to the protocol reported by Gao et al. [31] with minor modifications. Specifically, soluble or immobilized lipase (1–2 µg protein) was added to a reaction mixture which contained 10 µl of pNPA (100 mM in DMSO) in 980 µl of PBS. The reaction mixture was maintained for 15 min at room temperature with rotational mixing at 30 rpm (Intelli-Mixer RM-2, Elmi Ltd., Riga, Latvia). Samples were withdrawn every 5 min (in the case of immobilized lipase the magnetic biocatalysts were separated from the liquid phase using a magnet) and the appearance of p-nitrophenol (pNP) was measured spectrophotometrically (Beckman Coulter DU 800, Brea, CA, USA) at 405 nm (εpNP = 9.43 mM−1·cm−1). One unit (U) of esterase activity was defined as the amount of enzyme that catalyzes the appearance of 1 µmol pNP per min under the assay conditions.

Transesterification of olive oil.

Olive oil (0.2 g) and 2-propanol (1∶6 molar ratio oil∶alcohol) were incubated with 1% (w/w of oil) of magnetic catalyst. The reaction was maintained at 40°C and 30 rpm with rotational mixing. The initial reaction rate for biodiesel production was assessed by withdrawing aliquots (5 µl) of the liquid phase at defined intervals which were analyzed by high-performance liquid chromatography (HPLC) as indicated below. Transesterification activity was defined as mg of oil transformed to biodiesel (fatty acid propyl esters, FAPEs) per mg of MNP-NH2 and time (h) considering the initial reaction rate of transesterification.

Synthesis of biodiesel.

FAPEs were produced from vegetable oil (0.2 g) using 2-propanol as alkyl donor (1∶6 molar ratio oil∶alcohol) and 1% (w/w of oil) of magnetic catalyst in a solvent-free reaction. The reaction was followed by withdrawing aliquots (10 µl) of the liquid phase. Semi-quantitative analysis of samples was performed by thin layer chromatography (TLC) and the quantitative analysis using control olive oil was performed by HPLC as described below.

Analytical methods

HPLC analysis.

Five µl of samples withdrawn from the reaction mixture were diluted in 250 µl of n-hexane and analyzed by HPLC (Waters Corporation, Milford, MA, USA) using a diode array detector according to Holčapek et al. [32]. The C18 column (5 µm, 4.6×250 mm, Tracer Lichrosorb RP18) was eluted with 100% pure methanol (phase A) and a mixture of propanol∶n-hexane (5∶4 v/v) (phase B) at a flow rate of 0.5 ml/min using a gradient from 0 to 50% phase B in 25 min. Peaks were detected at 205 nm.

Thin layer chromatography (TLC) analysis.

A semi-quantitative analysis of non-edible or waste frying olive oil was also assessed using TLC. Silica gel 60 coated plates (Merck, Darmstadt, Germany) were activated for 30 min at 100°C and 0.5 µl samples were applied. The ternary mixture n-hexane∶ethyl acetate∶acetic acid (90∶10∶1 v/v/v) was used as the eluting phase [33]. After chromatography development (about 40 min), plates were air dried at room temperature, and then immersed for 1 min with gentle orbital shaking in a solution of 0.02% (w/v) Coomassie Blue R-350 [34], prepared in acetic acid∶methanol∶H2O (1∶3∶6 v/v/v) as indicated by the manufacturer. Finally, the plates were air dried at room temperature. Spots corresponding to substrates and products of the transesterification reaction were identified by using appropriate reference external standards (triolein, 1,3-diolein, 1-oleyl-rac-glycerol, oleic acid and propyl oleate) run in parallel.

Results and Discussion

Magnetic nanoparticles characterization

MNPs size was analyzed by XRD and TEM. X-ray diffraction patterns showed that magnetite constitutes the only crystalline phase present both in MNP–OH and MNP–NH2 (Fig. 1), with a crystallite size of 11.2 nm and 11.1 nm, respectively, according to Scherrer's equation, and 9.5 nm and 9.4 nm, respectively, according to Warren's equation. These results indicated that functionalization of MNPs with –NH2 groups did not change the phase, nor the crystallite size of the magnetic support. The shape and size of the MNPs was confirmed by TEM (Fig. 2), which showed that both types of MNPs are spherical particles with a mean diameter around 10 nm, indicating that coating their surfaces with –NH2 groups did not result in observable differences in their size, shape or aggregation state.

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Figure 1. XRD spectrum of magnetic nanoparticles.

MNPs were coated with –OH (solid line), and –NH2 (dotted line) groups.

https://doi.org/10.1371/journal.pone.0115202.g001

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Figure 2. TEM images of magnetic nanoparticles.

MNPs were coated with (a) –OH, and (b) –NH2 groups. Samples were dispersed in ethanol using an ultrasound bath and then placed onto a Formvar-covered copper grid and evaporated in air at room temperature. Bars represent 20 nm in both pictures.

https://doi.org/10.1371/journal.pone.0115202.g002

The surface areas were theoretically calculated from the particle size distribution provided by TEM data (Table 1). The results were similar to those reported by other authors, as Harris et al. [35] who determined a surface area of 110 m2/g for 8.7 nm nanoparticles, or Sahoo et al. [36] who calculated 93 m2/g for particles with mean diameter of 10–12 nm.

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Table 1. Main characteristics of MNPs coated with –OH and –NH2 groups.

https://doi.org/10.1371/journal.pone.0115202.t001

The density of –NH2 groups on the surface of particles was determined using naked MNPs as a control (Table 1). The calculated density of –NH2 groups on functionalized nanoparticles (43 µmol/g) was very similar to that reported by del Campo et al. [28] who found approximately 45 µmol/g of MNPs. These authors also calculated the density of –NH2 groups by elemental analysis obtaining higher values. This result may suggest that some –NH2 groups do not react with 4-nitrobenzaldehyde, and therefore all the amine groups are not available for the interaction with the enzyme. In this case, the calculated density would represent the functionally available groups for the enzyme immobilization.

Magnetic behavior of MNPs was analyzed at different magnetic fields and two temperatures: one below the blocking temperature of magnetite nanoparticles (i.e., the temperature below which magnetite nanoparticles show ferromagnetic characteristics, and corresponds to 75 K, [37]) and the other one at close to room temperature (Fig. 3). Both types of nanoparticles (MNP–OH and MNP–NH2) showed hysteresis behavior below the blocking temperature, although this characteristic disappeared at 300 K. At this temperature, magnetic remanence (Mr) and coercivity (Hc) values fell to near zero, which is typical of superparamagnetic nanoparticles. The saturation magnetization (Ms) was determined to be 86.0 and 82.5 emu/g for naked and NH2–functionalized nanoparticles, respectively, which is lower than that reported for bulk magnetite (89 emu/g, [38]). This decrease in Ms was also observed by other authors [26], [39] and could be related to the difference between macroscopic and nanoscopic magnetite [25], [27], [35], [39]. On the other hand, the binding of APTS to the nanoparticles caused a slight decrease of 4% in the Ms of the magnetic support, which has been previously observed when organic molecules were immobilized on MNPs [40], [41]. This fact could be explained because the binding of APTS on the nanoparticle surface might quench the magnetic moment [42], [43]. Fitting magnetic result to the Langevin's function, a magnetic core average diameter of 7.8 nm, with 3–4 nm dispersion, was calculated. This value is consistent with the size determined from XRD data as aforementioned.

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Figure 3. Magnetization analysis of magnetic nanoparticles at different temperatures.

Magnetization analysis of MNP–OH (black lines) and MNP–NH2 (grey lines) were performed at 300 K (solid lines) and 2 K (dotted lines). Inlet shows a detail of magnetization for values of magnetic field near to 0 Oe.

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Preparation of mCLEAs

Synthesis of mCLEAs involves a sequence of steps starting with enzyme insolubilization followed by cross-linking the resulting protein aggregates with themselves and the surfaces of NH2-functionalized magnetic nanoparticles. Optimization aspects concerning the selection of precipitation conditions, cross-linking agent, time or enzyme concentration were considered.

Effect of precipitating agent.

Commonly used lipase precipitating agents were selected to insolubilize CALB, i.e., ethanol, 2-propanol, acetone and ammonium sulphate (125 mmol/mg protein). After enzyme precipitation, mCLEAs were prepared at room temperature by cross-linking (for 24 h) 0.2 mg CALB/mg MNP–NH2 in the presence of 200 mM glutaraldehyde. A control using soluble enzyme was carried out in parallel, with initial protein concentration of 0.133 mg/ml and esterase activity of 2.532 U/ml. The end of the immobilization process was verified by analyzing the protein concentration in the liquid phase of the immobilization medium, and the esterase activity in both the liquid and formed mCLEAs. The selected precipitating agents allowed the formation of mCLEAs with 100% protein and esterase activity retention, with the exception of ethanol, which caused a drop in both the retained protein and esterase activity to 46.3% and 46.8%, respectively. In addition to ethanol, also 2-propanol and acetone strongly affected the esterase activity of the biocatalyst, resulting in values of 0.826, 0.655 and 0.383 U/mg MNP–NH2. However, the mCLEAs obtained with ammonium sulphate showed an activity of 1.823 U/mg MNP–NH2. When comparing these values with the theoretical immobilized activity (3.8 U/mg MNP–NH2), immobilization efficiencies of 21.7, 17.2, 10.1 and 48.0% were obtained when using ethanol, 2-propanol, acetone and ammonium sulphate, respectively. These results are in agreement with those reported by other authors [10], [11], [44], who proposed that ammonium sulphate was the best option because it usually preserves the enzymatic activity of the biocatalyst. Therefore, ammonium sulphate was selected in this work as the precipitating agent to prepare mCLEAs of CALB.

The insolubilizing effect of ammonium sulphate concentration (12.5–125 mmol/mg protein) was studied at room temperature by measuring the esterase activity retained by the resulting mCLEAs prepared using 50 µg to 1.2 mg lipase/mg MNP–NH2 and cross-linked for 5 h with 200 mM glutaraldehyde. At low concentration of lipase a good relationship between the immobilized esterase activity and ammonium sulphate was observed (Fig. 4). However at the highest concentration of salt (125 mmol/mg protein), lower activity recovery was measured at lipase concentrations higher than 0.4 mg protein/mg MNP–NH2. This effect is probably due to excessive cross-linking and/or size of aggregates which would lead to irreversible enzyme denaturation and/or the appearance of diffusional problems.

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Figure 4. Combined effect of CALB and insolubilizing agent concentrations on the esterase activity of mCLEAs.

Different concentrations of lipase were cross-linked for 5 h with 200 mM glutaraldehyde in the presence of the indicated concentrations of ammonium sulphate.

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It should be noted that the theoretical immobilized activity increases with the increase of enzyme concentration in the preparation. Maximum esterase activities of 0.95, 1.91, 3.82, 7.67, 15.27 and 22.91 U/mg MNP–NH2 correspond to protein concentrations of 0.05, 0.1, 0.2, 0.4, 0.8 and 1.2 mg protein/mg MNP–NH2, respectively. Maximum immobilization efficiencies of around 60% were obtained when 0.1 mg protein/mg MNP–NH2 were used. Further increase in enzyme concentrations was not reflected in an increase of recovery activity. This is a usual behavior of immobilized enzymes which is related to diffusional limitations occurring when diffusional rate of substrates and products is lower than reaction rate, thus decreasing the observed rate of the reaction.

Conclusively, 0.1 mg protein/mg MNP–NH2 and 100 mmol of ammonium sulphate/mg protein were selected in order to prepare mCLEAs of CALB.

Effect of detergents.

It is well known that the presence of a detergent at an appropriate concentration can often hyperactivate the enzyme, especially when using lipases [45][47]. Furthermore, detergents may prevent the enzyme immobilization through its active center and promote the enzyme orientation in the support so enhancing its activity and/or stability.

The esterase activity of soluble CALB was measured in the presence of Triton X-100, Tween 20, Tween 80 and SDS, at different concentrations below and above their critical micelle concentration (cmc) which were 0.6, 0.06, 0.012 and 8 mM (0.388, 0.074, 0.016 and 2.307 kg/m3), respectively. The activity of soluble CALB increased in the presence of Triton X-100 at concentrations above its cmc (S1A Fig.). However, the presence of Triton X-100 at such concentrations during the preparation of mCLEAs had a negative effect in oil transesterification (S1b Fig.). Fernández-Lorente et al. [45] also immobilized CALB in the presence of Triton X-100 on an aminated support, with a final detergent concentration of 1% (v/v) (i.e., 17 mM, 11 kg/m3), observing an increase in hydrolytic activity, but this was not tested in organic media [45], [46]. The detergent could enhance enzymatic activity in aqueous medium reactions, but it could lose the hyperactivation capability in hydrophobic media, due to the formation of inverse micelles.

Both Tween 20 and Tween 80 had no effect on CALB esterase activity nor on mCLEAs transesterification activity. The presence of SDS decreased the activity of poorly concentrated mCLEAs, whereas apparently caused a strong hyperactivation of highly concentrated samples. Such hyperactivation is similar to that described by López-Serrano et al. [48] and Gupta et al. [44], who prepared CLEAs in the presence of SDS and observed that the activity increased 2–3 fold. Actually, the transesterification activity of the biocatalyst prepared with high concentration of protein in absence of SDS should be 4-fold higher than the one with lower concentration. The presence of SDS when preparing mCLEAs with highly concentrated aggregates could protect the hydrophobic areas close to active centers, resulting in biocatalysts with lower steric hindrance and thus, higher values of specific activity.

The use of detergents during the formation of mCLEAs would only be recommended for the immobilization of high protein concentrations. However, detergents were not used for further experiments in this work as concentrations of protein above 0.1 mg/mg MNP–NH2 seem to result in low immobilized enzyme retentions.

Effect of cross-linker concentration.

The cross-linking effect of glutaraldehyde was investigated by assessing the esterase activity of mCLEAs prepared by incubating for 5 h the insolubilized lipase (0.1 mg CALB/mg MNP–NH2 with 100 mmol ammonium sulphate/mg protein) in the presence of glutaraldehyde at concentrations from 0 to 500 mM (Table 2). The immobilized esterase activity increased linearly when glutaraldehyde concentration was varied from 0 to 200 mM, the maximum value (1.24 U/mg MNP–NH2) representing 65% of offered activity (1.91 U/mg MNP–NH2). Above that concentration, the immobilized activity remained unchanged. At higher glutaraldehyde concentration, the cross-linking of MNP–NH2 could be favored, reducing the available surface area for the immobilization of aggregates. On the other hand, the immobilization time of 5 h could be insufficient for the formation of covalent bonds, and a more prolonged incubation at these conditions should be used in order to increase the activity retention.

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Table 2. Effect of cross-linker concentration on the preparation of mCLEAs of CALB.

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Effect of protein concentration and immobilization time.

At first approach, mCLEAs of CALB (0.1 mg protein/mg MNP–NH2, 100 mmol sulphate/mg protein, 200 mM glutaraldehyde, no detergent) were prepared by varying the time (0, 0.5, 1, 2, 3, 4, 5, 6 and 24 h) used to cross-link the enzyme aggregates onto the surface of MNP–NH2. Addition of the cross-linker agent resulted in an immediate activity retention of 42%. This value rose from 65% to almost 100% when the contact time was enlarged from 5 h to 24 h (Table 3). This increase indicates that the immobilization process requires large periods of time to completely establish covalent linkages between enzyme and support. With this in mind, the observed apparent low value of retained activity when high loads of protein were immobilized for 5 h (Table 3) could be due to low retention of protein during this insufficient period of time. When an immobilization time of 24 h was used, the complete protein immobilization was confirmed by analysis of unbound protein at the different steps of the process (S2 Fig.). Even so, high protein loads resulted in low apparent retained activities. Data suggest that 0.1 mg protein/mg MNP–NH2 is the maximum concentration that ensures the absence of steric hindrance observed in esterase activity measurement.

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Table 3. Effect of protein concentration and immobilization time on the preparation of mCLEAs of CALB.

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Lipases have been immobilized in a great variety of supports in several works [10], [49], obtaining immobilization efficiencies below 80%. Xie and Ma [18], [19] immobilized lipase on amino-functionalized magnetic nanoparticles and studied the optimization of the protein concentration to obtain maximum immobilization efficiencies. As a result, they obtained 70% efficiency at concentrations in the range of 0.025 to 0.05 mg protein/mg MNP–NH2. Our improved immobilization method allowed the load of a higher concentration of protein per mg of support with total activity retention, which leads to enzyme and support savings, and consequently economical benefits in production processes.

Morphology of mCLEAs.

The size and shape of mCLEAs of CALB were examined by TEM after staining the samples with 1% (w/v) phosphotungstic acid. Discrete arrangements of about 100 nm×75 nm (Fig. 5a) were routinely detected although larger aggregates could be also observed (Fig. 5b).

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Figure 5. TEM images of mCLEAs.

Samples were negatively stained with phosphotungstic acid and dispersed in ethanol as in Fig. 2. (a) and (b) represent different images of the same sample. Bars represent 50 nm in both pictures.

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Biodiesel production by mCLEAs

The ability of the magnetic CLEAs to catalyze the production of biodiesel from vegetable oils in a solvent-free system was tested. The transesterification reaction was performed using 200 mg olive oil and 2-propanol in a molar ratio of 6∶1 (alcohol∶oil) in the presence of different concentrations of mCLEAs (prepared using 0.1 mg protein/mg MNP–NH2, 100 mmol sulphate/mg protein, 200 mM glutaraldehyde, no detergent). After incubating the reaction mixtures containing mCLEAs (at 0.5, 1, 2 and 5% w/w of oil) for 24 h at 30°C, conversions of 64.0, 76.1, 81.5 and 82.2%, respectively, were obtained. These data indicate that a very low concentration of the biocatalyst (1% w/w of oil) is suitable to catalyze the transesterification of olive oil.

The time-course of the reaction was assessed during 72 h for both control olive oil and waste frying oil. Samples were withdrawn at time intervals and analyzed by either HPLC (olive oil) or TLC (waste frying oil). HPLC data revealed the appearance of diglycerides, monoglycerides and free fatty acids (Fig. 6) as intermediates in the synthesis of biodiesel (fatty acid propyl esters, FAPEs). These intermediates could be also observed in samples analyzed by TLC and stained with Coomassie Blue (Fig. 7a), indicating that this versatile semi-quantitative method can be useful to determine the reaction progress with time by following changes in substrate and products concentrations. It is worth mentioning that TLC analysis followed by plate revealing with Coomassie Blue permits to analyze in parallel at least 10 samples in less than 1 h. In addition it allows the use of crude and/or recycled vegetable oils which could originate troubles when analyzed by HPLC.

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Figure 6. Time-course of biodiesel (FAPEs) conversion catalyzed by mCLEAs of CALB.

The reaction mixture containing 200 mg olive oil, 2-propanol (6∶1 alcohol∶oil molar ratio) and 1% (w/w of oil) mCLEAs was incubated for 72 h at 30°C with rotational mixing. Samples (10 µl) were withdrawn at the indicated times and analyzed by HPLC. Triglycerides (•), FAPEs (▪), diglycerides (▵) and monoglycerides with free fatty acids (⋄).

https://doi.org/10.1371/journal.pone.0115202.g006

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Figure 7. Analysis by TLC of biodiesel (FAPEs) conversion using mCLEAs of CALB.

The reaction mixture and conditions were the same as in Fig. 6, except that (a) waste frying olive oil and (b) different vegetable oils were used as substrate. Olive oil was included as a control substrate. Triglycerides (TGs), diglycerides (DGs), monoglycerides (MGs) and free-fatty acids (FFAs).

https://doi.org/10.1371/journal.pone.0115202.g007

The efficiency of low concentrations of mCLEAs to catalyze the conversion into biodiesel of other non-edible vegetable triglycerides was tested using jatropha, cameline and crude (unrefined) soybean oils. Samples of these crude oils were used without any pretreatment. The transesterification reaction with 2-propanol was carried out using 1% of biocatalyst (w/w oil) at 30°C for 72 h, as described previously for olive oils, and the resulting FAPEs were analyzed by TLC. As shown in Fig. 7b, similar bioconversions were observed in all cases after 24 h of transesterification reaction.

The immobilization of lipase to different carriers for biodiesel production has been studied previously with high conversion results (64–100%), although elevated concentrations of biocatalyst (5–15% w/w of oil) were used in most of the cases [49][52]. Even when lipase was immobilized on NH2-functionalized magnetic nanoparticles, requirements from 17.3 to 40% (w/w of oil) of biocatalyst were reported [18][20]. Only a few number of researchers described the use of lower concentrations of enzyme to catalyze the transesterification reaction, as Mendes et al. [53] who used 0.2% (w/w of oil) of enzyme, although they worked at 45°C with high alcohol∶oil molar ratios. It is well known that temperature not only increases kinetics but also can affect stability of the enzyme.

The stability and reusability of mCLEAs of CALB was investigated by reusing the biocatalyst for several consecutive reaction cycles at temperatures from 30 to 60°C. After each cycle (24 h) the biocatalyst was recovered from the reaction mixture using a magnetic field. Two different catalysts, prepared using 0.05 and 0.1 mg CALB/mg MNP–NH2, were tested. The biocatalyst with lower concentration of lipase not only showed a 4-fold lower transesterification activity but it was also considerably less stable than its counterpart containing 0.1 mg protein/mg MNP–NH2 (Fig. 8). Using the latter, the 24 h-conversion was preserved for at least 10 consecutive reaction cycles without observing any significant loss of catalytic capacity. Although stability decreased with the increase in temperature, the highly-loaded biocatalyst maintained more than 60% of the activity after 10 cycles at 60°C.

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Figure 8. Reusability of mCLEAs of CALB at different temperatures.

Biocatalyst was used in consecutive reaction cycles of 24 h for biodiesel (FAPEs) conversion from olive oil at: (a) 30°C, (b) 40°C, (c) 50°C and (d) 60°C. The reaction mixture and conditions were the same as in Fig. 6. Relative conversion is referred to the final conversion after the first cycle and was calculated using samples analyzed by HPLC. Two types of mCLEAs were tested which were prepared using 0.05 (◯) and 0.1 mg protein/mg MNP-NH2 (•).

https://doi.org/10.1371/journal.pone.0115202.g008

Wang et al. [20] observed that the retained activity of their lipase catalyst decreased by more than 70% after 10 consecutive cycles of reaction at 40°C; Xie and Ma [18], [19] observed a decrease of 50% activity after the fifth cycle of catalysis using Thermomyces lanuginosus lipase immobilized on MNPs for the production of biodiesel at high temperatures (45–50°C). Our data reveal that the combination of cross-linked enzyme aggregates with MNPs results in a robust biocatalyst which is able to catalyze the synthesis of biodiesel at low enzyme concentration, and is more stable than other lipase preparations reported so far. The effectiveness of this biocatalyst for the synthesis of biosurfactants was also proved recently in a previous work from our group [54].

Novel enzyme engineering techniques are being applied for the improvement of catalytic efficiencies of CALB. Thus, Agarwal and coworkers [55] introduced a pothoactivatable molecule on the surface of the enzyme, which allowed the modulation of the enzyme conformation by light stimulation, obtaining an increase in 24% of CALB catalytic activity. A combination of protein engineering with mCLEAs formation could result in an easily recoverable and reusable enzyme with improved enzymatic activity and high stability, which could considerably increase the robustness and applicability of the biocatalyst.

Conclusions

In this work we report an efficient, facile and economical method to prepare mCLEAs of Candida rugosa lipase B by cross-linking with glutaraldehyde CALB aggregates onto the surface of MNPs functionalized with -NH2 groups. The resulting magnetic biocatalyst shows an enhanced stability and maintains the superparamagnetic behavior typical of MNPs, which allows for easy separation and reusability in consecutive catalytic cycles without apparent loss of activity. The utility of this robust biocatalyst for the efficiently production of biodiesel has been demonstrated although it could be also used to obtain other highly valuable compounds, such as biosurfactants, flavoring and aromatic compounds or bioactive compounds.

Supporting Information

S1 Fig.

Effect of detergents on enzymatic activity. (a) Relative esterase activity of soluble CALB; (b) Oil transesterification activity of mCLEAs: (•) 0.1 mg CALB/mg MNP−NH2; (◯) 0.4 mg CALB/mg MNP−NH2.

https://doi.org/10.1371/journal.pone.0115202.s001

(TIF)

S2 Fig.

Analysis of unbound protein after the different immobilization steps: (a) MNP-CALB (50 µg CALB/mg MNP-NH2 in absence of precipitant agent); (b) mCLEAs (100 µg CALB/mg MNP-NH2). Cont: control of offered protein (CALB, molecular mass  = 33.5 kDa); UR: unretained protein after 2 h of cross-linking; 1: first wash with PBS; 2: second wash with PBS; 3: third wash with PBS; BH4: unretained protein after NaBH4 reduction; NaCl: unretained protein after washing with 2 M NaCl; TX: unretained protein after washing with 1% (v/v) Triton X-100; B: liquid phase after incubating the MNP-CALB complex for 5 min at 100°C.

https://doi.org/10.1371/journal.pone.0115202.s002

(TIF)

S1 Video.

Synthesis of magnetic nanoparticles.

https://doi.org/10.1371/journal.pone.0115202.s003

(MPG)

Acknowledgments

We are grateful to Mr Ramiro Martínez (Novozymes A/S, Spain) for providing us with CALB samples.

Author Contributions

Conceived and designed the experiments: ACI CL JLS MJL. Performed the experiments: ACI EAP CL. Analyzed the data: ACI EAP CL JLS MJL. Contributed reagents/materials/analysis tools: ACI EAP CL JLS MJL. Wrote the paper: ACI CL JLS MJL.

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