Clay Minerals Change the Toxic Effect of Cadmium on the Activities of Leucine Aminopeptidase

Soil leucine aminopeptidase (LAP) is a hydrolytic enzyme involved in the acquisition of nitrogen by microorganisms. In contaminated soils, LAP activity is affected not only by the type and concentration of heavy metals but also by the form of enzyme. Here, we investigated the degree and mechanism of cadmium (Cd) inhibition of soil LAP and purified LAP. We also examined the effect of montmorillonite and kaolinite on LAP and LAP contaminated with Cd. The results showed that Cd inhibition of LAP activity increased with increasing Cd concentration and that Cd exerted noncompetitive inhibition of LAP. The addition of clay minerals decreases LAP activity and the maximum reaction rate ( V max ), regardless of the presence of Cd. Montmorillonite decreases the affinity of LAP to the substrate ( K m ), while kaolinite increases the affinity of LAP to the substrate. The clay mineral-immobilized LAP showed an increase in resistance to Cd contamination compared with the free LAP. The results obtained in this study may aid in understanding the toxic effects of heavy metals on soil enzymes.


Introduction
Cadmium (Cd) has become one of the most hazardous heavy metals in soil as a result of its potential, persistent, and irreversible toxicity [1][2][3].When Cd enters soil, it affects the environmental health of the soil and the stability of ecosystem, particularly soil microorganisms [4,5].Soil microorganisms are the most active and sensitive component of the soil ecosystem and can secrete most soil extracellular enzymes associated with the soil nutrient cycle [6,7].Since soil enzyme activity is closely related to soil microorganisms and is sensitive to changes in environmental conditions, soil enzyme activity is often used as an indicator to evaluate the level to which heavy metals influence soil microbial function and soil ecosystem health [8][9][10][11][12].
According to previous studies, the soil enzyme activity exponentially decreases with increasing heavy metal concentrations by displacing enzyme conformation-related metals and occupying the active center of the enzyme or by binding to sulfhydryl, amino, and carboxyl groups in the enzyme structure to reduce the active site of the enzyme [13][14][15][16].
However, the extent of soil enzyme activity in response to heavy metals is related not only to the type and concentration of heavy metals but also to the type of soil enzyme and soil properties, such as clay mineral content [17,18].Clay minerals form enzyme complexes whose molecular structure and catalytic properties differ from those of free enzymes, thus affecting the contact of enzymes with heavy metals and substrates [19][20][21].At the same time, heavy metals can interact with clay mineral surfaces and compete with enzymes to form heavy metal-enzyme-clay mineral complexes [22,23].Therefore, free enzymes, soil enzymes, and enzymes immobilized by clay minerals have different response to heavy metal pollution.
Leucine aminopeptidase (LAP, Enzyme Commission number: 3.4.11.1) catalyzes the hydrolysis of leucine and other hydrophobic amino acids at the N-terminus of polypeptides.It is one kind of enzyme involved in the microbial acquisition of N in soil [6].Cd acts as an enzyme inhibitor by replacing the metal associated with the active center of phosphatase [24,25].Additionally, soil properties (e.g., organic C, total N, pH, soil particle size, and clay contents) can influence the toxicity of heavy metals in soil on soil enzymes [26].On this basis, we anticipated that the inhibition of LAP by Cd may be due to the displacement of enzyme conformation-related metals and occupation of the active center of the enzyme; thus, the interaction of clay minerals with LAP might contribute to different Cd toxicity on free LAP, soil LAP, and immobilized LAP.It has been demonstrated that Cd shows exponential or logarithmic inhibition of other hydrolytic enzymes, such as phosphatase and β-glucosidase [27,28].However, the toxicity of Cd to LAP is poorly researched in existing studies, and there is barely any information available on the effects of the interaction between clay minerals and LAP on Cd toxicity.Consequently, we investigated the effect of Cd toxicity on the degree of LAP exposure (free LAP, LAP in soil, and LAP immobilized by clay minerals).A preliminary attempt was also made to investigate the reasons of cadmium toxicity to LAP (with reference to the toxicity of other heavy metals to LAP and experiments on the recovery of activity of Cd-LAP in the presence of Mg and Mn addition) in an attempt to reach the following conclusions: (1) the difference response between free LAP, soil LAP, and clay mineralimmobilized LAP on Cd toxicity and (2) the mechanism of LAP inhibition by Cd.
Our work is a preliminary investigation into the mechanisms of Cd contamination on LAP (soil LAP and purified  Adsorption Science & Technology LAP) and the role that clay minerals play in this process.This provides a theoretical basis for restoring the activity and function of LAP in Cd-contaminated soils, as well as providing some assistance in restoring nitrogen use efficiency and accelerating nitrogen cycling in contaminated soils.

Material and Methods
2.1.Purified Enzyme and Soils.The purified enzyme was purchased from Sigma-Aldrich (product number: L5006, Type IV-S, stored as ammonium sulfate suspension at 4 °C) and volumed with 2.5 mol L -1 (NH 4 ) 2 SO 4 to 5 mL to make an enzyme stock solution.The enzyme stock solution was stored at 4 °C.To make activated enzyme, the enzyme stock solution was diluted with 50 mmol L -1 pH 8 THAM and activated at 37 °C for 2 hours before use.
The soils used in this study are red soil and purple soil, which were collected from the Ecological Experimental Station of Red Soil in Jiangxi, China (28 °15 ′ N, 116 °55 ′ E) and Yanting Station of Chinese Ecosystem Research Network (CERN) in Sichuan, China (31 °16 ′ N, 105 °27 ′ E), respectively.Soil samples were sieved (<2 mm) and stored at 4 °C until enzyme assay.
Soil pH, particle size, organic C, and total N were determined using air-dried soils.The pH was determined using a 1 : 2.5 ratio between the mass of the soil sample and the volume of deionized water.Soil samples were pretreated with 30% H 2 O 2 and 10% HCl to remove organic matter and carbonates, and 0.05 mol L -1 sodium hexametaphosphate was added to disperse the soil aggregates for particle size distribution analysis by Malvern MS 2000 (Malvern Instruments, Malvern, England).The organic C and total N of the soil were determined by using 0.5 mol L -1 HCl to remove carbonates and then analyzed by an element analyzer (Elementar vario MACRO cube, Germany) (Table S1).S2).The surface morphology of clay minerals was analyzed by scanning electron microscopy (SEM) (Thermo Prisma E, Finland) at 20 kV and at a magnification of 3500x (Figure S1).The particle size distribution was determined by a Malvern ZEN 3600 (Malvern Instruments, Malvern, England).The specific surface area (SSA) of clay minerals was analyzed by the N 2 adsorption method [29,30].

Clay
Clay mineral colloid solution (0.5 mg mL -1 ) was prepared by adding 25 mg montmorillonite or kaolinite to 50 mL 50 mmol L -1 pH 8 THAM into a 150 mL beaker and performing ultrasonication for 5 minutes.The activated enzyme was diluted 2500 times using THAM to prepare the LAP working solution.To prepare clay mineral-immobilized LAP, 20 mL of montmorillonite or kaolinite colloids was added to 20 mL of the LAP working solution.The suspension was stirred for 30 minutes at 250 r min -1 at 25 °C before centrifugation at 8000 r min -1 for 5 minutes.The residue was washed with 40 mL deionized (DI) water and centrifuged twice to remove the unabsorbed LAP.Finally, the residue was resuspended in 40 mL of 50 mmol L -1 pH 8 THAM buffer.The clay mineral-immobilized LAP was mixed thoroughly before being added to a 96-well plate.
The soil LAP activity was determined as previously described [31,32].Briefly, a soil homogenate was prepared by stirring 0.5 g fresh soil and 120 mL DI water at 600 rpm for 30 minutes.Then, the homogenate was placed into the assay well (including 50 μL THAM buffer, 100 μL homogenate, and 50 μL L-leucine-AMC) and quenched well (including 50 μL THAM buffer, 100 μL homogenate, and 50 μL AMC).DI water was used in place of homogenate in a standard well (including 50 μL THAM buffer, 100 μL DI water, and 50 μL AMC) and substrate control well (including 50 μL THAM buffer, 100 μL DI water, and 50 μL L-leucine-AMC).THAM, AMC, and L-leucine-AMC were then added sequentially according to the type of well.The THAM concentration in all wells was 20 mmol L -1 , and the L-leucine-AMC was 200 μmol L -1 .The concentration of AMC was 10 μmol L -1 before being added.The mixture in 96-well plates was incubated for 1 h at 37 °C before being read by a fluorometer (Thermo Varioskan™ LUX, Finland) with 365 nm excitation and a 450 nm emission filter immediately.
For the purified enzyme and immobilized enzyme, the soil homogenate in the above method was replaced with the LAP working solution and clay mineral-immobilized enzyme LAP, respectively.The purified enzyme was incubated and measured under the same conditions as the soil.Different capital letters indicate significant differences in V max (P < 0:05), and different lowercase letters indicate significant differences in K m (P < 0:05), with V max in nmol μg -1 h -1 in purified enzyme and nmol g -1 h -1 in soil enzyme and K m in μmol L -1 .Tables 2-4 are the same.
3 Adsorption Science & Technology 2.3.2.Effect of Clay Minerals on LAP.For soil LAP, the effect of clay mineral addition on Cd toxicity was investigated in the natural state (0 mg clay mineral addition), low concentration (50 mg montmorillonite or kaolinite per gram fresh soil), and high concentration (100 mg montmorillonite or kaolinite per gram fresh soil).Clay minerals are added by mixing the corresponding quality and type of clay minerals with red and purple soil to produce homogenate.
For the purified enzyme experiment, the following levels of binding of clay minerals to enzymes were set to investigate Changes in kinetic constants (V max and K m ) of soil LAP and purified LAP were compared at final Cd concentrations of 0, 4, and 10 μmol L -1 to infer the type of inhibition of LAP by Cd.The enzyme activities of soil LAP and purified LAP were determined at different concentrations of substrate (final concentrations of 0, 10, 20, 40, 100, 200, 300, and 400 μmol L -1 , respectively), and V max and K m were calculated using the Michaelis-Menten equation.
In order to have a more insightful understanding of the inhibitory effect of Cd on LAP, we chose argentum (Ag) and hydrargyrum (Hg), which are both inhibitory metals to hydrolase like Cd, as a reference to observe the inhibitory   5 Adsorption Science & Technology effect and type of LAP inhibition by different inhibitory metals.We also chose cobalt (Co) and boron (B), which are accelerators of hydrolase, and magnesium (Mg) and manganese (Mn), metals that can occupy and substitute metal ions at two exchangeable sites in LAP to affect K m , to observe the effect of different metals on LAP activity under the same conditions [33][34][35][36][37][38].
Additionally, the recovery of Cd-contaminated LAP activity by the addition of Mg and Mn was used to infer the mechanism of Cd inhibition of LAP [37].In the recovery  experiment, after measuring the LAP activity inhibited by Cd, Mg and Mn solutions at a final concentration of 4 μmol L -1 were added to observe the change in LAP activity.

Data Analysis
2.4.1.Enzyme Activity.Soil LAP activity was expressed in units of nmol AMC•g -1 •h -1 and calculated by the following equations which were modified from Deforest [31] and Wang et al. [32]: where Net fluorescence is the actual fluorescence value of AMC produced by the enzymatic reaction of LAP in soil, which can be calculated by equation (2); V is the total volume of homogenate, 120 mL for this experiment; the Emission coefficient indicates the fluorescence value per unit AMC (nmol), which can be calculated by equation (4); v is the volume of homogenate in a single incubation well, 0.1 mL for this experiment; T is incubation time, 1 h for purple soil and purified LAP, 3 h for red soil; DM is the dry soil mass corresponding to 0.5 g of fresh soil.
where f is the fluorescence value measured by the marked well; the Quench coefficient indicates the effect of soil on the fluorescence values of AMC, which can be calculated by Emission coefficient fluorescence nmol Purified LAP activity was expressed in units of nmol AMC Inhibition Ratio and Type of Inhibition.Variation of the maximum rate of reaction (V max ) and the Michaelis constant (K m ) could deduce the type of inhibition of enzymatic reactions by inhibitors [35].
To better describe and compare the inhibition of LAP by different inhibitors (Cd, clay minerals, and other ion), the inhibition ratio was expressed by following equations from Acosta-Martínez [39]: The type of inhibition of LAP by the inhibitor can be known from the change in kinetic constants K m and V max , which can be calculated according to the Michaelis-Menten equation ( 7) and the Lineweaver-Burk double-reciprocal equation ( 8) [40,41]: where v is the initial reaction rate at the substrate concentration ½S; V max is the maximum rate of reaction and K m is the Michaelis constant.    of replicates n ≥ 3), with different letters indicating significant differences.The dependences of enzyme activity with substrate concentration were represented with the Michaelis-Menten equations.The fitting and calculation of kinetic constants were performed using a nonlinear fitting equation (Growth/Sigmoidal Hill) in OriginPro 9.1 (OriginLab Corp., Northampton, MA, USA).

Results and Discussion
3.1.Effect of Cd and Other Ions on LAP.Cadmium inhibited both soil LAP and purified LAP.The inhibition ratio of Cd on LAP increased sharply with increasing Cd concentration in the range of 0-200 μmol L -1 , and the inhibition ratio showed a logarithmic increase (Figure 1(a)).This is consistent with the findings that Cd is a strong inhibitor of LAP in both biochemical and soil studies [27,41,42].When contaminated with low concentrations of Cd (Cd concentration less than 10 μmol L -1 ), LAP in red soil was more sensitive to Cd than that in purple soil, while LAP in both soils responded equally to Cd contamination when Cd was greater than 10 μmol L -1 (Figures 1(a), 1(c), and 1(d)).This indicates that the pH of soil may influence Cd toxicity when the Cd concentration is less than 10 μmol L -1 .At low Cd concentrations, the effective Cd concentration in the soil also depends on the concentration of Cd being adsorbed.When soil pH is low, soil components such as clay minerals and organic matter are less able to sorb Cd and are less likely to produce Cd(OH) 2 precipitation, so more Cd 2+ is free in the soil solution; therefore, Cd toxicity is likely to be greater [43,44].In contrast, at higher Cd concentrations, soil properties, including pH (Table S1), did not affect Cd toxicity to soil LAP.The weaker inhibition of Cd on soil LAP than on purified LAP may be due to the adsorption of Cd by sorbent substances in soil homogenate, resulting in a lower effective concentration of Cd [45,46].Another explanation may be that certain components of the soil form a protective effect on LAP, resulting in a reduction in the toxicity of Cd to LAP [47].
Enzyme kinetic analysis indicated that Cd may be a noncompetitive inhibitor of both purified LAP and soil LAP (Figures 1(b)-1(d)).After the addition of 4 and 10 μmol L -1 of Cd, V max for the enzymatic reaction of soil LAP and purified LAP decreased, while no significant difference was observed in K m (Table 1).This indicates that the addition of Cd only reduced the effective amount of the enzyme without reducing the affinity between the enzyme and the substrate.It can be inferred that Cd disrupts the conformation on LAP and thus renders some LAP inactive [26,27].
The inhibitory effect of Cd on LAP activity was comparable Ag and Hg but stronger than that of Co, B, Mg, and Mn (Figures S2-S4).Generally, the effect of Ag on soil LAP and purified LAP was similar to that of Cd.Soil LAP and purified LAP activities were strongly inhibited by Ag.The inhibitory effect of Hg on LAP at the same concentration was slightly greater than that of Cd.Accelerator metal Co promoted soil LAP and purified LAP activities at low concentrations and inhibited them at high concentrations.The inflection points for purified LAP and LAP in red soil were 250 and 200 μmol L -1 , respectively.B, Mg, and Mn had little effect on LAP activities.The purified enzyme responded most strongly to their inhibition, relative to the two soil LAP contaminated by Cd; Ag and Hg had a noncompetitive inhibition on both LAP in purple soil and purified LAP (Figure 2, Tables S3-S5).Nevertheless, we also observed competitive inhibition  of Hg on LAP in the red soil, indicating that other isozyme may exist in the red soil compared with the purified LAP and LAP in the purple soil.The addition of Mg and Mn, which are metals in the active site of LAP [5,6], cannot restore the activity of purified LAP contaminated by Cd, and the addition of Mg and Mn only slightly changed the activity of LAP in red soil and purple soil (Figure 3).This suggests that Mg and Mn cannot effectively restore the activity of LAP by competing with Cd for the divalent metal sites on LAP.

Effect of Clay Minerals on LAP.
Clay minerals showed different effects on LAP activity (Figure 4).The addition of clay minerals does not significantly affect the activity of purified LAP (Figure 4(a)).In the soil system (Figures 4(b) and 4(c)), the addition of montmorillonite significantly reduced  the LAP activity in red soil and purple soil (P < 0:05).The greater the amount of montmorillonite added, the lower the enzyme activity.When the amount of montmorillonite was 50 and 100 mg g -1 soil, the inhibition rate of LAP in red soil was 30.96% and 36.42% and was 10.77% and 22.78% in purple soil.The addition of kaolinite had no significant effect on LAP activity.The different effects of the two clay minerals may be attributed to the fact that montmorillonite in the 2 : 1 layer has a higher specific surface area and adsorption capacity than kaolinite in the 1 : 1 layer-type structure (Figure S1 and Table S2).Thus, montmorillonite can mask some of the active sites by adsorption on LAP, resulting in a decrease in LAP activity [22].
Different lowercase letters a and b indicate significant differences in LAP activities caused by montmorillonite, and a ′ and b ′ indicate kaolinite.
Figure 5 shows the effect of adding clay minerals on the kinetics of soil LAP and purified LAP.The addition of low concentrations of montmorillonite and kaolinite (0.5 mg L -1 for purified LAP and 50 mg g -1 soil for soil LAP) resulted in a decreasing trend in V max values for both soil LAP and purified LAP, with only the addition of montmorillonite to the purple clay producing a significant decrease in V max (Table 2).When the substrate concentration was relatively low (concentration less than 200 μmol L -1 ), the enzyme activity decreased significantly after clay mineral addition (Figure 4), and the addition of both montmorillonite and kaolinite changed the K m value of the purified enzyme (Table 2), indicating that the affinity of LAP and substrates decreased in the presence of clay minerals.Clay minerals reduce enzyme activity because the adsorption of the mineral to the enzyme changes the conformational structure of the protein, ultimately altering its catalytic properties and reducing its activity and V max [48].
Clay minerals still had an effect on LAP activity with Cd contamination (Figure 6).Adding montmorillonite or kaolinite will cause a decrease in LAP activity, but there is no statistically significant difference in this decreasing trend, and in general, the greater the amount of clay mineral added, the greater the reduction in enzyme activity [49,50].This suggests that the presence or absence of Cd had no effect on the ability of the clay minerals to reduce enzyme activity (Figures 4 and 6).According to Figures 6(a) and 6(d), the addition of clay minerals had almost no effect on the enzymatic activity of purified LAP (0 μmol L -1 Cd); in the presence of Cd contamination with concentrations of 4 μmol L -1 and 10 μmol L -1 , the inhibition rate of Cd on LAP increases significantly with the addition of clay minerals.
In contrast, the inhibitory effect of Cd on LAP in red and purple soil did not increase significantly with the addition of clay minerals.The reason might be that soil enzymes are in different environments than the purified enzyme.There are only buffer, substrate, metal solution, and enzyme in the purified enzyme incubation systems.Thus, this system can be regarded as a homogeneous liquid wherein the metal ions and enzyme could diffuse easily.Clay minerals may adsorb and concentrate the enzyme and Cd ions from the dispersion system on their surface, which increases the chance of Cd-enzyme interaction and the inhibitive effect of Cd on LAP.
Lowercase letters a and b indicate significant differences in LAP activities caused by 0 μmol L -1 Cd, and a ′ and b ′ or a ″ and b ″ indicate significant differences in LAP activities caused by 4 and 10 μmol L -1 Cd, respectively.
According to Tables 1 and 2, the addition of clay minerals decreased the enzyme activity and V max of LAP, and the kinetic constants of LAP were affected by both clay minerals and Cd.The decrease in V max of the purified enzyme was mainly caused by Cd, but when Cd and clay minerals were present together, the clay minerals exacerbated the inhibitory effect of Cd, and the effect of kaolinite was stronger than that of montmorillonite (Figure 7 and Table 3).K m in purple soil was not affected by the addition of Cd or clay minerals, but, in both the purified enzyme and in the red soil, it was concluded that montmorillonite decreased the affinity of LAP to the substrate and kaolinite increased the affinity of LAP to the substrate.It can be concluded that the presence of both Cd and clay minerals in the purified enzyme system amplifies the inhibitory effect of Cd on LAP, possibly due to the ability of clay minerals to adsorb LAP and Cd [51].The reason for the different results observed in the two soils is that the type and content of clay minerals differ between the red and purple soils, and these differences make a difference in the effect of Cd on LAP contamination [47].

Effect of Cd on Immobilized LAP.
As shown in Figure 8 and Table 4, the montmorillonite-immobilized enzyme showed a nonsignificant decreasing trend in V max with increasing Cd concentration under the influence of 0, 4, and 10 μmol L -1 Cd, while the kaolinite-immobilized enzyme did not differ significantly under the three concentrations of Cd contamination.No significant change in K m was observed for the enzymes immobilized by the two clay minerals.Comparison with the kinetic constants of the purified LAP (free enzyme) in Figure 1(b) and Table 1 shows that 11 Adsorption Science & Technology the significant increase in K m of the immobilized enzyme suggests that the presence of clay minerals reduces the affinity between the enzyme and the substrate.When the free LAP was contaminated with 10 μmol L -1 of Cd, V max of the free LAP decreased to 63.29% and K m became 161.19% of that of the uncontaminated enzyme, respectively.In contrast, V max of montmorillonite-immobilized enzyme and kaolinite-immobilized enzyme changed to 70.89% and 119.35% of those when they were not contaminated, respectively, and K m changed to 119.12% and 109.34%,respectively.This indicates that the immobilized enzymes showed less change in V max and K m when contaminated with Cd, and therefore, the clay mineral-immobilized LAPs were more resistant to Cd contamination [49,[51][52][53].
The difference in the immobilized enzyme and free enzyme can also explain the difference in the response of soil LAP and purified LAP to Cd contamination.Clay mineralimmobilized enzymes are more resistant to Cd toxicity than free enzymes, so the same concentration of Cd inhibits the clay mineral-immobilized enzyme less than the free enzyme, which is why the inhibition ratio of soil enzymes under the same concentration of Cd is lower than that of purified enzyme.Since soil enzymes are a mixture of free and immobilized enzymes, the sensitivity of soil enzymes to Cd contamination should be somewhere between free and immobilized enzymes, and therefore, the inhibition rate of soil enzymes is usually lower than that of purified enzymes (free enzymes) when faced with the same concentration of Cd contamination.

Conclusion
The inhibitory effect of Cd on LAP increased logarithmically with the increasing Cd concentration, and Cd produced noncompetitive inhibition on both soil LAP and purified LAP.Cd inhibited the enzymatic reaction by disrupting the conformation of the enzyme protein, which cannot be restored by adding the metals associated with the LAP active site.Regardless of the presence of Cd, the addition of clay minerals will generally reduce the activity and maximum reaction rate (V max ) of LAP, and the effect of montmorillonite is stronger than that of kaolinite.Montmorillonite decreases the affinity between LAP and the substrate (increasing K m ), while kaolinite increases the affinity between LAP and the substrate (decreasing K m ).It should be noted that clay minerals can increase the inhibition ratio of Cd on purified LAP.The interaction between leucine aminopeptidase, clay minerals, and cadmium contamination in the soil is a complicated process that is related not only to the concentration of the three but also to the soil environment.Therefore, the process and mechanism by which clay minerals affect the toxicity of Cd to LAP are still unclear.In consequence, it is important to continue to study the interaction between clay minerals, Cd and LAP, and the inhibition mechanism of Cd on clay mineral-immobilized LAP.This can provide scientific evidence for restoring the activity and function of LAP in Cd-contaminated soils and to provide some help in restoring nutrient use efficiency and accelerating nutrient cycling in contaminated soils.

Figure 1 :
Figure 1: Effect of Cd on the inhibition rate and kinetic constants of LAP: (a) inhibition rate of soil LAP and purified LAP by different concentrations of Cd; (b) kinetic curve of purified enzyme affected by Cd; (c) kinetic curve of LAP in red soil affected by Cd; (d) kinetic curve of LAP in purple soil affected by Cd.

Figure 3 :
Figure 3: Proportion of change in the activity of Cd-contaminated LAP after the addition of Mg and Mn as restorative activators of LAP.

Figure 4 :
Figure 4: Effect of adding different amounts of montmorillonite and kaolinite on LAP activity in purified LAP, LAP in red soil, and LAP in purple soil.

Figure 5 :
Figure 5: Effect of adding different amounts of montmorillonite and kaolinite on the kinetic curve of LAP in purified LAP, LAP in red soil, and LAP in purple soil.

Figure 6 :
Figure 6: Effect of montmorillonite and kaolinite on the activity of purified LAP, LAP in red soil, and LAP in purple soil in the presence of 0, 4, and 10 μmol L -1 Cd.

Figure 7 :
Figure 7: Effect of montmorillonite and kaolinite on the kinetic curves of purified LAP, LAP in red soil, and LAP in purple soil in the presence of 10 μmol L -1 Cd.

Figure 8 :
Figure 8: Effect of Cd on the kinetics curves of montmorillonite-immobilized LAP and kaolinite-immobilized LAP.

Table 1 :
Changes in the kinetic constants (V max and K m ) of LAP by different concentrations of Cd.

Table 2 :
Changes in the kinetic constants (V max and K m ) of LAP by montmorillonite and kaolinite.

Table 3 :
Changes in the kinetic constants (V max and K m ) of LAP by montmorillonite and kaolinite with 10 μmol L -1 Cd contamination.

Table 4 :
Changes in the kinetic constants (V max and K m ) of montmorillonite-immobilized LAP and kaolinite-immobilized LAP with 0, 4, and 10 μmol L -1 Cd contamination.