Figures
Abstract
Background
The aim of this work is to investigate the structure and function of enzymes immobilised on nanomaterials. This work will allow better understanding of enzyme-nanomaterial interactions, as well as designing functional protein-nanomaterial conjugates.
Methodology/Principal Findings
Multiwalled carbon nanotubes (MWNTs) were functionalised with amino groups to improve solubility and biocompatibility. The pristine and functionalised forms of MWNTs were characterised with Fourier-transform infrared spectroscopy. Thermogravimetric analysis was done to examine the degree of the functionalisation process. An immobilised biocatalyst was prepared on functionalised nanomaterial by covalent binding. Thermomyces lanuginosus lipase was used as a model enzyme. The structural change of the immobilised and free lipases were characterised with transmission electron Microscopy, X-ray photoelectron spectroscopy, Fourier-transform infrared spectroscopy and Circular dichroism spectroscopy. Biochemical characterisation of immobilised enzyme showed broader pH and thermal optima compared to soluble form. Reusability of the immobilised enzyme for hydrolysis of long chain esters was demonstrated up to ten cycles.
Citation: Verma ML, Naebe M, Barrow CJ, Puri M (2013) Enzyme Immobilisation on Amino-Functionalised Multi-Walled Carbon Nanotubes: Structural and Biocatalytic Characterisation. PLoS ONE 8(9): e73642. https://doi.org/10.1371/journal.pone.0073642
Editor: Eugene A. Permyakov, Russian Academy of Sciences, Institute for Biological Instrumentation, Russian Federation
Received: May 31, 2013; Accepted: July 24, 2013; Published: September 12, 2013
Copyright: © 2013 Verma et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: The research was supported under the “ITRI think tank initiative (C0021.31.01)” and “Central Research Grant Scheme,” Deakin University (Project RM 25148). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Introduction
Various nanostructured forms such as nanoparticles, nanofibres, nanotubes, and nanocomposites have been employed as novel supports for enzyme immobilisation and stabilisation [1]–[4]. These robust nanoscaffolds have an inherently large surface area which leads to high enzyme loading and consequently high volumetric enzyme activity. Amongst various nanomaterial forms, carbon nanotubes possess unique structural, mechanical, thermal and biocompatibility properties. Carbon nanotubes have attracted considerable research interest for potential biotechnological applications, particularly in biosensors development [5]–[7]. The efficiency of nanomaterial can further be improved by the process of surface functionalization [8]. The surface functionalisation of nanomaterials involves grafting of desirable functional groups onto their surface to obtain nanomaterials with desired properties [9]. This functionalisation can affect their dispersability and interactions with enzymes, thus significantly altering the catalytic activity of the immobilised enzyme [10]. Although numerous attempts have been made to immobilise enzymes with nanomaterials, studies on the impact of nanomaterial properties (such as composition, morphology, and surface chemistry) on the structure and function of conjugated enzymes are hitherto sparse [5]. Investigating the structure and function of enzymes immobilised on nanomaterials will be crucial for developing a better understanding of enzyme-nanomaterial interactions, as well as for designing functional protein-nanomaterial conjugates [11].
Enzymes in the free form are fragile and prone to denaturation in extreme conditions of pH, temperature and organic solvents. To improve their stability, enzymes have generally been immobilised on a solid carrier [12]. Enzyme immobilisation can facilitate enhancement of catalytic stability, selectivity and reusability of the enzymes [13], [14]. Different techniques of enzyme immobilisation have employed either physical or covalent methods. Adsorption is a relatively simple method as it is a chemical free enzyme binding process [15]. However, leaching of the enzyme from the immobilised enzyme preparation after a certain number of reuses has limited its application at commercial scale. The aforementioned shortcoming can be overcome by the use of a covalent-binding using suitable cross linkers such as glutaraldehyde [13], [16]–[18]. Nanomaterial activation of either glutaraldehyde or carbodiimide has been most commonly and successfully employed for covalent immobilisation [3], [19]. Covalent binding methods produce relatively stable immobilised enzyme preparations with more reusability as compared to the physical adsorption method [2], [18]. Recently, researchers have immobilised lipase on carbon nanotube through adsorption for ester synthesis in non-aqueous medium [10], [19], [20]–[22], however, associated structural changes in the immobilised enzyme are not documented in the literature.
In this present work, multi-walled carbon nanotubes (MWNTs) were amino-functionalised with ethylenediamine and examined for the degree of functionalisation. Thermomyces lanuginosus lipase was then covalently immobilised onto the functionalised MWNTs supports using a glutaraldehyde cross-linker. Enzyme post immobilisation structural changes were analysed using various spectroscopy techniques. The free and MWNTs bound lipase was biochemically characterised with respect to ester hydrolysis in aqueous medium. The catalytic efficiency of the immobilised lipase, in terms of thermal stability and reusability, was also studied.
Materials and Methods
Materials
Multi-walled carbon nanotubes (MWNTs; length of 0.5-2 micron and outer diameter of 20–30 nm) were purchased from Arry International. All other chemicals used to functionalise MWNTs were purchased from Sigma-Aldrich. Lipase from Thermomyces lanuginosus (EC 3.1.1.3; 100,000 U/g; protein = 22.4 mg/mL), a purified enzyme in a liquid preparation, was obtained from Sigma-Aldrich Chemical Co., Australia. A protein assay kit (Bio-Rad protein dye reagent concentrate) and Tris-buffer were procured from Bio-Rad. p-Nitrophenyl palmitate, p-Nitrophenol, Triton-X-100, Phosphoric acid and Gum acacia, were purchased from Sigma-Aldrich Chemical Co., Australia. Deionised double-distilled water with 18.2 megaohm cm−1resistivity was used in making solutions. All chemicals (analytical grade) were used as received without any further purification.
Functionalisation and Characterisation of MWNTs
The as-received MWNTs were first treated with a 3∶1 v/v mixture of concentrated H2SO4 and HNO3 in a round-bottomed flask, and refluxed at 120°C for 30 min. After cooling to room temperature, the mixture was vacuum-filtered on a 0.2 mm pore Polytetrafluoroethylene (PTFE) membrane and washed with distilled water until no acid residual was present. The oxidised nanotubes were then redispersed and washed in a NaOH solution (0.01 M) followed by washing with distilled water until pH neutral. Finally, the product was redispersed in HCl solution (0.01 M), and repeatedly washed with distilled water until pH of the filtrate was neutral. The resulting oxidised nanotubes (100 mg) were dried in a vacuum oven at 80°C for 8 h and subsequently dispersed in ethylenediamine (EDA, 60 mL) to obtain amino-functionalised carbon nanotubes. The coupling agent, HATU (O-(7-Azabenzotriazol-1-yl)-N,N,N′,N′-tetramethyluroniumhexafluorophosphate, 8 mg) was added to increase the reaction yield and the dispersion was sonicated for 4 h at 40°C. The obtained product was diluted with 300 mL of methanol and vacuum-filtered using a 0.2 mm pore PTFE membrane filter, after which the filtrate was washed extensively with excess methanol following by vacuum drying at 60°C for 8 h. Thermogravimetric analysis (TGA) for pristine MWNTs and amino-functionalised MWNTs was conducted under a nitrogen atmosphere using a Perkin Elmer at a heating rate of 10°C/min.
The FTIR analysis of functionalised nanotubes was carried out to confirm the presence of amino groups in the functionalised carbon nanotubes. ATR-FTIR measurements were conducted using an Alpha FTIR spectrometer (BrukerOptik GmbH, Ettlingen, Germany) equipped with a deuterated triglycine sulfate (DTGS) detector and a single-reflection diamond ATR sampling module (Platinum ATR QuickSnap™). The ATR-FTIR spectra were acquired at 4-cm−1 spectral resolution with 64 co-added scans. Blackman-Harris 3-Term apodization, Power-Spectrum phase correction, and zero-filling factor of 2 were set as default acquisition parameters using the OPUS 6.0 software suite (Bruker). Background spectra of a clean ATR surface were acquired prior to each sample measurement using the same acquisition parameters.
The size and morphology of the amino-functionalised and enzyme conjugated nanotubes were characterised by transmission electron microscopy (TEM) using a JEOL 2100 M microscope (Frenchs forest, NSW, Australia) with an electron beam energy of 200 kV. TEM specimens were prepared by evaporating a drop of aqueous nanotube dispersion on the carbon-coated specimen grid. Once evaporated, the sample was loaded into the microscope for imaging.
Covalent Immobilisation of Enzyme on Functionalised MWNT
Lipase was immobilised on the functionalised nanotubes (Fig. S1). The nanotubes (5 mg/mL) were first sonicated in the aqueous buffer (50 mM, Tris Buffer, pH 9.0) for 30 min to ensure homogenously dispersion. Surface-activation of the amino-functionalised nanotubes was achieved by treating the nanomaterials with 1 M glutaraldehyde solution [13]. Support activation was carried out at 25°C in a shaker (250 rpm) for 1 h. The activated support (5 mg/mL) was removed by centrifugation (7000 rpm, 20 min), washed at least five times with 20 mL of distilled water to remove excess glutaraldehyde, and then washed with washed with assay buffer. Lipase was immobilised onto functionalised nanotubes through covalent linkage between amino group of nanotube and amino group of enzyme through a glutaraldehyde cross-linker. The purified enzyme (5–20 mg in 50 mM Tris buffer, pH 9.0) was mixed with the activated support (5 mg/mL) in an enzyme assay buffer to optimise the nanotube and protein-loading ratio. The immobilisation process was performed at 25°C in a shaker (150 rpm) for 10 h. Non-covalently adsorbed protein was removed thereafter by thorough washings of the nanotubes with saline solution (1 M NaCl) followed by enzyme assay buffer until no hydrolytic activity was detected in the washings. The supernatant was used for protein analysis. The washed carrier was directly used for the determination of enzyme activity and thermal stability.
The amount of immobilised enzyme was calculated by measuring the proportion of the enzyme remaining in the supernatant of the enzyme assay buffer after the immobilisation process. The amount of protein in the supernatant at each washing cycle was added to calculate the total amount of free enzyme until no protein was leached. It was found that the quantity of immobilised lipase was 0.50 mg protein/mg MWNT at equal ratio of protein and functionalised nanotube in mg was achieved using this immobilisation method. Activity retention of the immobilised form was 65% than the free enzyme. Protein content of the enzyme solution, before and after immobilisation, in the washing buffer was determined by the Bradford method with Bio-Rad protein dye reagent concentrate and bovine serum albumin as a standard protein [23].
Structural Characterisation of Immobilised Lipase
The enzyme-immobilised nanotubes were characterised by transmission electron microscopy (TEM). The size and morphology of nanotubes was observed by TEM. The sample for TEM analysis was obtained by placing a drop of well-dispersed nanotubes solution onto a carbon grid coated, followed by drying the sample at ambient temperature.
X-ray photoelectron spectroscopy (XPS) was used to investigate the chemical composition of the pristine, amino-functionalised and enzyme immobilised carbon nanotubes. The spectra were acquired using a Vacuum Generators Escalab V unit equipped with a non-monochromatic A1 Ka source at 200 W (20 mA at 10 kV) and a hemispherical analyser operating in the fixed analyser transmission mode. The photoemission peak areas of each element was normalised by the sensitivity factors of each element tabulated for the spectrophotometer used.
Circular dichroism (CD) spectroscopy was used to monitor the secondary structure of the native lipase and MWNT immobilised lipase. The UV CD spectra (200–260 nm) were recorded on a JASCO J-810 CD instrument (JASCO) with a bandwidth of 0.5 nm and a scan speed of 50 nm/min. Cell length was 10 mm. In all measurements, the lipase concentration was kept at 50 µg/mL. All CD measurements were performed at 25°C in diluted Tris buffer (10 mM, pH adjusted with phosphoric acid to 9.0). The CD spectrum of amino-functionalised MWNT was similarly recorded. All the spectra were corrected by subtracting a blank spectrum (without lipase). Each scan was repeated five times, after which the spectra were averaged.
Determination of Enzyme Activity
The activity of free and immobilised enzyme was measured by a colorimetric method [24]. The reaction mixture contained 80 µL of p-nitrophenyl palmitate (3 mg/mL; p-NP palmitate prepared in isopropyl alcohol), the test sample (lipase), and Tris buffer (0.05 251658240M, pH 9.0) containing 0.4% (w/v) Triton-X-100 and 0.1% (w/v) gum acacia (2.9 mL), to make final volume of 3 251658240mL. The reaction mixture was incubated at 60°C for 10 min in a water bath. The reaction was terminated by holding the reaction mixture at −20°C for 10 251658240min. An appropriate control with a heat-inactivated enzyme (5 min in a boiling-water bath) was included with each assay. The liberated 4-nitrophenol was measured by UV-Vis Spectrophotometer (Shimadzu, Japan) at 410 nm and its concentration calculated from a plot constructed for standard p-nitrophenol. One unit of enzyme activity is defined as 1 µmol of p-nitrophenol liberated per minute under standard assay conditions (pH 9.0, 60°C). Activity of immobilised lipase (20 µg) was measured with p-NP palmitate (equal amounts corresponding to free enzyme) at 60°C. All additives, including the buffer, were pre incubated for a short period (5 min) before the enzyme was added to initiate the reaction. All enzyme assays were performed in triplicate and reported as mean values ±SD.
Biochemical Characterisation of the Free and Immobilised Lipase
The optimum pH for immobilised and free lipase activity was determined using standard assay conditions in Tris buffer at varying pH (pH 7.0–9.5) at 60°C. Relative activities of the free and immobilised lipases at selected range of pH values were quantified relative to the control activities, and expressed as fractions thereof. These control activities, those representing 100% relative activity, were taken to be at pH 9.0 for both the free and immobilised lipases.
The effect of temperature on free and immobilised lipase activity at pH 9.0 was determined by varying the temperature in the 30–80°C range. Other experimental conditions adhered to the standard assay protocol. The activity at 60°C was taken as control for the calculation of 100% relative activity for the free and immobilised lipase.
Determination of Kinetic Parameters
Kinetic parameters of free and immobilised lipase at 60°C were determined using different p-NP palmitate concentrations in the range of 10–60 mM in 50 mM Tris buffer (pH 9.0) respectively. KM and Vmax values of free and immobilised lipases were calculated via non-linear regression fitting of the of the Michaelis-Menten equation using Prism 6 (Graphpad Software, Inc., CA, USA).
Thermal Stability of Free and Immobilised Enzymes
Thermal stability of the free lipase was quantified in terms of the loss in enzyme activity when incubated at selected temperatures (60, 70 and 80°C) in the absence of a substrate. The activity of free lipase at pH 9.0 (Tris buffer, 50 mM) was observed at regular intervals between 30 and150 min. Similarly, to determine the thermostability of the immobilised enzyme, the immobilised lipase was incubated at the above mentioned selected temperatures in the absence of a substrate. After varying periods of time, the residual lipase activity was determined. The relative activity of the free and immobilised lipase without incubation was defined as control and arbitrarily attributed 100% relative activity for each of their respective reactions.
Biocatalyst Reusability Study
The reusability of the immobilised preparation was assessed at 60°C by carrying out the hydrolysis of a long chain ester (p-NP palmitate) under standard assay conditions. After each cycle, the immobilised enzyme was removed by centrifugation (7000 rpm, 20 min). The immobilised lipase was collected and washed simultaneously with deionised water and enzyme assay buffer. In running the second cycle, the immobilised enzyme was resuspended in fresh enzyme assay buffer and added to fresh p-NP palmitate. The activity of the immobilised enzyme after the first cycle was defined as the control and attributed a relative activity of 100%. Each cycle is defined here as the complete hydrolysis of the substrate present in a reaction mixture.
Results and Discussion
The development of an efficient functionalised nanotubes support for enzyme immobilisation, using a covalent binding method for investigating its influence on the biocatalyst structure-function relationships, was the primary objective of the work. Analytical techniques have been used to characterise in situ structural stability of enzymes immobilised on supports [25]. The conformational changes of enzymes upon immobilisation and confirmation of the success of the immobilisation methods have been investigated using sophisticated analytical techniques such as TEM and spectroscopy (CD, FTIR and XPS).
FTIR spectra for pristine MWNT and amino-functionalised MWNT are shown in Figure 1. Since the pristine carbon nanotube is not sensitive to FTIR, no obvious peak is observed. This is similar to previous FTIR findings [26]. The IR spectrum of the amino-functionalised MWNT (MWNT-CO-NH (CH2)2-NH2) is shown in Figure 1. The absorption band at 1635 cm−1 is assigned to the stretching vibration mode of C = O in the amide group. The NH2 stretch band appeared at 3427 cm−1, whereas the peak at 1045 cm−1 is attributed to the C-N bond stretch vibrations. Bands at 2918 and 2848 cm−1 represent the stretching of the CH2 group [27].
Footnote: MWNT treated with a mixture of concentrated H2SO4 and HNO3 (v/v 3∶1), and refluxed at 120°C. After cooling to room temperature, the mixture was vacuum-filtered on a 0.2 mm pore Polytetrafluoroethylene membrane. The oxidised nanotube was washed in a NaOH solution. Finally, the product was redispersed in HCl solution. The obtained oxidised nanotubes were dried in a vacuum oven and then were dispersed in ethylenediamine to obtain amino-functionalised MWNTs. The coupling agent,O-(7-Azabenzotriazol-1-yl)-N,N,N′,N′-tetramethyluroniumhexafluorophosphate was added to increase the yield of reaction and the dispersion was sonicated. The product was diluted with methanol and vacuum-filtered using a 0.2 mm pore PTFE membrane filter, after which the filtrate was washed extensively with methanol following by vacuum drying.
The degree of functionalisation can be determined using Thermal gravimetric analysis (TGA). Figure 2 shows the TGA results for pristine MWNT and amino-functionalised MWNT. There is 4.5% weight loss for pristine MWNT which could be due to the removal of oxidised carbon groups. For amino-functionalised MWNT, the weight loss is about 22% which is attributed to the presence of amino groups on side walls of MWNT. Therefore the degree of functionalisation estimated to be 1 added in every 41 carbons, which is higher than that of amino functionalisation of nanotube through diazotiazation [26]. Identically processed functionalised MWNT with and without the immobilised enzyme were viewed by electron microscopy (Fig. 3). The size and morphology of the nanomaterial was observed by TEM with the same resolution. Increment in the thickness of the sidewall of the functionalised MWNT after covalently immobilised enzyme confirmed the presence of enzyme. Similar observations of uniform coating of the Candida rugosa lipase to the MWNT via physically adsorption were also reported [20].
XPS represents an effective technique for surface analysis [28] and was employed to determine the surface properties of the relative atomic composition of functionalised MWNT to immobilised lipase. High resolution XPS spectra for the as received MWNT, amino-functionalised MWNT and enzyme bound MWNT are shown in Figure 4a,b. Two points per sample were analysed and survey spectra were used to identify all elements present on the sample surfaces and to determine their concentrations. The high-resolution spectra were used to determine the presence or absence of chemically distinct species (e.g. functional groups). As shown in Figure 4a and b, there is a main peak at 284.6 eV for as-received MWNT, due to sp2 C-C bonds of graphitic carbon. Apart from a strong C-C peak, the additional peaks observed for amino-functionalised and enzyme bound MWNTs at higher binding energies are due to bonding of carbon atoms to other functional groups. For the amino-functionalised MWNTs, the additional binding energy at 286.9 eV is attributed to an amide group [29]. The absence of a peak around 288.0 eV also confirms the conversion of the carboxylic acid group to an amide. The binding energy at 401.0 eV in the N1s spectra is assigned to the formation of amides and amines on the carbon nanotubes, which further confirms the success of MWNT functionalisation as well as its covalent bonding to the enzyme. As expected, no peak was observed for the as received MWNT in the N1s spectrum. The atomic concentrations of oxygen and nitrogen in samples based on XPS analyses are presented in Table 1. The higher nitrogen content for the amino-functionalised MWNTs compared to as received nanotubes confirms the presence of amide groups on the surface of the nanotubes. The significant increase in both surface oxygen and nitrogen contents in nanotube bound enzymes indicates the covalent bonding between amino-functionalised MWNT and lipase (Table 1). Compared to that of MWNTs, the spectrum of lipase bound MWNTs shows an increase in the intensity of oxygen. This is attributed to the oxygen atoms in the immobilised lipase. A similar trend is also reported in a recent study of lipase immobilised on magnetic multi-walled carbon nanotubes [30].
The influence of covalent attachments on the secondary structure of enzyme was analysed by CD spectroscopy. The structural change of the immobilised lipase was compared to the free enzyme through CD spectra analysis (Fig. 5). MWNTs contribute to the spectrum of the nanotube bound lipase. The CD Pro software package (CONTIN) was used to interpret the secondary structure fractions. Compared to free enzyme, the amount of α-helix in MWNT-immobilised enzyme decreased, whereas β-sheet and unordered polypeptide amount increased (Table 2). Immobilised lipase retains approximately 80% of its native α- helix content, as obtained from the mean residue ellipticity at 222 nm. The degree of α-helix content of native lipase (63%) was retained after its immobilisation on magnetic multi-walled carbon nanotubes [29], with 62% retention of the α-helix content of the native lipase after immobilisation on multi-walled carbon nanotubes [31]. Recently, the α-helix content of the magnetic nanoparticle immobilised enzyme was not significantly changed and subsequently, the preserved secondary structure of the enzyme following nanoparticle conjugation demonstrated the high catalytic activity as compared to the native enzyme [32]. These results were encouraging where secondary structure changes remained unaffected contributing towards higher stability of the biocatalysts.
Effects of pH and Temperature on the Catalytic Activity of Free and Bound Biocatalyst
The optimum pH value for the activity of both free and immobilised enzymes was found to be 9.0 (Fig. 6a). The immobilised enzyme was comparatively more active at lower pH values as compared to high pH value. This result is consistent with the previously reported study where cyanogen bromide (CNBr) activated octyl-sepharose support was used for immobilising Thermomyces lanuginosus lipase at pH 9.0 [33].
Footnote: The lipolytic activity was determined following the method of Winkler and Stuckmann (1979) [21], using p-NP palmitate as substrate. Bars indicate the standard deviation from triplicate determinations. b) Effect of temperature on the activity of free and immobilised lipase. Footnote: The lipolytic activity was determined following the method of Winkler and Stuckmann [21], using p-NP palmitate as substrate. Bars indicate the standard deviation from triplicate determinations.
Kinetic Parameters
Kinetic parameters of free and immobilised lipase were determined by measuring initial reaction rates for each form with varying amounts of substrates (p-NP palmitate). For all forms, Michaelis-Menten kinetic behaviour was observed. As shown in Table 3, KM value of the immobilized lipase (4.5 mM) was slightly more than that of the free enzyme (3.1 mM). The maximum reaction rates (Vmax) of the free and immobilised enzyme were 20.1 U/mg and 22.9 U/mg. A 4-fold increase in the KM value was observed for the immobilised enzyme compared to free enzyme [36]. KM value of the immobilized Thermomyces lanuginosus lipase on hydrophobic and hydrophilic mesoporous supports was 3.4 and 1.5 mM respectively, compared to a free enzyme value of 0.8 mM. These changes in the kinetic parameters indicate that covalent binding of lipase onto the glutaraldehyde-activated functionalised nanotubes resulted in change of affinity for the substrate. This may be due to slightly decreased access of the substrate to the active site of enzyme in the bound lipase [37].
Thermal Stability of Free and Immobilised Lipase
Figure 7 shows the thermostability of free and immobilised lipases at temperatures of 60, 70 and 80°C, respectively. It is evident that the thermal stability of the lipase immobilised on nanotubes was improved and prominent compared to the free enzyme at 80°C. The free enzyme lost its activity after 2 h of incubation at 80°C, whereas the immobilised lipase retained 57% of its initial activity after 2 h incubation (Fig. 7). This trend is in agreement with the findings reported in the literature. For example, all activity was lost in Thermomyces lanuginosus lipase dissolved in phosphate buffer at 80°C after 2 h and authors claimed the improvement in thermostability of the enzyme using an ionic liquid [38]. The increased stability observed for the immobilised enzyme, either thermal or due to interactions with solvents, observed may be attributed to a reduction in the protein structure mobility, due to anchorage to the support promoted by the covalent bonds and subsequent translation of the rigidity at each anchorage point to the whole enzyme structure, thus shielding it from the denaturing effects of the environment [39].
Footnote: The lipolytic activity was determined following the method of Winkler and Stuckmann [21], using p-NP palmitate as substrate. Bars indicate the standard deviation from triplicate determinations.
In a recent study, the enzyme-carbon nanotube interactions significantly improved the thermal stability and catalytic activity of enzymes and confirmed that a significant confirmation is controlled by the functional group on the nanomaterial’s surface and less on their geometry [19]. Thus, effect of functionalisation agent (ethylenediamine) in conjugation with coupling agent (HATU) to MWNTs, played an important role in improving the reaction yield of amino-functionalisation and subsequently enhanced the catalytic property of immobilised enzyme in this present study. These nanoscale carriers are stable at high temperatures and high enzyme-loadings on MWNT can be achieved [31].
Biocatalyst Reusability Study
The immobilised enzyme retained residual activity above 80% up to the 4th recycle, demonstrating stability up to 10 cycles of 10 min at 60°C, and retaining approximately half of its initial activity at the end the enzymatic derivative (Fig. 8). Pavlidis et al. [19] demonstrated that the lipase (Cal B) activity of the immobilised enzyme in amine-functionalised carbon nanotube preparations retain more than 50% of their activity after five repeated uses at 60°C.This immobilisation method reduces the enzyme leaching into media and decreases protein contamination in the product. Superior reusability of lipase was observed due to nanotube binding, thus presenting a cost-based argument for its potential role in economically viable enzyme catalysed process.
Footnote: The lipolytic activity was determined following the method of Winkler and Stuckmann [21], using p-NP palmitate as substrate. Bars indicate the standard deviation from triplicate determinations. Residual activity of immobilised enzyme at different cycles. 1 cycle = 100±4.2; 2 cycle = 88±3.9; 3 cycle = 84±4.0; 4 cycle = 80±2.9; 5 cycle = 70±3.0; 6 cycle = 64±4.4; 7 cycle = 62±3.9; 8 cycle = 56±4.5; 9 cycle = 54±4.8; 10 cycle = 51±4.3; 11 cycle = 49±4.2.
Conclusion
Successful functionalisation and post immobilisation changes in the enzyme were confirmed at structure-function level using analytical techniques such as TEM and spectroscopy (XPS, CD, FTIR), respectively. The kinetics of immobilised enzyme indicated that the enzyme undergoes a slight change in kinetics parameters during immobilisation, while retaining the same pH and temperature optima of the free lipase. The satisfactory immobilisation yield, improved thermostability, and encouraging reusability of nanotube bound lipase, makes this nanobiocatalyst system of potential interest for biosensor applications.
Supporting Information
Figure S1.
Schematic representation of the covalent immobilisation of enzyme to amino-functionalised MWNT.
https://doi.org/10.1371/journal.pone.0073642.s001
(TIF)
Author Contributions
Conceived and designed the experiments: MP MLV. Performed the experiments: MLV MN. Analyzed the data: MLV MN MP. Contributed reagents/materials/analysis tools: MLV MN CJB MP. Wrote the paper: MLV MN MP.
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