Adsorption of Extracellular Polymeric Substances Derived from S. cerevisiae to Ceria Nanoparticles and the Effects on Their Colloidal Stability

In order to understand the adsorption preferences of extracellular polymeric substances (EPS) components derived from fungus Saccharomyces cerevisiae on sparingly soluble CeO2 nanoparticles (CeNPs), the adsorption experiments of the EPS including organic matter with low molecular weight have been performed at pH 6.0 at room temperature (25 ± 1 ◦C). The subsequent effects of the coating on the dispersibility of CeNPs was systematically measured as a function of time and ionic strength ranging from 1 to 1000 mmol L−1. Among the EPS and other components, orthophosphate and saccharides preferentially adsorb onto CeNPs, and proteins are the only major N-compounds adsorbing onto the CeNP surfaces. Adsorption of orthophosphate resulted in a dramatic decrease in ζ potential to −40 mV at pH > 5, whereas the EPS adsorption suppressed the deviation of ζ potential within a narrow range (−20–+20 mV) at pHs ranging from 3 to 11. Critical aggregation concentrations (CAC) of an electrolyte (NaCl), inorganic orthophosphate, and EPS solutions are 0.01, 0.14, and 0.25 mol L−1, respectively, indicating that the EPS adsorption suppresses aggregation of CeNPs by the electrostatic repulsive forces derived from the adsorbed orthophosphate and the steric barrier formed by organic matter on the nanoparticle surfaces. Therefore, the EPS derived from fungus S. cerevisiae can potentially enhance colloidal dispersibility of CeNPs at circumneutral pH.

Groundwater colloid transport, even at the nano-scale, is generally governed by the hydrology and geochemistry of the subsurface, although very different principals often apply in the nano-scale relative to larger colloids. The mobility of nano-scale colloids in subsurface environments are often delicately dependent on their physico-chemical properties such as their size and shape, including surface topography, as well as surface charge, attached ligands, and aggregation state. In such processes, for 10 min. For comparison, three kinds of solutions were prepared; (i) 1 mM NaCl solution (Control); (ii) 1 mM NaCl + 0.16 mM H 3 PO 4 solution (inorganic H 3 PO 4 ), of which the P concentration is the same as that in the EPS solution; and (iii) EPS solution that contains 1 mM NaCl solution due to the condition during the extraction procedure. The pH of these suspensions was adjusted to 6.0 ± 0.1 by mixing 1.0 mol L −1 NaOH solution at the appropriate proportion. 30 mL portions of these solutions were added to an aliquot of CeNPs stock solution in such a way that the concentration of CeNPs was adjusted to 10 or 100 mg L −1 . The CeNPs concentrations were chosen for measurements using multi analytical techniques. The 3.0 mL of the supernatants was sampled at 0, 0.16, 0.5, 1, 3, 6, 13, 18, and 24 h. The suspension was filtered through a 10 kDa ultrafiltration unit (Amicon Ultra, Millipore Ltd., Carrigtwohill, Ireland). Prior to separation, the filter unit was thoroughly washed with 0.1 mol L −1 NaOH solution and Milli-Q water to remove trace glycerin from the ultrafiltration unit. The ultrafiltration was completed using an Eppendorf ultracentrifuge system at 13,400 rpm (maximum rotation speed) that generates 12,100 G, and the filtrate was used for the subsequent solution analyses. To determine the amount of organic matter and phosphorous that adsorbed on CeNPs, the concentrations of DOC and total P in the filtrate were measured by the same analytical methods described in the previous section. For the ATR-FTIR and X-ray photoelectron spectroscopy (XPS) analyses on the adsorbed EPS, either 200 mL or 2000 mL of three different solutions was added to aliquots of CeNPs stock solutions in such a way that the concentration of CeNPs was 10 or 100 mg L −1 at pH 6.0. These suspensions were batch (statically) reacted for 24 h, and collected by using a 0.025 µm nitrocellulose membrane filter (VSWP04700, ADVANTEC MFS, Inc., Dublin, CA, USA). Then, the residue was rinsed thoroughly with ultra-pure water, and dehydrated at 70 • C in a thermostatic oven overnight. The ATR-FTIR measurement of EPS adsorbed on CeNPs was completed using the same procedure as described in the previous section. The XPS analysis of both EPS and EPS adsorbed onto CeNPs was performed on a ESCA 5800 (ULVAC-PHI Inc., Chigasaki, Japan) system. The binding energies of each spectrum were calibrated by shifting the main O 1s peak to 529.0 eV. The zeta (ζ) potential was measured for the CeNPs suspensions (100 ppm or 10 ppm) in 1 mM NaCl solution using a Zeta Sizer Nano ZS (Malvern Instruments Inc., Worcestershire, UK). The pH was first adjusted to 6.0 and adjusted to the targeted value by using NaOH or HNO 3 .

Aggregation and Sedimentation
Prior to the aggregation and sedimentation experiments, the stock suspension was sonicated for 10 min. Three solutions, (i)~(iii) were added to aliquots of CeNPs stock solution to adjust the concentration of CeNPs to 100 mg L −1 . The colloidal size was intermittently measured during the aggregation process using dynamic light scattering (DLS; ELSZ-2PS, Otsuka Electronics Co. Ltd., Osaka, Japan). The dynamic aggregation process was monitored using a UV-vis spectrophotometer (V-530; JASCO, Tokyo, Japan), measuring the back scattering intensity of the CeNPs at 340 nm in the solutions as a function of time. The absorbance was measured every 5 s for 10 min. The longer period was not considered in this study to eliminate the effects of deposition processes so that the results can be simply interpreted as aggregation process based on the Mie theory (see Appendix A). The scattering intensity depends on the concentration of particles in the solvent and the particle size. In the present experiment, the effect of particle size on the absorbance is negligibly small according to the Mie theory as discussed in the Appendix A. Thus, the absorbance changes depend only on the particle concentration. In general, the time-dependent decrease in the concentration of particles (particles per cm 3 ) in a mono-dispersed suspension due to collisions by Brownian motion can be represented by a second-order rate law: 1 where K p is the rate constant (cm 3 s −1 ). N(t) is the number of particles (particles cm −3 ) at the reaction time, t. N 0 is the initial number of particles. Because, in the present experiment, the absorbance is directly correlated with only the concentration of CeNPs, the term N in Equation (1) can be replaced by the absorbance, A, with the modified coefficient K p as follows: The critical aggregation concentration (CAC) was determined for the conditions (i)~(iii) based on the K p plot as a function of the electrolyte (NaCl) concentration ranging from 1 to 1000 mmol L −1 to compare the effects of EPS with that of other substances. In the diagram, the electrolyte concentration showing the maximum reduction in absorbance was assigned to be the CAC. Table 1 summarizes the composition of the EPS in 1.0 mmol L −1 NaCl after 72 h of incubation for yeast to release EPS, showing that the EPS is mainly composed of~70 mg L −1 organic carbon, 0.50 mmol L −1 K + , and~0.16 mmol L −1 total phosphorous including~0.12 mmol L −1 orthophosphate. The Na + concentration does not represent sodium release from the yeast, but the sodium initially added to the solution to adjust the ionic strength. The fraction of orthophosphate is approximately 80% in the total P concentration and the rest is P associated with organic compounds. Masaki and others have already reported that the dissolved organic matter in the EPS consists of various species as determined by HPLC [29].

Compound Concentration
Dissolved organic carbon 72 ± 20 mg L −1 Dissolved nitrogen 42 ± 11 mg L −1 Total phosphate 0.16 ± 0.07 mmol L −1 Orthophosphate 0.12 ± 0.02 mmol L −1 K + 0.49 ± 0.03 mmol L −1 Figure 1 shows the ATR-FTIR spectra of EPS prior to contact with CeNPs. The band assignments are summarized in Table 2, along with supporting references. A large absorption band at 1374 cm −1 corresponds to symmetric stretching of COO-groups (ν s C-O) that are derived from proteins and carboxylated polysaccharides [30]. The band at~1600 cm −1 corresponds to the stretching vibration of C=O groups in amide I (amides associated with proteins). The band at~1514 cm −1 corresponds to the stretching vibration of C-N groups and deformation vibrations of N-H groups in amide II (-CO-NHof proteins) [31]. These bands at 1600 and 1514 cm −1 indicate the presence of proteins in the EPS. The band at~1110 cm −1 corresponds to ring vibrations of C-O-C in polysaccharides and stretching vibrations of P=O bonds in proton dissociated orthophosphate. In addition, the band at~1044 cm −1 corresponds to symmetric stretching vibrations of P=O in the phosphoryl group. It should be noted that the phosphate bands overlap the band of polysaccharide vibrations and these features are difficult to separate; nevertheless, it is concluded that polysaccharides and phosphoryl species can be identified as the EPS constituents released from S. cerevisiae. These species are also contained in the EPS released from other microorganisms [32][33][34].   Figure 1 shows the ATR-FTIR spectra of EPS prior to contact with CeNPs. The band assignments are summarized in Table 2, along with supporting references. A large absorption band at 1374 cm −1 corresponds to symmetric stretching of COO-groups (νs C-O) that are derived from proteins and carboxylated polysaccharides [30]. The band at ~1600 cm −1 corresponds to the stretching vibration of C=O groups in amide I (amides associated with proteins). The band at ~1514 cm −1 corresponds to the stretching vibration of C-N groups and deformation vibrations of N-H groups in amide II (-CO-NHof proteins) [31]. These bands at 1600 and 1514 cm −1 indicate the presence of proteins in the EPS. The band at ~1110 cm −1 corresponds to ring vibrations of C-O-C in polysaccharides and stretching vibrations of P=O bonds in proton dissociated orthophosphate. In addition, the band at ~1044 cm −1 corresponds to symmetric stretching vibrations of P=O in the phosphoryl group. It should be noted that the phosphate bands overlap the band of polysaccharide vibrations and these features are difficult to separate; nevertheless, it is concluded that polysaccharides and phosphoryl species can be identified as the EPS constituents released from S. cerevisiae. These species are also contained in the EPS released from other microorganisms [32][33][34].    Figure 2 shows the XPS spectra of the EPS prior to the adsorption to CeNPs. Based on a peak assignment proposed by Badireddy and others [37], the C 1s peak (Figure 2A) was resolved into four component peaks, which were assigned as follows: (i) the peak at 284.8 eV is attributed to C-(C, H) in lipids, amino acid side chains, or saccharide ring chains; (ii) the peak at 286.2 eV is derived from C-(O, N) that is associated with alcohol, ester, amine, or amide; (iii) the peak at 287.8 eV is assigned to C=O or O-C-O, which is included in carboxylate, carbonyl, amide, or hemiacetal; (iv) the peak at 289.0 eV arises from O=C-OH and O=C-OR, commonly found in carbonyl or ester groups. The O 1s peak ( Figure 2B) was decomposed into two peaks: the peak at 531.3 eV is mainly a contribution from O=C, as in carboxylate, carbonyl, ester, or amide, whereas the peak at 532.7 eV is assigned to O-(C, H), including hydroxide, acetal, and hemiacetal. Identification of acetal, hemiacetal, and hydroxide indicates the presence of carbohydrates, while carboxylate and carboxyl groups most likely represent the presence of proteins and acidic carbohydrates [37].  [30,35], 3 [36].
Environments 2017, 4, 48 6 of 18 Figure 2 shows the XPS spectra of the EPS prior to the adsorption to CeNPs. Based on a peak assignment proposed by Badireddy and others [37], the C 1s peak (Figure 2A) was resolved into four component peaks, which were assigned as follows: (i) the peak at 284.8 eV is attributed to C-(C, H) in lipids, amino acid side chains, or saccharide ring chains; (ii) the peak at 286.2 eV is derived from C-(O, N) that is associated with alcohol, ester, amine, or amide; (iii) the peak at 287.8 eV is assigned to C=O or O-C-O, which is included in carboxylate, carbonyl, amide, or hemiacetal; (iv) the peak at 289.0 eV arises from O=C-OH and O=C-OR, commonly found in carbonyl or ester groups. The O 1s peak ( Figure 2B) was decomposed into two peaks: the peak at 531.3 eV is mainly a contribution from O=C, as in carboxylate, carbonyl, ester, or amide, whereas the peak at 532.7 eV is assigned to O-(C, H), including hydroxide, acetal, and hemiacetal. Identification of acetal, hemiacetal, and hydroxide indicates the presence of carbohydrates, while carboxylate and carboxyl groups most likely represent the presence of proteins and acidic carbohydrates [37]. The N 1s peak was also resolved into two component peaks ( Figure 2C). The peak at 399.6 eV can be assigned to nonprotonated nitrogen, Nnonpr, such as in amines and amides, and the other peak at 401.3 eV is mainly ascribed to protonated amines, Npr [37]. Since the EPS specimen for the present XPS analysis was prepared after adjusting the pH of the EPS solution to 6.0, the amount of nonprotonated amine groups in the EPS is minimal. Thus, the peak at 399.6 eV is mainly derived from amides.
It was difficult to resolve the P 2p peak due to low intensity ( Figure 2D). However, two peaks typically appear at 133.2 eV and 134.2 eV, which are derived from orthophosphate and phosphoryl group such as adenosine monophosphate, respectively. The peak assigned to phosphoryl group was not observed in this analysis because most of the phosphorus compounds in the EPS is orthophosphate ( Table 1). The concentration of phosphoryl group in the EPS was too low to further analyze the peak in detail. Consequently, the results of XPS analyses suggest that the EPS released The N 1s peak was also resolved into two component peaks ( Figure 2C). The peak at 399.6 eV can be assigned to nonprotonated nitrogen, N nonpr , such as in amines and amides, and the other peak at 401.3 eV is mainly ascribed to protonated amines, N pr [37]. Since the EPS specimen for the present XPS analysis was prepared after adjusting the pH of the EPS solution to 6.0, the amount of nonprotonated amine groups in the EPS is minimal. Thus, the peak at 399.6 eV is mainly derived from amides.
It was difficult to resolve the P 2p peak due to low intensity ( Figure 2D). However, two peaks typically appear at 133.2 eV and 134.2 eV, which are derived from orthophosphate and phosphoryl group such as adenosine monophosphate, respectively. The peak assigned to phosphoryl group was not observed in this analysis because most of the phosphorus compounds in the EPS is orthophosphate ( Table 1). The concentration of phosphoryl group in the EPS was too low to further analyze the peak in detail. Consequently, the results of XPS analyses suggest that the EPS released from S. cerevisiae is composed of lipids, proteins, saccharides, amines, and orthophosphate, which is consistent with the results of FTIR. On the other hand, the functional groups of EPS determined by both methods are not inconsistent with typical functional groups of the cell surfaces described in previous reports [38,39].

Adsorption of EPS on CeNPs
Adsorption measurements of DOC and phosphate on CeNPs at pH 6.0 reached apparent equilibrium within only ten minutes both in the solutions with 10 mg L −1 ( Figure 3A) and 100 mg L −1 ( Figure 3B). The amount of adsorbed species per unit surface area on 10 mg L −1 of CeNPs was about an order of magnitude greater than that on 100 mg L −1 of CeNPs. This is because the number of availabel adsorption sites decreased for CeNPs at 100 mg L −1 concentration due to aggregation at this high particle concentration. both methods are not inconsistent with typical functional groups of the cell surfaces described in previous reports [38,39].

Adsorption of EPS on CeNPs
Adsorption measurements of DOC and phosphate on CeNPs at pH 6.0 reached apparent equilibrium within only ten minutes both in the solutions with 10 mg L −1 ( Figure 3A) and 100 mg L −1 ( Figure 3B). The amount of adsorbed species per unit surface area on 10 mg L −1 of CeNPs was about an order of magnitude greater than that on 100 mg L −1 of CeNPs. This is because the number of available adsorption sites decreased for CeNPs at 100 mg L −1 concentration due to aggregation at this high particle concentration.   Figure 4B) adsorbed onto CeNPs as a function of pH after 1 h of the adsorption experiment. The amount of adsorbed DOC exhibited maximum content at pH 8 at the level of ~4 mmol/m 2 . There was no pH dependence for the adsorption of inorganic phosphate; however, adsorption of phosphorus species derived from the EPS revealed similar pH dependency to that of DOC (Figure 4), despite that the majority of phosphorus compounds adsorbed onto the CeNP surfaces was identified to be orthophosphate (Table 3). Gerke found a similar phenomenon, in which phosphorous exhibited higher affinity to Fe complex with organic matter than to Fe in Fe-oxide [40]. Similarly, adsorption of DOC facilitated the phosphate adsorption onto the CeNP surfaces in the present experiment as well.  There was no pH dependence for the adsorption of inorganic phosphate; however, adsorption of phosphorus species derived from the EPS revealed similar pH dependency to that of DOC (Figure 4), despite that the majority of phosphorus compounds adsorbed onto the CeNP surfaces was identified to be orthophosphate (Table 3). Gerke found a similar phenomenon, in which phosphorous exhibited higher affinity to Fe complex with organic matter than to Fe in Fe-oxide [40]. Similarly, adsorption of DOC facilitated the phosphate adsorption onto the CeNP surfaces in the present experiment as well. dependence for the adsorption of inorganic phosphate; however, adsorption of phosphorus species derived from the EPS revealed similar pH dependency to that of DOC (Figure 4), despite that the majority of phosphorus compounds adsorbed onto the CeNP surfaces was identified to be orthophosphate (Table 3). Gerke found a similar phenomenon, in which phosphorous exhibited higher affinity to Fe complex with organic matter than to Fe in Fe-oxide [40]. Similarly, adsorption of DOC facilitated the phosphate adsorption onto the CeNP surfaces in the present experiment as well.  Table 3. Summary of phosphorus compounds analyzed by an inductively coupled plasma mass spectrometry system (ICP-MS) and ion chromatography (IC). Phosphorus concentration before or after 1 h or adsorption experiment at pH of 6 is tabulated. The adsorption experiments of phosphorus compounds onto 100 mg L −1 CeNPs were repeated four times to gain better statistics. The results from ICP-MS analysis represent total phosphorus concentration in EPS solution, while IC measures only the orthophosphate concentration. Data from both analytical methods display almost same values within the standard deviation. The amount of adsorption was calculated based on the difference between before and after adsorption experiment followed by normalization to the unit mass of CeNPs.

Concentration (µmol L −1 )
The Amount of Adsorption (µmol g −1 )  Figure 5 shows the results of the FTIR spectra of pristine CeNPs (i) and CeNPs adsorbing EPS (ii); and the difference between these two spectra (red line (iii)); which corresponds to the spectrum of only the adsorbed EPS components. The band assignments are summarized in Table 2. The FTIR spectrum explicitly revealed the significant difference in the relative intensity of the band between the adsorbed EPS (red line (iii)) and that of unreacted EPS (blue line (iv)); suggesting the preferential adsorption of particular EPS components onto the CeNPs; phosphoryl group and saccharides were preferentially adsorbed, while the relative intensity of the bands assigned to amide I, amide II and carboxyl group were suppressed after adsorption. In particular, the relative intensity of the amide II band was suppressed more than that of the amide I band. Because the amide I absorbance band is derived from the vibration of C=O in the amide I and carboxylate, the relative decrease of amide I band indicates that protein adsorption was not a dominant process. These results are consistent with a previous study by Omoike and others reporting that polysaccharide and phosphate groups selectively adsorb onto amorphous Al(OH) 3 surfaces [35], whereas less protein was adsorbed. It is already known that the adsorption of phosphate groups is configured by inner-sphere surface complexes between phosphoryl-containing compound such as phospholipids, and Fe-oxide minerals (goethite and hematite) [41], while sugar acids adsorb on the amorphous Al(OH) 3 surface by weaker electrostatic interactions [32]. One can expect that the adsorption onto CeNP surfaces may be controlled by inner-sphere coordination and weaker electrostatic interaction.  Figure 6 shows the FTIR spectra of orthophosphate in aqueous solution and orthophosphate adsorbed onto CeNPs. In aqueous solution, orthophosphate can dissociate to four species depending on the solution pH through the following reactions:

ICP-MS IC ICP-MS IC
The dissociation constants of the above reactions are Ka1 = 10 −2.2 , Ka2 = 10 −7.2 , and Ka3 = 10 −12.3 , respectively [42]. A diagram plotting the speciation of orthophosphate reveals that H2PO4 − is the predominant species at solution pH 6 ( Figure S1). For the FTIR spectrum of orthophosphate in aqueous solution, the bands at 1157 and 1078 cm −1 can be assigned to the P=O stretching mode of the H2PO4 − ion, and the one at 941 cm −1 to the P-O stretching mode of the H2PO4 − ion. The band at 993 cm −1 can be assigned to the P=O stretching mode of the HPO4 2− ion [36]. The FTIR spectrum of orthophosphate adsorbed onto CeNPs revealed the P=O stretching band of the adsorbed orthophosphate species at 1070-1250 cm −1 and P-OX stretching mode of adsorbed orthophosphate (X = H or Ce) at 845-1070 cm −1 . Broadness of the bands is attributed to two factors: one is the change in the P-OX vibration frequency. The electron density of the P-OCe bond is greater than that of the P-OH bond because of the smaller electronegativity of Ce than that of H. Thus, the frequency of the P-OCe vibration became greater than that of the P-OH mode. The broadness represents that both P-OH and P-OCe vibration are present at the CeNPs surface. The other factor is various adsorption forms such as monodentate or bidentate complexes. The frequency values of the P=O and P-OX vibration are altered by the adsorption form. Barja and others reported that the adsorption form is constrained by the adsorption density, where bridging bidentate complexes can transform to protonated monodentate complexes with increasing the adsorption density [43]. Similarly, the broadening of the bands should be partly ascribed to the multiple adsorption forms at the CeNPs surface in the present experiments. Thus, orthophosphate adsorbs onto CeNPs as an inner-sphere surface complex under both conditions with and without organic matter in the present experiment.  Figure 6 shows the FTIR spectra of orthophosphate in aqueous solution and orthophosphate adsorbed onto CeNPs. In aqueous solution, orthophosphate can dissociate to four species depending on the solution pH through the following reactions: The dissociation constants of the above reactions are K a1 = 10 −2.2 , K a2 = 10 −7.2 , and K a3 = 10 −12.3 , respectively [42]. A diagram plotting the speciation of orthophosphate reveals that H 2 PO 4 − is the predominant species at solution pH 6 ( Figure S1). For the FTIR spectrum of orthophosphate in aqueous solution, the bands at 1157 and 1078 cm −1 can be assigned to the P=O stretching mode of the H 2 PO 4 − ion, and the one at 941 cm −1 to the P-O stretching mode of the H 2 PO 4 − ion. The band at 993 cm −1 can be assigned to the P=O stretching mode of the HPO 4 2− ion [36]. The FTIR spectrum of orthophosphate adsorbed onto CeNPs revealed the P=O stretching band of the adsorbed orthophosphate species at 1070-1250 cm −1 and P-OX stretching mode of adsorbed orthophosphate (X = H or Ce) at 845-1070 cm −1 . Broadness of the bands is attributed to two factors: one is the change in the P-OX vibration frequency. The electron density of the P-OCe bond is greater than that of the P-OH bond because of the smaller electronegativity of Ce than that of H. Thus, the frequency of the P-OCe vibration became greater than that of the P-OH mode. The broadness represents that both P-OH and P-OCe vibration are present at the CeNPs surface. The other factor is various adsorption forms such as monodentate or bidentate complexes. The frequency values of the P=O and P-OX vibration are altered by the adsorption form. Barja and others reported that the adsorption form is constrained by the adsorption density, where bridging bidentate complexes can transform to protonated monodentate complexes with increasing the adsorption density [43]. Similarly, the broadening of the bands should be partly ascribed to the multiple adsorption forms at the CeNPs surface in the present experiments. Thus, orthophosphate adsorbs onto CeNPs as an inner-sphere surface complex under both conditions with and without organic matter in the present experiment.   (Figure 2), the P/C molar ratio of the EPS adsorbed onto CeNPs, which was calculated based on the integrated intensity of the P and C peaks, increased from 0.026 to 0.137 (Table 4), indicating that phosphorus compounds preferentially adsorbed onto CeNP surfaces. This is consistent with the FTIR results, revealing the preferential adsorption of phosphate. The peak position of P 2p did not shift after EPS adsorption ( Figures 2D and  7D), because orthophosphate is dominantly present in both cases. Table 5 summarizes the fraction of the functional groups among each element based on the integrated intensity of each corresponding peak after peak separation compared with the total intensity of peaks for each element. Notably, the fraction of C-(C,H) species among total C species increased compared with that of the pristine EPS, indicating that organic matter containing carbon chains such as lipids, amino acid side chains, or ring chains of saccharides preferentially adsorbed onto CeNP surfaces compared with proteins and carboxylates. As for the N 1s peak in the pristine EPS before the adsorption experiments, the fraction of amides (non-protonated) that are generally characterized as adenosine, nucleic acid, and amino acid is less than that of the protonated amine group ( Figure 2C, Table 5). In contrast, the N compounds adsorbed onto CeNPs were protonated amine groups, indicating the presence of only proteins among the N compounds. As a consequence, XPS analysis revealed that the lipids, saccharides, and phosphates preferentially adsorbed onto CeNP surfaces, while only a small amount of proteins adsorbed. These results are consistent with that of FTIR analysis.   (Figure 2), the P/C molar ratio of the EPS adsorbed onto CeNPs, which was calculated based on the integrated intensity of the P and C peaks, increased from 0.026 to 0.137 (Table 4), indicating that phosphorus compounds preferentially adsorbed onto CeNP surfaces. This is consistent with the FTIR results, revealing the preferential adsorption of phosphate. The peak position of P 2p did not shift after EPS adsorption ( Figures 2D and 7D), because orthophosphate is dominantly present in both cases. Table 5 summarizes the fraction of the functional groups among each element based on the integrated intensity of each corresponding peak after peak separation compared with the total intensity of peaks for each element. Notably, the fraction of C-(C,H) species among total C species increased compared with that of the pristine EPS, indicating that organic matter containing carbon chains such as lipids, amino acid side chains, or ring chains of saccharides preferentially adsorbed onto CeNP surfaces compared with proteins and carboxylates. As for the N 1s peak in the pristine EPS before the adsorption experiments, the fraction of amides (non-protonated) that are generally characterized as adenosine, nucleic acid, and amino acid is less than that of the protonated amine group ( Figure 2C, Table 5). In contrast, the N compounds adsorbed onto CeNPs were protonated amine groups, indicating the presence of only proteins among the N compounds. As a consequence, XPS analysis revealed that the lipids, saccharides, and phosphates preferentially adsorbed onto CeNP surfaces, while only a small amount of proteins adsorbed. These results are consistent with that of FTIR analysis. Table 4. Summary of the XPS analysis of major constituents in pristine EPS and EPS adsorbing onto CeNPs. The molar ratio was semi-quantitatively calculated by integrating the peak of each constituent and normalized by that of total C. amides (non-protonated) that are generally characterized as adenosine, nucleic acid, and amino acid is less than that of the protonated amine group ( Figure 2C, Table 5). In contrast, the N compounds adsorbed onto CeNPs were protonated amine groups, indicating the presence of only proteins among the N compounds. As a consequence, XPS analysis revealed that the lipids, saccharides, and phosphates preferentially adsorbed onto CeNP surfaces, while only a small amount of proteins adsorbed. These results are consistent with that of FTIR analysis.   Table 5. Summary of XPS analysis of the speciation of C, O, N, and P in pristine EPS and EPS adsorbed onto CeNPs reacted with EPS. After deconvolution, the intensity of each peak was integrated and normalized to the total integration of each element. *N.D. represents "not detected".

Effects of EPS on Zeta Potential of the CeNPs
The ζ potential of 10 or 100 mg L −1 CeNPs in 1 mM NaCl solution is plotted as a function of solution pH in Figure 8. The isoelectric point (iep) of the pristine CeNP surface was estimated to be 7.5 ( Figure 8A), which is in good agreement with the value previously reported; 6.6 and 8.0 [9,44]. In the presence of phosphate, the ζ potential decreased dramatically, and the iep decreased to ~2.0. Regardless of the CeNP concentration, the reduction of ζ potential remained unchanged. At pH > 1, H2PO4 − and/or HPO4 2−, can be present in the solution and the ζ potential decreased due to the  Table 5. Summary of XPS analysis of the speciation of C, O, N, and P in pristine EPS and EPS adsorbed onto CeNPs reacted with EPS. After deconvolution, the intensity of each peak was integrated and normalized to the total integration of each element. * N.D. represents "not detected".

Effects of EPS on Zeta Potential of the CeNPs
The ζ potential of 10 or 100 mg L −1 CeNPs in 1 mM NaCl solution is plotted as a function of solution pH in Figure 8. The isoelectric point (iep) of the pristine CeNP surface was estimated to be 7.5 ( Figure 8A), which is in good agreement with the value previously reported; 6.6 and 8.0 [9,44].
In the presence of phosphate, the ζ potential decreased dramatically, and the iep decreased to~2.0. Regardless of the CeNP concentration, the reduction of ζ potential remained unchanged. At pH > 1, H 2 PO 4 − and/or HPO 4 2− , can be present in the solution and the ζ potential decreased due to the adsorption of anionic species on CeNP surfaces ( Figure 8B). A similar mechanism was recognized in case of the phosphate adsorption onto goethite [36]. In contrast, the adsorption of EPS neutralized the ζ potential regardless of the CeNPs concentration ( Figure 8C). Slight difference in the pH dependence of ζ potential between the two different CeNP concentrations may be ascribed to the different coverage of adsorbed EPS compounds over the CeNP surfaces. In the experiment of EPS adsorption, phosphate also adsorbed onto CeNP surfaces as described in the previous section, and the amount of adsorbed phosphate is greater than that in the adsorption experiment of inorganic P (Figure 3). Despite the fact that a greater amount of P is adsorbed onto the CeNP surfaces, the ζ potential appeared to be neutralized and unaffected by the phosphate adsorption. It is known that low molecular weight organic matter such as citric acids can modify the surface charge by adsorption, which typically lower the ζ potential. Thus, the neutralizing effect of EPS on the ζ potentials cannot be fully explained by the adsorption of organic matter with low molecular weight [12,45]. In general, the ζ potential reflects the potential difference between the shear plane and the bulk phase, and the shear plane potential is affected by charge of the outermost surface. In case of the EPS adsorption, saccharides and proteins are likely present at the outermost surface because the molecular size is much larger than the molecular size of orthophosphate. Thus, the effects of phosphate adsorption on the ζ potential was suppressed by adsorption of these large molecules in the EPS solution.
Environments 2017, 4, 48 12 of 18 which typically lower the ζ potential. Thus, the neutralizing effect of EPS on the ζ potentials cannot be fully explained by the adsorption of organic matter with low molecular weight [12,45]. In general, the ζ potential reflects the potential difference between the shear plane and the bulk phase, and the shear plane potential is affected by charge of the outermost surface. In case of the EPS adsorption, saccharides and proteins are likely present at the outermost surface because the molecular size is much larger than the molecular size of orthophosphate. Thus, the effects of phosphate adsorption on the ζ potential was suppressed by adsorption of these large molecules in the EPS solution.

Effects of EPS on Aggregation and Sedimentation
In the present experiments, the optical absorbance was measured using UV-Vis to analyze the turbidity of solution in three different conditions: control solution, inorganic orthophosphate solution, and EPS solution with 100 mg L −1 CeNP concentration. Then, the absorbance was converted to the number of particle based on theoretical considerations, which are described in detail in the appendix. The aggregation rate constant, Kp′, was calculated based on Equation (2) as described in the materials and methods section, and the results were summarized in Table 6. The Kp' plot as a function of ionic strength revealed a drastic increase at the different ionic strengths in the three solutions: 0.01 mol L −1 for control, 0.14 mol L −1 for inorganic phosphate, and 0.25 mol L −1 for EPS solution, which corresponds to the critical aggregation concentration, CAC. Obviously, the CACs in the inorganic phosphate and EPS solutions are greater than that in the control solution at pH of 6, indicating that the adsorption of phosphate and saccharides increased the dispersibility. The enhanced dispersibility was also confirmed by the DLS analysis ( Figure S2). It is noted that the CAC in the EPS solution is slightly higher than that in the inorganic phosphate

Effects of EPS on Aggregation and Sedimentation
In the present experiments, the optical absorbance was measured using UV-Vis to analyze the turbidity of solution in three different conditions: control solution, inorganic orthophosphate solution, and EPS solution with 100 mg L −1 CeNP concentration. Then, the absorbance was converted to the number of particle based on theoretical considerations, which are described in detail in the Appendix A. The aggregation rate constant, K p , was calculated based on Equation (2) as described in the materials and methods section, and the results were summarized in Table 6.
The K p plot as a function of ionic strength revealed a drastic increase at the different ionic strengths in the three solutions: 0.01 mol L −1 for control, 0.14 mol L −1 for inorganic phosphate, and 0.25 mol L −1 for EPS solution, which corresponds to the critical aggregation concentration, CAC. Obviously, the CACs in the inorganic phosphate and EPS solutions are greater than that in the control solution at pH of 6, indicating that the adsorption of phosphate and saccharides increased the dispersibility. The enhanced dispersibility was also confirmed by the DLS analysis ( Figure S2). It is noted that the CAC in the EPS solution is slightly higher than that in the inorganic phosphate solution, which may be attributed to the presence of organic molecules such as saccharides and proteins in the EPS solution. In the inorganic phosphate solution, the surface charge is strongly negative (−40 mV) compared with that in the control solution (+23 mV) at pH 6 ( Figure 8). It is known that the electrostatic repulsive force is effective between the particles with negative charge, because the energetic barrier appears over ±20 mV according to the DLVO theory ( Figure S3). In case of the inorganic phosphate solution, the enhanced dispersibility was simply attributed to electrostatic repulsion. The aggregation rate constant dramatically increased above the CAC, because the thickness of the diffuse double layer collapses with increasing ionic strength (Equation (S5) in Supplementary Materials). On the other hand, in the EPS solution, the dispersibility of CeNPs was also enhanced despite the ζ potential being 0 mV at pH 6, indicating that the dispersibility was not enhanced only by electrostatic interaction and there is additional mechanism constraining the ζ potential in EPS. In particular, the adsorbed organic matter of EPS, predominantly saccharides and proteins, might play a role on enhancing the dispersibility in the EPS solution. Indeed, Safinajafabadi and others also reported that the colloidal stability was enhanced by the adsorption of saccharides including glucose, maltose, and dextrin [46]. Protein (bovine serum albumin) adsorption can also enhance the dispersibility of SiO 2 nanoparticles near the isoelectric point [47]. In general, the adsorption of organic matter forms a steric barrier over the particles, leading to the colloidal stabilization. The steric barrier can occur even with the molecular weight as low as~650 and becomes more significant with increasing molecular weight [48]. Hence, it is plausible that the adsorption of saccharides enhanced the colloidal stability by forming the steric barrier over CeNPs in the EPS solution in the present experiment. Although the difference in CAC between EPS solution and inorganic phosphate solution was small as revealed in Figure 9, the increment of the aggregation rate constant near CAC in the EPS solution is slightly more moderate than that in the inorganic phosphate solution, implying that the steric stabilization is relatively resistant to the effect of ionic strength compared with the electrostatic stabilization. solution, which may be attributed to the presence of organic molecules such as saccharides and proteins in the EPS solution. In the inorganic phosphate solution, the surface charge is strongly negative (−40 mV) compared with that in the control solution (+23 mV) at pH 6 ( Figure 8). It is known that the electrostatic repulsive force is effective between the particles with negative charge, because the energetic barrier appears over ±20 mV according to the DLVO theory ( Figure S3). In case of the inorganic phosphate solution, the enhanced dispersibility was simply attributed to electrostatic repulsion. The aggregation rate constant dramatically increased above the CAC, because the thickness of the diffuse double layer collapses with increasing ionic strength (Equation (S5) in Supplementary Materials). On the other hand, in the EPS solution, the dispersibility of CeNPs was also enhanced despite the ζ potential being ~0 mV at pH 6, indicating that the dispersibility was not enhanced only by electrostatic interaction and there is additional mechanism constraining the ζ potential in EPS. In particular, the adsorbed organic matter of EPS, predominantly saccharides and proteins, might play a role on enhancing the dispersibility in the EPS solution. Indeed, Safinajafabadi and others also reported that the colloidal stability was enhanced by the adsorption of saccharides including glucose, maltose, and dextrin [46]. Protein (bovine serum albumin) adsorption can also enhance the dispersibility of SiO2 nanoparticles near the isoelectric point [47]. In general, the adsorption of organic matter forms a steric barrier over the particles, leading to the colloidal stabilization. The steric barrier can occur even with the molecular weight as low as ~650 and becomes more significant with increasing molecular weight [48]. Hence, it is plausible that the adsorption of saccharides enhanced the colloidal stability by forming the steric barrier over CeNPs in the EPS solution in the present experiment. Although the difference in CAC between EPS solution and inorganic phosphate solution was small as revealed in Figure 9, the increment of the aggregation rate constant near CAC in the EPS solution is slightly more moderate than that in the inorganic phosphate solution, implying that the steric stabilization is relatively resistant to the effect of ionic strength compared with the electrostatic stabilization. Apparently natural sub-surface environment is a more complex system than the present experimental setting, because there are EPS derived from numerous kinds of microorganisms and a variety of nanoparticle phases along with many other molecular species in solution. Nevertheless, the present study at least demonstrates that EPS derived from microorganisms can adsorb to metal oxide nanoparticles with specific organic species preferentially adsorbed, modified the surface Apparently natural sub-surface environment is a more complex system than the present experimental setting, because there are EPS derived from numerous kinds of microorganisms and a variety of nanoparticle phases along with many other molecular species in solution. Nevertheless, the present study at least demonstrates that EPS derived from microorganisms can adsorb to metal oxide nanoparticles with specific organic species preferentially adsorbed, modified the surface properties, and changed their stability through the steric barrier derived from organic compounds as well as the electrostatic repulsive forces of the adsorbed ionic species in EPS. In the present experiments, the EPS was released after the incubation in YPD media that contains high P content and thus, the P concentration in the EPS is most likely higher than the one released from microorganisms in subsurface environments except for the microorganisms colonized adjacent to apatite [49]. In typical shallow groundwater with the ionic strength of the order of 10 −2 mol L −1 [14]. Hence, the adsorption of microbial EPS can potentially modify stability and transport of these colloids in groundwater.

Conclusions
Adsorption of EPS onto the surface of CeNPs and the effects on their aggregation were investigated to understand the role of microorganisms on the colloidal stability of low solubility cerium oxide nanoparticles as a surrogate of actinide oxide nanoparticles. The EPS derived from S. cerevisiae was composed of orthophosphate, organic phosphorous compounds, and various types of organic matter including polysaccharides and proteins. Among the EPS constituents, polysaccharides and orthophosphate preferentially adsorbed onto CeNPs. Aggregation of CeNPs was suppressed by the adsorption of EPS because of the electrostatic repulsive forces derived from the adsorbed orthophosphate and the steric barrier formed by the organic matter on the surface of CeNPs. The present study suggests that the specific EPS components adsorbed to metal oxide nanoparticles during the interaction between microorganisms and nanoparticles can cause colloidal stabilization depending on the pH conditions in the environment, which may facilitate colloid transport.