Abstract
Synchrotron small-angle X-ray scattering (SAXS) was measured from aqueous solutions of polyion complexes (PICs), which were prepared by mixing oppositely charged diblock copolymers MAPTAC-b-PMPC and AMPS-b-PMPC. MAPTAC represents polycationic (3-(methacryloylamino)propyl)trimethylammonium chloride, AMPS represents polyanionic sodium 2-(acrylamido)-2-methylpropanesulfonate and PMPC represents hydrophilic poly-zwitterion (2-(methacryloyloxy)ethyl phosphorylcholine). The degrees of polymerization of MAPTAC and AMPS were selected to be the same for each complex, and the ratio (Rp) of the polymerization degree for the cationic to neutral chains was changed from 0.27 to 9.5. The aggregation number (Nagg) of PIC was determined with light scattering combined with field-flow fractionation (FFF). The inner structures of PIC were determined by analyzing SAXS with the core-corona model. When the MPC chain was much longer than the charged ones (Rp=0.27), a star-like spherical conformation was formed. With an increase of Rp, Nagg increased, while the spherical form was maintained up to Rp=1.0. When Rp=4.7 and 9.5, the PIC became a worm-like cylinder and vesicle, respectively. Based on the determined structural parameters and aggregation numbers, the index to describe how the tethered PMPC chains were crowded on the shell was determined. It was observed that the crowding parameter was much smaller than that of poly(ethylene glycol in spherical core-shell polymeric micelles.
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Introduction
Mixing two oppositely charged homo-polyelectrolytes results in polyion complexes (PICS), and their isoelectric mixing normally results in water-incompatible aggregates, which gradually coagulate to form larger aggregates and eventually precipitates.1, 2 Harada and Kataoka3 reported that when oppositely charged diblock copolymers H-A and H-C are mixed, where H, A and C represent non-ionic hydrophilic, anionic and cationic chains, the A and C blocks form a water-incompatible complex and the hydrophilic H chains cover to conceal the A/C complex from water. Thus, secondary coagulation is drastically reduced. In other words, the isoelectric H-A/H-C mixtures take a core-shell type micelle. In contrast to the case of classical PICs, the aqueous solutions dispersing these micelles are quite stable and their size shows an extremely narrow distribution. Presumably, their micellar structures are determined by a combination of the polyions and hydrophilic chain lengths and their chemical structures. This type of PIC micelles is denoted by PIC micelles in distinction from classical PICs prepared from homopolymers. It is interesting that the PIC micellar formation is quite similar to that of amphiphilic block copolymers.4
One of the major applications of PIC micelles is drug-delivery systems.5 In most cases, poly(ethylene glycol) (PEG) is used as the hydrophilic block with a similar purpose, with micelles made from amphiphilic block copolymers, that is, biocompatibility and enhancement of blood circulation.6 Thus, PEG has been used in many systems in biological applications and the coined term of ‘pegylation’ has become popular. Recently, several groups have emphasized a drawback of PEG: it can induce an immunological response for frequent dosing. This phenomena was first reported by Ishida et al.7, 8 for pegylated liposomes. According to these authors, pegylated liposome was rapidly cleared from the blood and accumulated in the liver when injected twice in the same rat or mouse at several-day intervals, called the ‘accelerated blood clearance phenomenon’. As an alternative, a photophilic polymer bearing a zwitterion as a side chain such as poly poly(2-(methacryloyloxy)ethylphosphorylcholine) (pMPC) has been synthesized using the reversible addition-fragmentation chain transfer radical polymerization method.9 According to Morisaku et al.,10 each MPC repeating unit is associated with ∼24 water molecules, whose number is much larger than that of PEG, which explains why pMPC is more biocompatible than PEG. In fact, biological systems use zwitterion-type phospholipids in which an anionic phosphate group is combined with a cationic choline. These phospholipids are the major component of all cell membranes, and these zwitterions form the biological surface of cells.
Recently, we synthesized a series of diblock copolymers consisting of an MPC block and either a cationic MAPTAC or anionic AMPS block using reversible addition-fragmentation chain transfer-controlled radical polymerization. Here, MAPTAC and AMPS represent poly(3-(methacryloylamino)propyl)trimethylammonium chloride and poly(2-(acrylamido)-2-methylpropanesulfonate), respectively (Figure 1). The mixing of aqueous solutions of oppositely charged diblock copolymers, pMPC-b-pMAPTAC and pMPC-b-pAMPS, led to the spontaneous formation of PIC micelles.11 The aim of this study is to characterize these PIC micelles using synchrotron small-angle X-ray scattering (SAXS) and multi-angle light scattering (MALS) to elucidate the details of the micellar architecture.
Experimental procedure
Materials and micelle preparation
Ten samples of pMPC-b-pMAPTAC or pMPC-b-pAMPS were newly synthesized using a pMPC-based chain-transfer agent for this study. The synthetic details are presented elsewhere.12 The molecular characters and the sample codes used in this paper are summarized in Table 1, where P, M and A represent pMPC, pMAPTAC and pAMPS, respectively, and the following number indicates the degree of polymerization for each block. The number-averaged molecular weight was determined using 1H NMR.12 PEG with a molecular weight of 400 g mol−1 was obtained from Wako Pure Chemical Industries, Ltd (Osaka, Japan) and denoted PEG400.
The obtained pMPC-b-pMAPTAC and pMPC-b-pAMPS were dissolved separately in distillated water containing 0.1 M NaCl (the salt concentration was the same unless otherwise noted). After being left overnight at room temperature, a pMPC-b-pMAPTA solution was added dropwise to a pMPC-b-pAMP solution with stirring. The mixing ratio defined by f=[MAPTAC]/([AMPS]+[MAPTAC])) was 0.5 at the isoelectrical composition. We prepared five PIC samples for the present work, and the sample codes and combination of pMPC-b-pMAPTAC and pMPC-b-pAMPS are presented in Table 2. Here we introduce the ratio of the polymerization degree of the cationic to neutral chains (Rp), as indicated in the second column of the table.
FFF coupled with MALS
An Eclipse 3+ separation system (Wyatt Technology Europe, Dernbach, Germany) was used as FFF, which was sequentially connected to a Dawn Heleos II multiangle static LS detector (Wyatt Technology) and an Optilab rEX DSP differential refractive index (RI) detector (Wyatt Technology) operating at a wavelength of 658 nm, in that order from the upper stream. A Wyatt channel (Eclipse 3 channel LC) was used, which had a tip-to-tip length of 17.4 cm and a nominal thickness of 250 μm and a membrane (Nadir cellulose membrane 10 kDa LC) was attached to the bottom of the channel. The specific refractive index increment (∂n/∂c) of the PIC micelles in 0.1 M NaCl aqueous solution was determined for each sample using a DRM-1021 differential refractometer (Otsuka Electronics, Osaka, Japan). The obtained value was used to determine the molar mass (MFFF) for each fraction from the LS intensity using the Berry plots. The weight-averaged and number-averaged molar masses (Mw and Mn) were calculated from RI and MFFF fractograms, assuming monodispersity for all fractions. The average aggregation number Nagg was determined using the relation of Nagg=Mw/(MpMPC-b-pMAPTAC+MpMPC-b-pANPS), where MpMPC-b-pMAPTAC and MpMPC-b-pANPS are the number-averaged molecular weight indicated by each subscript.
Synchrotron SAXS measurements
SAXS measurements were performed at BL40B2 of SPring-8, Japan.13 A 30 cm × 30 cm imaging plate (Rigaku R-AXIS VII, Tokyo, Japan) detector was placed at 0.75 or 1.65 m away from the sample. The wavelengths of the incident beam (λ) were 0.071 or 0.10 nm. The 0.75 and 1.65 m set-ups provided q ranges of 1.0–8.0 and 0.08–2.0 nm−1, respectively. The irradiation time was fixed at 300 s for all the measurements. A bespoke SAXS vacuum sample chamber14 was used and the X-ray transmittance of the samples was determined with an ion chamber located in front of the sample and a Si photodiode for the X-ray (Hamamatsu Photonics S8193, Shizuoka, Japan) after the sample. We verified that no irradiation damage occurred in preliminary experiments.
As one of the strongest X-ray sources in the world was being used, we were able to obtain the scattering profiles with a large S/N even at low concentrations of 1.0 mg ml−1 for C03, C05, C10 and C50, and 0.5 mg ml−1 for C100. In the previous study, we confirmed that the interparticle diffraction, that is, the structural factor, was negligibly small and, thus, we considered only form factors from scattering objects at these concentrations. The fitting model and its theoretical equations are presented in the Supplementary Information.
Results and Discussion
Determination of the aggregation number with FFF
Figure 2 presents the FFF elution fractograms recorded with LS at 90° (upper) and the concentration determined from refractive index (lower) for three NaCl concentrations ([NaCl]) of C03. The values of MFFF determined from MALS are plotted in the upper panel, indicating that MFFF of the 0.1, 0.5 and 1.0 M solutions ranged from 2 to 3 × 106, 2 to 5 × 105 and 3 to 8 × 104, respectively. Here, [NaCl] of the eluting solvent was adjusted to be the same as that of the sample solution. We injected the same amount of the sample; however, the 0.1 M solution exhibited a much larger peak area than the others. When we calculated the recovery ratio (defined by the ratio of the injected to eluted amounts of solute), the ratio for the 0.1 M solution was almost 100%, while those of the 0.5 and 1.0 M solutions were 47% and 58%, respectively, indicating that almost half of the solutes for the 0.5 and 1.0 M solutions did not come out and most likely went through the membrane filter attached to the bottom of the FFF channel during the focusing or measurement processes. These results can be interpreted as follows: at the higher [NaCl], the polyion parings in PIC were more disturbed by the ion exchange with sodium or chloride ions and, thus, the unimer/micelle equilibrium shifted to be more favorable for unimer formation. As the size of the unimer was small enough that the unimer was able to pass through the membrane filter, the recovery decreased with an increase of [NaCl]. As almost 100% recovery was attained at 0.1 M, hereinafter, we performed all the measurements at [NaCl]=0.1 M.
According to Yusa at et al.,12 dynamic LS revealed a similar ionic strength dependence as that in Figure 2 (see Supplementary Figure 1). The hydrodynamic radii thus obtained remained constant up to 0.1 M and gradually decreased, eventually reaching <3 nm at [NaCl]>0.9 M. These results indicated that in this high [NaCl], PIC micelles dissociated into unimers. These results indicated that PIC formed stable aggregates unless [NaCl] exceeded 0.15 M, which is another reason why we performed all the measurements at [NaCl]=0.1 M.
Although the data are not shown, FFF-MALS were performed for the other samples and the calculated Mw, Mw/Mn, and Nagg are listed in Table 2. For C03: Rp=0.27, Nagg was 2.3. For this complex, the charged chains were much shorter than the neutral one, and the aggregation number is considerably low. Therefore, we can presume that C03 assumes a star-like conformation15 rather than core-shell-16 or core-corona-17 type micelles. With an increase of Rp up to 1.0, Nagg increased. At Rp=1.0, Nagg became 30. In the range of Rp>1.0, different results were observed. At Rp=4.7, Ngg increased to 70 and at Rp=9.5, Nagg reached a magnitude of 104.
Small angle X-ray scattering
Figure 3 presents the SAXS profiles for all of the samples. For C03, C05 and C10, the exponent α defined by I(q)∼qα was ∼0 at low q, while α∼−2 at high q. For C03 and C05, the scattering intensities at q<0.1 nm−1 contained parasitic scattering due to the beam stop. Therefore, we did not use these regions for discussion. With an increase of Rp, that is, from C03 to C05, the intensity minimum near q=0.35 nm−1 became more obvious and slightly shifted toward lower q. For C10, the q dependence of I(q) at both high and low regions were α∼0 and α∼−2, respectively; however, there was a clear minimum at q=0.40 nm−1. The value of α∼−2 is characteristic for the Gaussian chains, which means that the second term in Supplementary Equation 1 dominates at high q for these three samples due to relatively small Nagg. As described above, this second term can be expressed by the Debye function of Supplementary Equation 3, and its asymptotic behaviors at low-q and high-q are Fch∼q0 and ∼q−2 (see the Supplementary Information), respectively. Therefore, one may suppose that the scattering profiles for these three samples, especially for C03, can be fitted by an equation only consisting of the Debye functions and an appropriate model corresponding to such an expression, for example, star polymers without solid core parts.18, 19 However, such a model cannot rationalize the presence of the intensity minimum at q=0.35 nm−1. To reproduce both the intensity minimum and the decay of I(q)∼q−2, we need a Debye function and an additional function that has a larger exponent of α, that is, α<−2 at high q. Thus, we selected Supplementary Equation 4 to fit the data. As Nagg is relatively small for C03, C05 and C10, we presumed that this core-corona model is appropriate in terms of physical standpoints. For analyzing the data, we rewrote Supplementary Equation 4 as follows:
Here, ρ1, ρ2 and ρsol are the electron density of the core, corona and solvent regions, respectively. For ρsol, we used 334 e nm−3 as calculated from the density and composition of the solvent. V1 and V2 are the volumes of the core and core-plus-corona region given by Vi=4/3πRi3, respectively. When we fit the data to obtain R1, R2 and Rg, we used the aggregation number given in Table 2 for Nagg and treated ρ1 and ρ2 as adjustable parameters. For the fitting model to make physical sense, we selected the same values of ρ1 and ρ2 for all three samples, and Rg,pMPC <1/2(R2−R1). The best-fitting curves are presented in Figure 3 as solid lines and are compared with the data, and the used-fitting parameters are listed in Table 3. The agreement between experiments and the model is sufficient to conclude that the core-corona micelle model well represents the spherical micellar structures of C03, C05 and C10.
With increasing Rp and thus the increasing Nagg, the core size increased from 4 to 9 nm. The fully stretched chain lengths of pAMPS were calculated to be 6.2, 12.4 and 24.9 nm, respectively, and these lengths are much longer than the core sizes. This result implies that the polyion pairs are randomly folded in the core, as expected. The values of RS−RC are ∼6 nm and the values of Rg,pMPC are 3 nm for all the samples. These unchanged corona sizes are consistent with the length of pMPC not changing for all the samples.
The scattering profile for C50 contained a clear secondary peak at q=0.4 nm−1, and there was no Guinier region observed in the present q range. These results indicated that the scattering object for C50 was much larger than C10, which is consistent with a large Nagg, and its local structure was well defined to yield the secondary peak. Yusa et al.12 performed a transmission electron microscopy examination for C50 and observed short worm-like cylinders (see Supplementary Figure 2). Cylindrical objects are consistent with the low-q behavior of SAXS, where the intensity appears to become I(q)∼q−2 at q<0.1 nm−1. We fit the data using Supplementary Equation 6 and the resultant parameters are summarized in Table 3.
Yusa et al.12 also performed transmission electron microscopy observations and observed that C100 took a mono-layered vesicle.20 As the SAXS intensity at low-q appears to asymptotically merge into the line of I(q)∼q−2, the vesicle model is consistent with the SAXS data. To fit the data using Supplementary Equation 5, we need to adjust seven parameters, although some of these parameters are not independent. Fitting with such multiple parameters may not lead to a unique combination of the parameters. We adopted a contrast-matching technique21 to solve this problem as follows.
Contrast matching
When we sequentially add a third component that has a relatively large electron density to the solvent and if we can assume that such an addition does not change the micellar structure, the scattering profile dramatically changes even from the same structures21 because such an addition changes the ρ-value for the layer adjacent to the solvent, for the monolayered vesicles described by Supplementary Equation 5, ρ2 and ρ4. As depicted in Figure 4 (right), we need to determine three geometric parameters: R1, the inner diameter of the vesicle; tcorona=R2−R1=R4−R3, the thickness of the corona layer; and tcore=R3−R2, the thickness of the core layer. Among these parameters, there are rules to follow in terms of the chemical structures. The electron densities of bulk PEG and water are known to be ρPEG=370 e nm−3 and ρwater=334 e nm−3, respectively, and thus, ρsol=wρwater+(1−w)ρPEG. Furthermore, we assumed that the added PEG chains did not enter the pMPC domain, and thus, ρCh=360 e nm−3 for all the experiment that have been determined for the other samples.
Figure 4 demonstrates how the scattering profile was changed by the addition of PEG400. On adding PEG to the C100 solution, the secondary peak near q=0.3 nm−1 become apparent at 5 and 10 wt%, and then further addition caused the peak to shift to lower angles and become less apparent at 30 wt%. The addition of PEG400 changed ρsol from 334 to 345 e nm−3 at 30 wt%. For each profile, we attempted to fit all the data using the same parameters, except for ρsol. The resulting theoretical curves are compared with the data in Figure 4, and the obtained parameters are listed in Table 4. The agreement between the values is good, indicating that the monolayered vesicle model is sufficient to describe C100.
The contrast-matching technique has been used commonly in neutron scattering, normally changing the composition of H2O/D2O.22 In this case, there is almost no risk that changing the solvent composition alters the conformation or structures of the solutes. To do the same in SAXS, we must add a third component to the solvent to change its electron density, which may cause a change in the structures of the solutes. As illustrated in Figure 4 (left), all of the scattering profiles were able to be fitted by the same structural parameters, although the scattering profiles were dramatically changed on adding PEG. This fact ensures that the added PEG did not cause major changes in the structures as well as proving that the obtained parameters were suitable.
Overcrowding nature of the MPC block
The manner in which the tethered chains are crowding on the flat surface can be described by the chain density (d) reduced by the sum of the cross-sectional area of the corona chains per surface area, where Rg is the radius of gyration of the isolated chain at its unperturbed state.23 When this index is <4, the tethered chains are not interacting with each other. When this index is from 4 to 10, the chains cross over with each other and the conformation of each chain deviates from a sphere. In the range of σ>10, the chains are more stretched to the direction normal to the surface. Svaneborg and Pedersen24 extended this concept to the shell of polymeric micelles, and the reduced chain density is given by
In this model, each corona chain is assumed to contact at RC+Rg,pMPC from the center of the core. From the same viewpoint, σ can be expanded to the surface of cylindrical and unilamellar vesicles:
where Rg,pMPC is the radius of gyration of the pMPC single chain; in our case Rg,pMPC=3 nm for Mw∼5000, and RC,in and RC,out are the inner and outer radii of the core of the vesicle, respectively.
We already know all of the parameters needed to determine the surface chain density d given by the three equations. The obtained d-values of pMPC are listed in Table 3; these values increased from 0.1 to 1.0 with an increase of Nagg. Compared with the polymeric micelles composed of PEG hydrophilic blocks, the values of d for C03, C05 and C10 were very small.25 It can be assumed from d=0.11 for C03 that the pMPC chain was not crowded to completely cover the core. In fact, the graft density of the pMPC on the core surface was ∼0.02 chains per nm2 (this value increased from 0.011 to 0.029 with an increase of Nagg), which was quite small, compared with nm−2. If the core is sufficiently hydrophobic, this less-crowded shell may cause secondary aggregation. The stable micelle formation for the present case can be attributed to the less hydrophobic nature of the core prepared from polyion paring and/or to the chemical nature of MPC, which can be associated with ∼24 water molecules.9
Conclusions
We performed FFF-MALS and SAXS for five PIC samples with different block lengths. Nagg increased from 2.3 to 104 with an increase of Rp from 0.27 to 9.5. The PIC structures were determined by analyzing the SAXS data using an appropriate model. When Rp=0.27, a star-like spherical conformation was observed. With an increase of Rp, the spherical form was maintained up to Rp=1.0, although the conformation transformed from the star to core-corona type. For Rp=4.7, the complex transformed into a worm-like cylinder, and when Rp=9.5 the complex became a vesicle. Based on the determined structural parameters and the aggregation numbers, the crowding parameter (d) was determined. For all of the samples, d was much smaller than that of PEG.
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Acknowledgements
This work was financially supported by the JST CREST program and all the SAXS measurements were performed at SPring-8 40B2 (2011B1735, 2012A1218, 2012B1252, 2012B1662, 2013A1207 and 2013A1594).
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Sakamoto, S., Sanada, Y., Sakashita, M. et al. Chain-length dependence of polyion complex architecture bearing phosphobetaine block explored using SAXS and FFF-MALS. Polym J 46, 617–622 (2014). https://doi.org/10.1038/pj.2014.25
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DOI: https://doi.org/10.1038/pj.2014.25