磁性凹凸棒土温敏性微凝胶的合成及其体外实验

通过乳液聚合法制备了叶酸(FA)接枝的磁性FA-Fe3O4/凹凸棒土-聚(N-异丙基丙烯酰胺-丙烯酰胺)(FA-Fe3O4/ATP-P(NIPAM-AAM))复合微凝胶(凹凸棒土=ATP,N-异丙基丙烯酰胺=NIPAM,丙烯酰胺=AAM),并通过X射线衍射(XRD)、振动样品磁强计(VSM)、热重(TG)、红外分析(I...     

Kinetics of thermo-induced micelle-to-vesicle transitions in a catanionic surfactant system investigated by stopped-flow temperature jump

The kinetics of thermo-induced micelle-to-vesicle transitions in a catanionic surfactant system consisting of sodium dodecyl sulfate (SDS) and dodecyltriethylammonium bromide (DEAB) were investigated by the stopped-flow temperature jump technique, which can achieve T-jumps within ～2-3 ms. SDS/DEAB aqueous mixtures ([SDS]/[DEAB] = 2/1, 10 mM) undergo microstructural transitions from cylindrical micelles to vesicles when heated above 33 °C. Upon T-jumps from 20 °C to final temperatures in the range of 25-31 °C, relaxation processes associated with negative amplitudes can be ascribed to the dilution-induced structural rearrangement of cylindrical micelles and to the dissolution of non-equilibrium mixed aggregates. In the final temperature range of 33-43 °C the obtained dynamic traces can be fitted by single exponential functions, revealing one relaxation time (τ) in the range of 82-440 s, which decreases with increasing temperature. This may be ascribed to the transformation of floppy bilayer structures into precursor vesicles followed by further growth into final equilibrium vesicles via the exchange and insertion/expulsion of surfactant monomers. In the final temperature range of 45-55 °C, vesicles are predominant. Here T-jump relaxations revealed a distinctly different kinetic behavior. All dynamic traces can only be fitted with double exponential functions, yielding two relaxation times (τ(1) and τ(2)), exhibiting a considerable decrease with increasing final temperatures. The fast process (τ(1)～ 5.2-28.5 s) should be assigned to the formation of non-equilibrium precursor vesicles, and the slow process (τ(2)～ 188-694 s) should be ascribed to their further growth into final equilibrium vesicles via the fusion/fission of precursor vesicles. In contrast, the reverse vesicle-to-micelle transition process induced by a negative T-jump from elevated temperatures to 20 °C occurs quite fast and almost completes within the stopped-flow dead time (～2-3 ms).     

Aloe vera–eluting collagen I microgels: physicochemical characterization and in vitro biological performance

Microgels absorb and retain high amounts of solvents, especially water. Because of their size, and association, the release kinetics of active molecules from microgels is easier to control than in hydrogels. Collagen I is one of the most extensively investigated biomaterials, although the key process parameters to produce microgels must be understood well before they can be used in veterinary and human medicine. Emulsification-gelation is widely used to obtain microgels because of its ease of handling and high yields. The concentration of the biomaterial and the homogenization method are among the critical parameters in this method. In this work, we produced cytocompatible collagen I microgels by emulsification-gelation and evaluated the effect of three different concentrations and homogenization methods on their physicochemical, mechanical, and biological properties. As proof of concept, microgels were loaded with an Aloe vera extract and the loading efficiency and the polyphenol release kinetics, as well as their properties assessed. When the same homogenization method (e.g. magnetic stirring) was used, the size of the microgels decreased with an increase of collagen I concentration, and the size distribution increased. In addition, the size and size distribution of microgels prepared with the same collagen I concentration were smaller when produced by high-energy homogenization methods (shear stress and ultrasound) than with a low-energy one (magnetic stirring). Collagen I concentration and the homogenization method also influenced the zeta-potential, the enzymatic degradation, and the encapsulation efficiency of the microgels. Overall, we show that the size of these microgels can be fine-tuned by the collagen I concentration and the homogenization method. Moreover, the integration of microgels of different sizes into the same carrier platform will pave the way for the combination of active compounds with different release kinetics.     

Swelling kinetics for a pH-induced latex-to-microgel transition

The kinetics of swelling of a series of six near-monodisperse, lightly cross-linked poly(2-vinylpyridine) latexes with mean diameters ranging from 380 to 1010 nm has been investigated by the pH jump method using a commercial stopped-flow instrument. These pH-responsive particles become substantially protonated at around pH 4.1, which leads to a rapid latex-to-microgel transition within a time scale of tens of milliseconds. The characteristic swelling time correlates linearly with the mean particle diameter, as predicted by the Tanaka equation. However, faster swelling is observed in the presence of added salt. This is contrary to the theory developed by Tanaka, which assumes that the relaxation of the polymer chains is the rate-limiting step. An alternative viewpoint, in which infusion of solvent determines the characteristic swelling time, satisfactorily explains the experimental observations and collapses most of the data, except for the largest microgels. This discrepancy is suggested to be due to the inaccurate sizing of these micrometer-sized swollen microgels by dynamic light scattering.     

Fluorine-containing pH-responsive core/shell microgel particles: preparation,characterization, and their applications in controlled drug release

A kind of novel fluorine-containing pH-responsive core/shell microgels poly(DMAEMA-co-HFMA)-g-PEG were prepared via surfactant-free emulsion polymerization using water as the solvent. The well-defined chemical structure of the copolymers was characterized by FTIR, ¹H-NMR, ¹⁹F-NMR, and elemental analysis. The microgel particles were studied by florescence probe technique, dynamic light scattering, and zeta potential measurement; the microgels displayed a significant pH-responsive behavior. Furthermore, the cytotoxicity assay indicated that the copolymer microgels had low toxicity, and 5-FU-loaded microgels offered a certain killing potency against cancer cells. In addition, the drug loading and in vitro drug release demonstrated that 5-FU was successfully incorporated into polymeric microgels, and the drug-loaded microgels showed a marked pH-dependent drug release behavior. This study suggests that the poly(DMAEMA-co-HFMA)-g-PEG microgels play an important role in the release mechanism stimulated by the change in the pH and have potential applications as a controlled drug release carrier.     

动态多孔海绵结构多层膜负载溶菌酶用于抗菌涂层的研究

以聚丙烯酸(PAA)和聚乙烯亚胺(PEI)为构筑单元,运用层层自组装技术制备了聚电解质多层膜.该多层膜具有独特的动态特点——经酸处理后膜内部形成海绵状通孔结构,该海绵结构在饱和水蒸气的处理下,多孔结构能够闭合,重新回到致密的膜结构.借助该种动态多层膜平台,能够简单有效地通过毛细作用力将溶菌酶负载并固定于多层膜中,为制备基于抗菌蛋白的抗菌涂层提供了新的方法.扫描电镜表征了多层膜动态变化过程,激光共聚焦显微镜表征了溶菌酶在膜内的分布情况,并测定了溶菌酶载入量及其释放动力学.进一步的抗菌测试表明该种抗菌涂层在溶菌酶和PEI的共同作用下可以有效地抑制金黄色葡萄球菌.将多层膜同时负载溶菌酶和乳铁蛋白,提升了涂层对大肠杆菌的杀菌效果.     

Preparation of Medium Cation Exchange Stationary Phase of Polymeric Matrix and Their Chromatographic Properties

Based on the monodisperse poly（glycidyl methacrylate-co-ethylenedimethacrylate） beads （PGMA/EDMA） with macropore as a medium, a new hydrophilic medium cation exchange （MCX） stationary phase for HPLC was synthesized by a new chemically modified method. The stationary phase was evaluated with the property of ion exchange, separability, reproducibility, hydrophilicity, effect of salt concentration, salt types, column loading and pH on the separation and retention of proteins in detail. It was found that it follows ion exchange chromatographic （IEC） retention mechanism. The measured bioactivity recovery for lysozyme was （96 ± 5）%. The dynamic protein loading capacity of the synthesized MCX packings was 21.8 mg/g. Five proteins were almost completely separated within 6.0 min at a flow rate of 4 mL/min using the synthesized MCX resin. The MCX resin was also used for the rapid separation and purification of lysozyme from egg white with only one step. The purity and specific bioactivity of the purified lysozyme was found more than 95% and 70345 U/mg, respectively.     

Synthesis and light scattering study of microgels with interpenetrating polymer networks

Monodispersed microgels composed of poly(acrylic acid) (PAAc) and poly(N-isopropylacrylamide) (PNIPAM) interpenetrating polymer networks (IPN) were synthesized by a two-step method, first preparing PNIPAM microgel and then polymerizing acrylic acid that interpenetrates into the PNIPAM network. The growth kinetics of the IPN particle formation was obtained by measuring the turbidity and particle hydrodynamic radius (Rh) as a function of reaction time. IPN and PNIPAM microgels were characterized and compared by dynamic and static light scattering techniques. The concentrated aqueous solutions of the PNIPAM-PAAc IPN microgels exhibit an inverse thermoreversible gelation. In contrast to polymer solutions of poly(NIPAM-co-AAc) that have the inverse thermoreversible gelation, our system can self-assemble into an ordered structure, displaying bright colors. Furthermore, IPN microgels undergo the reversible volume phase transitions in response to both pH and temperature changes associated with PAAc and PNIPAM networks, respectively.     

Ion concentration of external solution as a characteristic of micro- and nanogel ionic reservoirs

Ion-sensitive hydrogel is regarded as an ionic reservoir, i.e., a system capable of changing the external pH or ionic strength by accumulating or releasing ions. The concept of a hydrogel ionic reservoir was demonstrated for hydrogel particles of three different size ranges: macrogel (1000-6000 microm), microgel (approximately 20-200 microm), and nanogel (approximately 0.2 microm). Ion sensitivity of poly(N-isopropylacrylamide-co-1-vinylimidazole) (PNIPA-VI) microgels with imidazolyl (ionizable) groups was confirmed by the pH dependence of their volume, while nanogels were characterized by dynamic light scattering. On the contrary, the volume of poly(N-isopropylacrylamide) (PNIPA) microgels without ionizable groups was pH independent in the whole range of pH from 10 to 2. Four distinct regions of pH-behavior were observed for PNIPA-VI hydrogel micro- and nanoparticles using potentiometric titration of their suspensions. Time-resolved measurements of ion concentrations in the suspension of hydrogel particles revealed a substantial difference in kinetics of pH equilibration for (i) ion-sensitive hydrogels (PNIPA-VI) vs hydrogels without ionizable groups (PNIPA) and (ii) PNIPA-VI hydrogels of different sizes. On the basis of the experimental observations, a two-step mechanism affecting the kinetics of proton uptake into the hydrogel particles with ionizable groups was proposed: (1) fast binding of ions to the immediate surface of each particle and (2) a slower successive diffusion of bound sites into the next inner layer of polymer network. In accord with the mechanism proposed, a quasi-chemical kinetic model of pH relaxation to equilibrium was developed to fit the experimental data for the time course of proton uptake by macro-, micro-, and nanogels into two exponentials with the characteristic times of tau(1) and tau(2). We believe the same kinetic model will be pertinent to describe phenomenological and molecular mechanisms controlling proton transport in/out bacteria, cells, organelles, drug delivery vehicles, and other natural or artificial multifunctional ionic containers. The approach can be easily extended for the other ions (e.g., Na(+), K(+), and Ca(2+)).     

Kinetics of swelling of polyether-modified poly(acrylic acid) microgels with permanent and degradable cross-links

Spherical particles of 50-100 mum size composed of poly(acrylic acid) networks covalently bonded to Pluronic polyether copolymers were tested for swelling in aqueous media. The microgels were cross-linked either by permanent ethylene glycol dimethacrylate (EGDMA) cross-links alone or by EDGMA together with reversible disulfide or biodegradable azoaromatic cross-links. Optimum conditions for a rapid, diffusion-limited swelling of the pH- and temperature-sensitive microgels with nondegradable cross-links were found. The microgels cross-linked by disulfide groups and equilibrium-swollen in the buffer solution exhibited degradation-limited kinetics of swelling under physiological conditions, with a first-order reaction constant, k(1), linearly proportional to the concentration of reducing agents such as dithiotreitol and tris(2-carboxyethyl)phosphine (TCEP). A severalfold faster swelling in the presence of more powerful reducing agent, TCEP, was observed, indicating the chemical specificity of the microgel swelling. The reoxidation of the thiol groups into disulfide cross-links by sodium hypochlorite led to the restoration of the microgels' diameter measured prior to the reduction-reoxidation cycle, which confirms the shape memory of the microgels. Enzymatically degradable azoaromatic cross-links enabled slow microgel swelling due to degradation of the cross-links by azoreductases from the rat intestinal cecum. The low rate of swelling of the Pluronic-containing microgels can enable sustained drug release in colon-specific drug delivery.     

Colorimetric assay for lysozyme using Micrococcus luteus labeled with a blue dye, Remazol brilliant blue R, as a substrate.

Micrococcus luteus (M. lysodeikticus) labeled with Remazol brilliant blue R (blue ML) was prepared as a novel substrate for the colorimetric assay of lysozyme. The treatment of the labeled substrate with lysozyme resulted in the release of soluble blue products which can be easily measured spectrophotometrically at 600 nm. The blue color was most efficiently released at pH 7 and ionic strength of 0.2 on incubation with hen lysozyme at 40 degrees C. A new colorimetric method for the assay of lysozyme using this substrate was developed. The assay system gave a linear dose-response curve, and as little as 0.1 microgram of human lysozyme (1 microgram/ml, 100 microliters) can be detected. The present method is more convenient and reproducible than the conventional lysozyme assay with bacterial cells. Application of the system to the determination of lysozyme in human serum is described.     

Spreading of proteins and its effect on adsorption and desorption kinetics

The kinetics of adsorption of lysozyme and alpha-lactalbumin from aqueous solution on silica and hydrophobized silica has been studied. The initial rate of adsorption of lysozyme at the hydrophilic surface is comparable with the limiting flux. For lysozyme at the hydrophobic surface and alpha-lactalbumin on both surfaces, the rate of adsorption is lower than the limiting flux, but the adsorption proceeds cooperatively, as manifested by an increase in the adsorption rate after the first protein molecules are adsorbed. At the hydrophilic surface, adsorption saturation (reflected in a steady-state value of the adsorbed amount) of both proteins strongly depends on the rate of adsorption, but for the hydrophobic surface no such dependency is observed. It points to structural relaxation ("spreading") of the adsorbed protein molecules, which occurs at the hydrophobic surface faster than at the hydrophilic one. For lysozyme, desorption has been studied as well. It is found that the desorbable fraction decreases after longer residence time of the protein at the interface.     

Ligand Binding and Release Investigated by Contact-Guided Iterative Multiple Independent Molecular Dynamics Simulations

Binding and releasing ligands are critical for the biological functions of many proteins, so it is important to determine these highly dynamic processes. Although there are experimental techniques to determine the structure of a protein-ligand complex, it only provides a static picture of the system. With the rapid increase of computing power and improved algorithms, molecular dynamics (MD) simulations have diverse of superiority in probing the binding and release process. However, it remains a great challenge to overcome the time and length scales when the system becomes large. This work presents an enhanced sampling tool for ligand binding and release, which is based on iterative multiple independent MD simulations guided by contacts formed between the ligand and the protein. From the simulation results on adenylate kinase, we observe the process of ligand binding and release while the conventional MD simulations at the same time scale cannot.     

Synthesis of Monodisperse Poly（glycidylmethacrylate-co-ethylene dimethacrylate） Beads and Their Application in Separation of Biopolymers

Introduction Since 19541 the polymeric separation media has attracted much attention due to their chemical stability over the entire pH range. The rigid, highly cross-linked styrene copolymers were first used for chromatography by Moore.2 The macroporous copolymers currently available are not only chemically stable but also more resistant to mechanical forces prevailing in a column and therefore are comparable to the traditional packings based on silica gel. Most polymer separation media are …     

Protein refolding assisted by periodic mesoporous organosilicas

Herein we report a new strategy for protein refolding by taking advantage of the unique surface and pore characteristics of ethylene-bridged periodic mesoporous organosilica (PMO), which can effectively entrap unfolded proteins and assist refolding by controlled release into the refolding buffer. Hen egg white lysozyme was used as a model protein to demonstrate the new method of protein refolding. Through loading of denatured proteins inside uniform mesoporous channels tailored to accommodate individual protein, protein aggregation was minimized, and the folding rate was increased. Poly(ethyleneglycol) (PEG)-triggered continuous release of entrapped denatured lysozyme allowed high-yield refolding with high cumulative protein concentrations. The new method enhances the oxidative refolding of lysozyme (e.g., over 80% refolding yield at about 0.6 mg/mL).     

Effect of molecular architecture on micellization, drug loading and releasing of multi-armed poly(ethylene glycol)-b-poly(ε-caprolactone) star polymers

This study investigated the effect of molecular architecture of amphiphilic star polymers on micelle formation and drug loading and releasing. For this, multi-armed star block copolymers having poly(ethylene glycol) as a hydrophilic block and poly(ε-caprolactone) as a hydrophobic block were synthesized by using a divergent synthetic method consisting of a coupling reaction and a ring opening polymerization. The molecular weight and molecular weight distribution of the block copolymers were characterized by ¹H NMR and GPC measurements. Dynamic light scattering and fluorescence spectroscopic analysis were employed to observe micellization, drug loading, and drug release behaviors. We have figured out that the number of arms is a critical factor that changes critical micelle concentration as well as drug loading and releasing behaviors; increase in the number of arms not only led to lowering the critical micelle concentration and drug release rate but also increased the micelle size and drug loading efficiency.     

体积相转变温度可调的温敏性N-异丙基丙烯酰胺共聚物微凝胶的制备与性能研究

选用甲基丙烯酸异丙酯(iPMA)与N-异丙基丙烯酰胺(NIPAM)共聚,制备了一系列疏水改性、相转变温度可调的温敏性P(NIPAM-co-iPMA)微凝胶.利用透射电子显微技术(TEM)、浊度法、动态光散射(DLS)技术及示差扫描量热(DSC)技术对所得微凝胶的形态及去溶胀行为进行了表征.TEM与DLS结果表明,所制备的微凝胶具有规则的球型形态.浊度、DLS及DSC结果表明,疏水性单体iPMA的引入能有效调节共聚物微凝胶的相转变温度;在所考察的范围内,微凝胶的相转变温度随iPMA投料比的增加几乎呈线性降低.     

无皂种子分散聚合法制备单分散双重响应性微凝胶

以N-异丙基丙烯酰胺及2-乙烯基吡啶为主要单体, 采用无皂种子分散聚合法制备了单分散的、具有温度及pH双重响应性能的核-壳结构微凝胶, 并以扫描电镜及动态激光光散射等手段对微凝胶粒子的结构和性能进行了研究. 溶胀行为研究表明, 微凝胶粒子具有独立的互不干扰的温度及pH敏感性能, 其体积相变温度与纯聚N-异丙基丙烯酰胺(PNIPAM)凝胶基本一致, 说明局部分布的弱电离单体不会对PNIPAM凝胶的体积相变温度造成影响.     

钼氧卟啉(MovO(TPP)Cl)和二甲基亚砜(DMSO)反应动力学和反应机理研究

本文应用停-流快速反应动力学测定仪器研究氯钼氧卟啉(MoVO(TPP)Cl)同二甲亚砜(DMSO)的反应动力学. 实验结果表明, 反应至少含有四个基元步骤. 动力学研究得到驰豫时间τ与加入的初始二甲亚砜(DMSO)的浓度成线性关系, 本文提出了一种反应机理, 比较满意地解释了上述化学反应动力学实验结果。     

Polyurethane acrylate microgel synthesized by emulsion polymerization using unsaturated self-emulsified polymer

Polyurethane (PU) acrylate microgels were obtained by emulsion polymerization of self-emulsified PU acrylate terminated by 2-hydroxyethyl methacrylate without any extra emulsifier and crosslinker. Moreover, the PU acrylate was also used as stabilizer and crosslinker to synthesize poly(methyl methacrylate) (PMMA)–PU composite microgels via emulsion polymerization, which provided a new method to synthesize PU microgels and their composite microgels. The kinetics of microgel synthesis was studied by gel permeation chromatography. The dynamic rheological behaviors indicated that a crosslinked structure was formed. The frequency dependency of the loss tangent and complex viscosities showed strong relationships with the microgel structure. Those microgels with rigid PMMA core showed higher ability to slide than the soft PU acrylate microgel, which had influence on the changing of loss tangent with frequency. All the microgels swollen in tetrahydrofuran exhibited high viscosities and strong shear-thinning behaviors. As a sort of flexible microgel, the PU microgel was able to form a coherent film at room temperature, which was distinct from hard microgels.