Abstract
We present an investigation of horseradish peroxidase (HRP)/H2O2-mediated crosslinking in an inverse miniemulsion for the successful preparation of a stable colloidal nanogel from a poly(amino acid)-based polymer precursor. The precursor was obtained by the aminolysis of polysuccinimide with aminoethan-2-ol and tyramine, resulting in a poly(α,β-N-(2-hydroxyethyl)-D,L-aspartamide-co-N-(2-(4-hydroxyphenyl)ethyl)-D,L-aspartamide) polymer (PHEA-Tyr). Various concentrations of the PHEA-Tyr in aqueous solution with HRP were emulsified in the presence of cyclohexane and SPAN 80. The addition of a hydrogen peroxide solution induced crosslinking between the polymer chains via the phenol groups (Tyr) and targeted nanogel formation. The hydrodynamic radii (R h 0), mean size documented by hydrodynamic radius (R h ), and morphology of the nanoparticles were investigated by dynamic light scattering (DLS) measurements, nanoparticle tracking analysis (NTA), and cryogenic transmission electron microscopy (cryo-TEM). It was found out that nanoparticle radius, morphology, and architecture of the nanogel could be regulated by the initial concentration of the precursor.
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Introduction
Nanogels are widely studied nanomaterials since they integrate distinctive and unique properties of hydrogels and nanoparticles [1]. These nanoparticles with three-dimensional networks have been of great interest due to their favorable characteristics, including proper size, swelling in aqueous media, porosity, softness, stimuli-responsive behavior, hydrophilicity, degradability, and biocompatibility [2]. These new types of nanoparticles have also gained significant attention for their large surface area for bioconjugation and their internal network for cell encapsulation and incorporation of inorganic nanoparticles or biomolecules, such as DNA, peptides, and proteins. Thus, they are attractive for applications in drug delivery, tissue engineering, bionanotechnology, bioimaging, sensing, antifouling, etc. [3, 4].
Nanogel synthesis can be based on natural materials, for example, chitosan, dextran, and proteins, or synthetic monomers and polymers or on their combination, including acrylic acid, N-isopropylacrylamide, 2-(dimethylamino) ethyl methacrylate, methoxydiethylene glycol methacrylate, aminoethyl methacrylamide hydrochloride, oligo(ethylene glycol) monomethyl ether methacrylate, and poly(ethylene glycol) dimethacrylate [5,6,7,8,9,10,11,12]. As is evident from the term “nanogel,” the polymer chains of the nanoparticles are physically or chemically crosslinked to form the interior network between macromolecular chains [13]. Physical crosslinking comprises relatively weak non-covalent interactions between polymer chains, including hydrogen bonds, hydrophobic interactions, or ionic interactions, whereas chemically crosslinked polymer chains are joined covalently by various approaches. Examples include an addition of crosslinking monomer during polymerization, click chemistry, and enzyme-mediated crosslinking [1].
Neamtu et al. simply classified the preparation of nanogels into two groups: top-down and bottom-up approaches [7]. The process in which nanoparticles are synthetized from larger materials by physical, chemical, or mechanical degradation is called the top-down approach. Bottom-up nanogels are prepared from monomers or polymer precursors. The latter method usually employs free or controlled radical polymerization adopting inverse miniemulsion, inverse microemulsion, precipitation, reversible addition fragmentation chain transfer, or atom transfer radical polymerization, as well as their combinations [14,15,16,17,18,19,20]. For example, conventional inverse miniemulsion polymerization is a suitable technique for the preparation of ~100–500-nm hydrophilic latexes in diameter from 2-hydroxyethyl methacrylate, acrylamide, and N-isopropylacrylamide. Briefly, the liquid monomer phase is dispersed into small droplets in a continuous organic phase using a high-energy input, such as a sonifier, in the presence of a hydrophobic emulsifier and osmotic agent to retard the diffusional degradation of the miniemulsion. The monomer droplets serve as the main polymerization locus [21, 22].
Due to fact that hydrogels based on amino acids or synthetic poly(amino acids) have suitable properties for biomedical applications and tissue engineering, they are also very promising for the preparation of hydrophilic crosslinked nanostructures [23, 24]. For example, Park et al. synthetized a poly(ethylene glycol)-grafted poly(succinimide) nanogel to analyze cellular uptake [25]. Furthermore, the triclosan-loaded, L-lysine-based nanogel prepared by a top-down approach showed antibacterial activity against some pathogens [26]. Additionally, linear water-soluble polymers based on synthetic poly(amino acids), such as poly(α,β-N-(2-hydroxyethyl)-D,L-aspartamide) (PHEA), meet all the requirements for preparation of hydrogels in terms of hydrophilicity, non-cytotoxicity, and biocompatibility and are generally used as model systems for their non-degradability [27,28,29,30]. In case that poly(amino acid)-based polymers bear functional groups on their chains, such as aromatic phenols, amines, or phenolic acids, they can easily form crosslinked structures via horseradish peroxidase (HRP)-catalyzed reaction [31]. The HRP catalyzes a decomposition of hydrogen peroxide (H2O2) in presence of reducing substrate (e.g., phenolic substrates) which is converted to radical product. One equivalent of H2O2 induces the formation of two aromatic radicals which are readily coupled by covalent bond to form crosslinked structure under mild conditions.
Herein, we report a combination of inverse miniemulsion and HRP/H2O2-mediated crosslinking for the preparation of a hydrophilic and colloidal stable nanogel. The poly(α,β-N-(2-hydroxyethyl)-D,L-aspartamide-co-N-(2-(4-hydroxyphenyl)ethyl)-D,L-aspartamide) (PHEA-Tyr) was initially obtained by aminolysis of polysuccinimide (PSI) and was used as a polymer precursor for the bottom-up synthesis at different concentrations. By taking advantage of PHEA-Tyr behavior in water solutions, the combination of inverse miniemulsion and HRP/H2O2-mediated crosslinking resulted in water-stable colloidal nanogels. The particles were then investigated by dynamic light scattering (DLS), nanoparticle tracking analysis (NTA), and cryogenic transmission electron microscopy (cryo-TEM); the obtained nanogels had different radii and morphology varying from globule-composed to low-crosslinked, hydrogel-related structures depending on PHEA-Tyr concentration.
Materials and methods
Materials
N,N-dimethylformamide (DMF) and cyclohexane (CHX) were purchased from Lach-Ner (Czech Republic). Aminoethan-2-ol (Fluka) was purified by vacuum distillation. Tyramine, hydrogen peroxide solution 30% (w/w) in water, peroxidase from horseradish (type VI), and sorbitane monooleate (Span 80) were purchased from Sigma-Aldrich and were used without further purification. PSI with M w ~30,000 was obtained from F. Rypáček (Institute of Macromolecular Chemistry, Academy of Sciences of the Czech Republic, Heyrovsky Sq. 2, 162 06 Prague 6, Czech Republic). It was prepared from D,L-aspartic acid (Loba Chemie, Wien, analytical grade) by thermal polycondensation in the presence of phosphoric acid according to Neri et al. [32].
Synthesis of the polymeric gel precursor PHEA-Tyr
The PHEA-Tyr gel precursor was prepared from PSI through stepwise aminolysis using tyramine and aminoethan-2-ol in DMF (Scheme 1). Briefly, PSI (10 g, 0.103 mol) was dissolved in DMF (250 mL), then the tyramine was added (2.82 g, 0.0206 mol), and reaction mixture was stirred at room temperature for 24 h. Subsequently, the residual PSI groups were aminolyzed with aminoethan-2-ol (8 g, 0.1310 mol) to obtain a water-soluble polymer PHEA-Tyr. The reaction was carried out for 5 days at room temperature. The resulting polymer was purified by dialysis (molecular weight cutoff < 3000 Da) successively against a 100 mM sodium chloride solution for 2 days, a mixture of distilled water and ethanol (3:1) for 1 day, and distilled water for 2 day. The purified solution was lyophilized to obtain PHEA-Tyr with a yield of 53%.
Gel permeation chromatography (GPC) was performed on a system (Knauer) equipped with a diode array detection (DAD; wavelengths 205, 254, and 280 nm), an evaporative light scattering detection (ELSD) (Altech 3300, Grace, USA), and Phenomenex PolySep™-SEC GFC-P Linear Column 300 × 7.8 mm using a mixture of 0.05 M ammonia acetate buffer, pH 6.5/acetonitrile 80:20 as the eluent at the flow rate of 0.3 mL/min. The system was calibrated with polyethylene oxide standards.
The degree of tyramine substitution of PHEA-Tyr was determined using UV-Vis spectrometry (Specord 250 Plus, Analytik Jena AG, Germany).
The presence of covalently bonded tyramine units was confirmed by the GPC measurements using the DAD detector and by 1H-NMR (Bruker 300 MHz, D2O, δ, ppm): 6.99 (d, 2H), 6.65 (d, 2H), 4.64 (m, 1H, NH-CH-CO), 3.41 (s, 2H, NHCH 2 CH2OH), 3.13 (s, 2H, NgHCH2CH 2 OH), 2.57 (s, 2H, NHCHCH 2 CO), 2.50 (s, 2H, CHCH 2 CO).
Preparation of PHEA-Tyr nanogel in inverse miniemulsion
Preparation of PHEA-Tyr nanogels in inverse emulsion was carried out in a 30-mL glass reaction vessel equipped with an anchor-type stirrer. In a typical experiment, PHEA-Tyr (0.18 g) and NaCl (0.263 g) were dissolved in water (4.32 g). Simultaneously, Span 80 (0.655 mL) was dissolved in cyclohexane (20.4 g). Then, both solutions were mixed together and horseradish peroxidase (0.1 mg) was added into to mixture. The mixture was cooled at 0 °C and sonicated using a W-385 sonicator (Heat System Ultrasonics; Farmingdale, NY) for 150 s at amplitude 50%. The dispersion was transferred into the glass reaction vessel under stirring (500 rpm) and hydrogen peroxide (11.25 μL) was added, and the reaction was allowed to proceed at 25 °C for 18 h. At the end of the reaction, PHEA-Tyr nanogel was removed by centrifugation (9000 rpm) and washed with methanol, ethanol, and water. Then, the nanogels were purified by dialysis (molecular weight cutoff < 3000 Da) against ethanol/distilled water mixture (1:1) for 48 h and against distilled water for 24 h. Methanol, ethanol, and water were used to remove unreacted components such as cyclohexane, SPAN 80, and unreacted PHEA-Tyr. The nanogels were finally freeze-dried from water.
DLS
Dispersions of nanoparticles were investigated by dynamic light scattering (DLS) using ALV-6010 correlator equipped with an ALV/CGS-8F goniometer, a 22-mW He-Ne laser (wavelength λ = 632.8 nm), and pair of avalanche photodiodes operated in a pseudo-cross-correlation mode. The measured intensity correlation function g2(t) was analyzed using the algorithm REPES [33] performing the inverse Laplace transformation according to
where t is the delay time of the correlation function and β is an instrumental parameter and yielding distribution A(τ) of relaxation times τ. The relaxation time τ is related to the diffusion coefficient D and relaxation (decay) rate Γ by the relation:
where q is the scattering vector defined as
where n is the refractive index of the solvent and θ is the scattering angle. The hydrodynamic radius R h of the particles can be calculated from the diffusion coefficient using the Stokes-Einstein equation:
where T is the absolute temperature, η is the viscosity of the solvent, and k B is the Boltzmann constant. The hydrodynamic radius R h 0 of nanogels was obtained by subsequent double extrapolation of measured data to q = 0 and concentration c = 0 to compare obtained results with another method. In case of the initial droplets of polymer precursor in 1 M NaCl and the emulsion of polymer precursor in inversion emulsion, the DLS measurements were made at a 90° angle due to time instability of the analyzed samples and values of hydrodynamic radius R h was obtained.
The samples for DLS measurement (5 mL; 1 mg/mL) were dispersed in Milli-Q water in glass vials by UP200S ultrasonic processor (Hielscher Ultrasonics GmbH, Teltow, Germany) for 5 min at intensity 50%, and 1 mL of each sample was used for the measurement.
NTA
NTA measurements were performed using a NanoSight NS300 (Malvern, Worcestershire, UK) containing a sample chamber of about 1 mL, 532-nm laser and camera sCMOS. The sample was pumped into the chamber with a sterile 1-mL syringe. Each sample was analyzed for 60 s and five times with manual adjustment, and all measurements were performed at 25 °C. The NTA 2.3 Dev Build 3.2.16 analytical software was used for data capturing and data evaluation.
The samples for NTA (5 mL; 1 mg/mL) were dispersed in Milli-Q water in glass vials by UP200S ultrasonic processor (Hielscher Ultrasonics GmbH, Teltow, Germany) for 5 min at intensity 50%. Then, each sample was diluted by Milli-Q water at concentration 10 μg/mL and about 0.8 mL of the sample was pumped into the chamber with a sterile 1-mL syringe.
cryo-TEM
Cryo-TEM observations were performed on a Tecnai G2 Spirit Twin 120 kV (FEI, Czech Republic), equipped with cryo-attachment (Gatan, cryo-specimen holder) using a bright-field (BF) imaging mode at accelerating voltage 120 kV.
Cryo-TEM allows direct investigation of samples in the vitrified, frozen-hydrated state.
The dispersion of each sample was applied to an electron microscopy grid covered with holey carbon-supporting film (300 MESH, Cu) after hydrophilization by glow discharge (Expanded Plasma Cleaner, Harrick Plasma, USA). The excess of the solution was removed by blotting (Whatman no. 1 filter paper) for ~1 s, and the grid was immediately plunged into liquid ethane held at − 182 °C. The frozen sample was immediately transferred into the microscope and observed at − 173 °C under the conditions described above.
The samples for cryo-TEM measurement (5 mL; 4 mg/mL) were dispersed in Milli-Q water in glass vials by UP200S ultrasonic processor (Hielscher Ultrasonics GmbH, Teltow, Germany) for 5 min at intensity 50%, and 3 μL of each sample was used for the measurement.
Results and discussions
First, PSI (M w ~30,000) was converted into linear PHEA-Tyr by an aminolysis reaction (Scheme 1). The content of Tyr on the PHEA-Tyr polymer was determined to be 18.5 mol% by UV spectroscopy at 275 nm. The PHEA-Tyr polymer was analyzed with GPC, and it was found that the synthesized polymer had a dispersity of Ð = 1.71 and that the number average (M n ) and weight average (M w ) molecular weights were 7900 and 13,500, respectively.
The PHEA-Tyr was then used for the preparation of crosslinked nanoparticles with the assumption that linear PHEA exists in a random coil conformation in aqueous solution [34], which could contribute to the desired formation of spherical particles. Before the nanoparticle synthesis, the PHEA-Tyr solution in 1 M NaCl (1 mg/mL) was examined by DLS because the reaction environment for the preparation of the nanogels contains NaCl in this concentration. The results showed a bimodal intensity-based distribution, indicating the presence of clusters with R h ~200 nm (ca. 20%) and small particles with R h ~6 nm (ca. 80%). This result indicates that the majority of PHEA-Tyr polymer is present in molecularly dissolved form, which is visualized in Fig. 1 by the conversion of the measured intensity- to volume-based distribution. This observation is well correlated with the results of Coviello et al., who found that PHEA with a molecular weight M w = 52,000 formed random coils with a radius of gyration of ~6 nm in aqueous solution [35].
The main objective of this work was to prepare crosslinked nanometer-sized hydrophilic particles from biocompatible PHEA-Tyr by enzymatic crosslinking in an inverse miniemulsion. The effect of various concentration of aqueous solution of PHEA-Tyr (4 to 12 wt%) in aqueous solution was investigated on the final particle size and morphology. As the first, the stable inverse miniemulsion consisting of PHEA-Tyr, water, HRP, CHX, SPAN 80, and NaCl, which acted as a lipophobe preventing the droplets from coalescence, known as Ostwald ripening, was obtained after the sonication procedure because it represented a crucial point of overall procedure [21]. The initial inverse miniemulsions were analyzed by DLS to obtain R h values of the formed droplets which grew from 202 ± 15 to 357 ± 90 nm with increasing PHEA-Tyr concentration. Secondly, the formed inverse miniemulsion was transferred into a reactor, and while being vigorously stirred, the H2O2 was added to ensure an immediate formation of the nanogel. In this system, each droplet composed of the PHEA-Tyr random coils represented a small reactor. The introduction of H2O2 molecules into the droplet initiated the enzymatic covalent crosslinking between the globular coils and the formation of the intrinsic network within the nanoparticle. We assumed that H2O2 mainly acted as the crosslinking agent after penetration into the droplets when appeared on the oil-water interface and also during collision of the droplets. The resulting colloidally stable nanogels (NG1–5) were then purified, freeze-dried, and sonicated in water for further examination by DLS, NTA, and cryo-TEM.
The DLS analysis with double extrapolation of final NG1–5 nanogels demonstrated that the R h 0 increased from 271 ± 5 to 449 ± 23 nm with increasing concentration of PHEA-Tyr in the miniemulsion (Table 1) as was observed with the sizes of initial emulsions. This observation suggested that at higher concentrations of PHEA-Tyr, the inverse miniemulsion with larger polymer precursor-based droplets were formed resulting in the larger final nanogel. The increase of polymer precursor concentration also led to formation on nanogels with broad particle size distribution.
Although all DLS measurements of the original emulsions were performed at one angle and the measurement of nanogels with double extrapolation, it was possible to trace that the sizes of the nanogels were close to R h of the corresponding inverse miniemulsion droplets. This could support our assumption that the sizes of final nanogels could be regulated by initial concentration polymer precursor and droplet size of starting inverse miniemulsion which was in agreement with theory about conventional miniemulsion polymerization when the average particle size is comparable to the original droplet size [36]. Due to the fact that the DLS measurements of the original emulsions were performed only at 90° angle, these values were not mentioned in Table 1.
The NG1–5 nanogels were further analyzed by NTA, because this analysis enables more accurate sizing and high resolution of particle size distribution compared to DLS and visualization of nanoparticles in dispersion [37]. The measurements confirmed that the R h of the NG1–NG5 increased with increasing polymer precursor concentration (Table 1). However, the sizes collected by NTA were approximately two times lower than data obtained by DLS. The differences could be explained by the fact that DLS method is not sensitive in resolving of sample peak with broad size distribution, and the results can be affected by presence of larger particles which scatter the light more that smaller particles [37]. This effect may complicate the accurate sizing. Table 1 also includes the standard deviation (SD) values of the five independent measurements for each sample calculated by the NTA software. The SDs were rather high, indicating that sizes of NG1–5 were spread out over a wider range of values.
Contrary to the size of nanogels, the reaction conversion decreased with increasing PHEA-Tyr concentration in the dispersed phase (Table 1). This decline was explained by the fact that H2O2 was maintained at a constant concentration and thus always initiated a crosslinking of the same amount of the polymer precursor regardless of the increase of PHEA-Tyr concentration in the reaction feed. Therefore, more unreacted and non-crosslinked polymer precursor was removed during washing step in the case of HRP/H2O2-mediated crosslinking in inverse miniemulsion of PHEA-Tyr with the higher concentration.
Figure 2a–e demonstrates the NTA video frames of visualized and analyzed NG1–NG5 in aqueous dispersion. It was obvious that HRP/H2O2-mediated crosslinking of PHEA-Tyr polymer precursor in an inverse miniemulsion resulted in the nanoparticles which were individual and had broad size distribution. But our poly(amino acid)-based nanogels were insoluble in water and colloidally stable in aqueous dispersion because they did not form aggregates.
The cryo-TEM analysis was carried out to deeply investigate the architecture, morphology, and size of the purified nanoparticles. However, it is important to emphasize that the measurement was complicated due to the low contrast and softness of the nanogels. Therefore, we analyzed NG1 and NG5 nanogels which represented the most different samples in our set of experiments.
Figure 3a–f shows the cryo-TEM images of NG1 and NG5 nanogels, which confirmed that the combination of HRP/H2O2-mediated crosslinking in the inverse miniemulsion led to the successful formation of spherical nanoparticles from the PHEA-Tyr polymer precursor. The cryo-TEM images of NG1 nanoparticles (Fig. 3a, b) documented that prepared nanogel were spherical in shape and had compact structure, seemingly composed of the small ~5-nm globules corresponding to the PHEA-Tyr coils. This similarly composed architecture was also observed with elastin-like recombinamer nanogels [38]. Moreover, our finding was in agreement with the DLS measurement of solution of PHEA-Tyr in 1 M NaCl which contained the polymer coils with R h ~6 nm. This also suggested our primary hypothesis about particle formation from the PHEA polymer precursor.
In contrast to NG1, the NG5 nanogel (Fig. 3c–f) was softer, contained large pores with the approximate radius from 20 to 70 nm, and its morphology resembled low HRP/H2O2-crosslinked poly(amino acid)-based hydrogels [39]. Our cryo-TEM observations proved that final architecture of the nanogels was strongly dependent on the initial concentration of PHE-Tyr polymer precursor. In case of 4 wt% of PHEA-Tyr, the miniemulsion contained smaller droplets and the addition of H2O2 induced the crosslinking of more polymer chains in each droplet resulting in less optically transparent NG1 nanogel with more rigid structure and less unreacted polymer precursor was removed during washing step. Also, Koul et al. observed that the interpenetrating polymer network nanogels composed of poly(acrylic acid) and gelatin with high cross-linked density prepared by inverse miniemulsion technique showed higher contrast during transmission electron microscopy [40]. In spite of that, less polymer chains were transformed into the crosslinked nanostructure when initial concentration of PHEA-Tyr was 12 wt%, and the obtained NG5 was larger with highly porous and soft structure, more optically transparent. Moreover, these hydrogel nanoparticles seemed to be lower crosslinked in comparison with NG1 and structurally similar to low crosslinked hydrogels. Wu et al. described a preparation of ~200-nm polyglycerol nanogels in diameter with spherical shape and porous structure by HRP/H2O2-catalyzed crosslinking in inverse miniemulsion [41]. However, the authors stated that their porous nanogel was water-soluble, what seemed to be inconsistent with their conclusions. Despite the fact that our cryo-TEM images did not show a sufficient number of particles to analyze their average radius, the average size of the depicted NG5 particles was evaluated and found to be in range from 80 to 290 nm and average radius was 175 ± 58 nm.
Conclusions
In summary, we found that the two approaches, HRP/H2O2-mediated crosslinking and inverse miniemulsion technique, can be applied for the preparation of spherical and colloidal stable poly(amino acid)-based nanogels. By taking advantage of PHEA-Tyr polymer precursor behavior in aqueous solution and knowledge of conventional inverse miniemulsion polymerization, the nanogels with various sizes and morphologies were prepared depending on initial concentration of the polymer precursor. The average R h 0 values were determined by DLS and mean R h by NTA. Both measurements showed that the size of the nanogels increased with the increasing concentration of the polymer precursor. The prepared nanogels were visualized by NTA confirming their colloidal stability in water and nanoparticle character. The architecture and morphology of the final nanogels varying from compact to soft and highly porous structures also depended on the initial concentration of the polymer precursor which was documented by cryo-TEM images. While these nanogels were prepared from a non-degradable precursor, this study provides an important background for subsequent synthesis of a poly(α,L-amino acid)-based biodegradable nanogel and proved the usefulness of the method to synthesize covalently crosslinked, colloidal stable nanoparticles from other polymer precursor with reactive functional groups.
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Petr, Š., Jana, D., Peter, Č. et al. Poly(amino acid)-based nanogel by horseradish peroxidase catalyzed crosslinking in an inverse miniemulsion. Colloid Polym Sci 296, 995–1003 (2018). https://doi.org/10.1007/s00396-018-4318-7
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DOI: https://doi.org/10.1007/s00396-018-4318-7