两种磁性复合微球的制备及其性能对比

为了得到蛋白吸附性能良好的免疫磁性载体,文章用反相微乳的方法合成了壳聚糖磁性复合微球(Chitosanmagneticcompositemicrospheres简称CMCM),与常用的单体聚合法制备的聚苯乙烯磁性复合微球(Polystyrenemagneticcompositemicrospheres,简称PMCM)从粒径和表观形貌、微球铁含量、磁响应性、表面官能基团等性质做了对比表征,结果表明,CMCM是一种比PMCM更理想的免疫磁性微球载体材料。     

亚微米级免疫磁球及其在细菌分离中的应用

以亚微米级的单分散磁性微球为基础,制备出了表面包被有沙门氏菌抗体的免疫磁球. 利用表面电位、荧光和ELISA等方法研究了抗体在磁性微球表面的吸附行为. 在沙门氏菌磁分离实验中,通过调节投料抗体的浓度,研究了免疫磁球表面抗体浓度和磁分离效率的相关性,与微米级商品化免疫磁球的对比中,亚微米级的免疫磁球表现出了更高的磁分离效率.     

Fe3O4-PMMA复合纳米微球的制备与表征

采用化学共沉淀法合成了超顺磁Fe3O4纳米粒子,并采用油酸和油酸钠对其表面进行修饰,制备了可稳定分散于水中的磁流体。以该磁流体为种子,通过一步乳液聚合制备了表面带有功能化羧基的Fe3O4-聚甲基丙烯酸甲酯复合纳米微球（Fe3O4-PMMA）。利用动态光散射、透射电镜观察、傅里叶红外光谱、热失重分析、振动样品磁强计测试等手段表征了复合微球的尺寸、形态、结构、组成和磁性能。结果表明,复合微球的平均直径约120nm,表面带有羧基功能基团,在室温下具有超顺磁性和较高的饱和磁化强度。     

新型亚微米亲水作用色谱的制备及其在加压毛细管电色谱中的应用

采用改良Stöber法合成580 nm亚微米单分散的二氧化硅微球，并以此为基质，通过"巯基-烯"点击化学反应将半胱氨酸成功键合到修饰有乙烯基团的二氧化硅微球表面，合成了一种新型亚微米亲水作用固定相（Cys-VTMS-SiO₂）。采用高压匀浆法制备了新型亚微米亲水色谱填充柱，通过不同乙腈比例、缓冲盐浓度和pH条件下对甲苯、丙烯酰胺和硫脲的分离分析揭示其亲水机理。依托加压毛细管电色谱平台，成功实现了对核苷、酚类、胺类及多肽等亲水性物质的快速有效分离，其有望应用于其他强极性和亲水性化合物的分离分析。     

P(St-GMA)/Fe3O4磁性聚合物微球的制备及表征

采用沉淀法制备了Fe3O4纳米粒子, 以苯乙烯(St)、甲基丙烯酸缩水甘油酯(GMA)为聚合单体, 使用分散聚合法制备了P(St-GMA)/Fe3O4磁性聚合物微球. 分析了Fe3O4粒子的形貌和结构. 研究了制备条件对磁性聚合物微球磁含量的影响. 采用FTIR, XRD, TG及TEM等手段对磁性聚合物微球的微观结构及形貌、磁含量等进行了分析表征. 研究结果表明, 制备的磁性聚合物微球粒径均一, 磁含量高达74%.     

高分子-无机复合纳米微球的制备和诊疗应用

目前,高分子-无机复合纳米微球因兼有高分子微球和无机纳米材料两者的性能优势而备受关注。其中,由可塑生物相容性的高分子与拥有特殊光、磁及电学性质的无机物组成的纳米微球,在疾病诊疗中应用前景广阔。功能高分子同多种无机粒子、活性分子可以复合形成多功能纳米微球,用于实现多模态成像诊断和可视化跟踪治疗。本文基于复合纳米微球的各种合成方法介绍,阐述了它们在靶向药物传输、生物成像、细胞分离、生物传感及热疗等诊疗领域的应用。同时,对纳米医疗领域前景和挑战进行了评述,为构建新型诊疗复合纳米微球提供有用信息。     

氧化铁磁性纳米粒子的制备、表面修饰及在分离和分析中的应用

氧化铁磁性纳米粒子通过表面化学修饰得到无机、有机或聚合物壳包覆在其表面。其中的壳结构既具有生物适应性,又具有可键合生物分子如细胞、蛋白质、酶、抗体和核酸的活性基团,而核具有磁性特性。本文总结了氧化铁磁性纳米粒子的制备方法,介绍了其表面化学修饰及在分离和分析应用的最新进展。     

刺激响应性聚合物微球的制备、性能及应用

作为典型的软物质材料,聚合物微球因其独特的微尺度、扩散性、渗透性及可修饰性而广泛应用于催化、药物传输、生物传感、微反应器、化学分离以及涂层材料等领域。为满足苛刻应用环境对微球的性能要求,相继出现了各类环境响应性聚合物微球。针对近年来刺激响应性微球的研究进展,本文综述了聚合物响应性微球的制备策略及形貌,以及对温度、pH、磁场、离子强度、光和CO₂敏感的响应性聚合物微球体系;并讨论了不同类型刺激响应微球的响应机理及应用,分析了其存在的不足,展望了其应用前景和发展方向。     

1,1-二苯基乙烯存在下无皂乳液聚合制备磁性复合微球

报道了一种制备磁性复合微球的方法——DPE法.在自由基控制剂1,1-二苯基乙烯(DPE)存在条件下,甲基丙烯酸甲酯(MMA)与丙烯酸(AA)发生无皂乳液聚合,制备能与Fe3O4粒子相螯合的活性短链共聚物,加入Fe3O4粒子把短链共聚物引到其表面,引发其它单体继续在Fe3O4粒子表面聚合,制备磁性复合微球.研究了AA、DPE、引发剂及Fe3O4粒子加入量等对制备磁性复合微球的影响.并在此基础上,对优化后工艺制备的磁性复合微球进行了TEM、TGA及磁响应性表征.结果表明,利用该新的方法制备出了磁含量为20%、比饱和磁化强度为32.2emu/g、平均粒径为265nm且表面不含任何杂质的磁性复合微球.     

磁性蛋白印迹复合微球的研究进展

磁性蛋白印迹复合微球因其特异性识别、高效分离目标蛋白的优点在蛋白分离和检测中具有重要的应用价值。由于蛋白分子自身的结构性质,磁性蛋白印迹材料在制备及进一步提升性能方面还面临着诸多的挑战。本文综述了磁性蛋白印迹复合微球的制备方法及提高其印迹效率的设计策略方面的研究进展,并介绍了磁性蛋白印迹复合微球在蛋白分离、免疫分析、生物传感等方面的应用研究新进展。     

多孔磁性硅胶微球的制备及其在基因组脱氧核糖核酸提取中的应用

采用模板法制备了多孔磁性硅胶微球,用于生物样品中基因组脱氧核糖核酸(DNA)的分离纯化。以球形和无定型硅胶为对照,考察了吸附液组成和洗脱时间等实验参数对小牛胸腺基因组DNA在磁性硅胶固相载体上的提取回收率的影响。实验结果表明:20%(W/V)聚乙二醇和2 mol/L氯化钠,洗脱10 m in,DNA的回收率可达80%;采用简单的细胞裂解体系和合适的吸附液组成,磁性微球应用于酿酒酵母中基因组DNA的提取,得到了平均长度约为5 kb、A260/A280大于1.77的高纯度DNA片段。     

Surface molecularly imprinted magnetic microspheres for the recognition of albumin

A new approach, combining metal coordination with the molecular imprinting technique, was developed to prepare affinity materials. Magnetic poly(glycidyl methacrylate) microspheres in monosize form were used for specific recognition toward the target protein. The magnetic poly(glycidyl methacrylate) microspheres were prepared by dispersion polymerization in the presence of magnetite nanopowder. Surface imprinted magnetic poly(glycidyl methacrylate) microspheres based on metal coordination were prepared and used for the selective recognition of human serum albumin. Iminodiacetic acid was used as the metal coordinating agent and human serum albumin was anchored by Cu²⁺ ions on the surface of magnetic poly(glycidyl methacrylate) microspheres by metal coordination. The magnetic poly(glycidyl methacrylate) microspheres were coated with a polymer formed by condensation of tetraethyl orthosilicate and 3‐aminopropyltrimethoxysilane. The human serum albumin imprinted magnetic poly(glycidyl methacrylate) microspheres were characterized by scanning electron microscopy, attenuated total reflectance Fourier transform infrared spectroscopy and particle size analysis. The maximum adsorption capacity of human serum albumin imprinted magnetic poly(glycidyl methacrylate) microspheres was 37.7 mg/g polymer at pH 6.0. The selectivity experiments of human serum albumin imprinted magnetic poly(glycidyl methacrylate) microspheres prepared with different concentrations in the presence of lysozyme, bovine serum albumin and cytochrome C were performed in order to determine the relative selectivity coefficients.     

Synthesis of polymer magnetic microspheres for immunomagnetometric assay

A method for the synthesis of polymer magnetic microspheres which allows the production of magnetic labels with a high magnetic susceptibility was developed. The microspheres contain surface functional groups for immobilization of bioligands and meet the requirements for immunomagnetometric assay. The obtained polymer magnetic microspheres were subject to comparative tests with commercial magnetic latexes.     

Fe3O4@Al2O3 magnetic core-shell microspheres for rapid and highly specific capture of phosphopeptides with mass spectrometry analysis

Selective detection of phosphopeptides from complex biological samples is a challenging and highly relevant task in many proteomics applications. In this study, a novel phosphopeptide enrichment approach based on the strong interaction of Fe(3)O(4)@Al(2)O(3) magnetic core-shell microspheres with phosphopeptides has been developed. With a well-defined core-shell structure, the Fe(3)O(4)@Al(2)O(3) magnetic core-shell microspheres not only have a shell of aluminum oxide, giving them a high-trapping capacity for the phosphopeptides, but also have magnetic property that enables easy isolation by positioning an external magnetic field. The prepared Fe(3)O(4)@Al(2)O(3) magnetic core-shell microspheres have been successfully applied to the enrichment of phosphopeptides from the tryptic digest of standard phosphoproteins beta-casein and ovalbumin. The excellent selectivity of this approach was demonstrated by analyzing phosphopeptides in the digest mixture of beta-casein and bovine serum albumin with molar ratio of 1:50 as well as tryptic digest product of casein and five protein mixtures. The results also proved a stronger selective ability of Fe(3)O(4)@Al(2)O(3) magnetic core-shell microspheres over Fe(3+)-immobilized magnetic silica microspheres, commercial Fe(3+)-IMAC (immobilized metal affinity chromatography) resin, and TiO(2) beads. Finally, the Al(2)O(3) coated Fe(3)O(4) microspheres were successfully utilized for enrichment of phosphopeptides from digestion products of rat liver extract. These results show that Fe(3)O(4)@Al(2)O(3) magnetic core-shell microspheres are very good materials for rapid and selective separation and enrichment of phosphopeptides.     

Preparation of magnetic microspheres with thiol-containing polymer brushes and immobilization of gold nanoparticles in the brush layer

Narrow-disperse magnetic microspheres were prepared by alkaline coprecipitation of Fe²⁺ and Fe³⁺ ions within poly(acrylic acid–divinylbenzene) microspheres that were prepared by distillation–precipitation copolymerization. Magnetic microspheres with polymer brushes that contain epoxy groups were prepared by graft copolymerization of glycidyl methacrylate and glycerol monomethacrylate via atom transfer radical polymerization (ATRP) from the magnetic microsphere surfaces. Subsequently, magnetic microspheres with thiol-containing polymer brushes were prepared by treating the epoxy group-containing magnetic microspheres with sodium hydrosulfide. Gold nanoparticles were immobilized in the brush layer of the thiol-containing magnetic microspheres through Au–S coordination. The catalytic activity of the gold nanoparticle-immobilized magnetic microspheres was investigated using the reduction of 4-nitrophenol to 4-aminophenol with sodium borohydride as a model reaction. The catalyst could be reused for over 10 cycles without noticeable loss of catalytic activity.     

Fabrication and functionalization of dendritic poly(amidoamine)-immobilized magnetic polymer composite microspheres

The synthesis of functionalized magnetic polymer microspheres was described by a process involving (1) preparation of the monodisperse magnetic seeds according to a two-step procedure including the preparation of bilayer-oleic acid-coated Fe3O4 nanoparticles followed by soap-free emulsion polymerization with methyl methacrylate (MMA) and divinyl benzene (a cross-linking agent, DVB); (2) seeded emulsion polymerization proceeding under the continuous addition of glycidyl methacrylate (GMA) monomers in the presence of the magnetic PMMA seeds; and (3) chemical modification of the PGMA shells with ethylenediamine (EDA) to yield amino groups. As such, the magnetic poly(MMA-DVB-GMA) microspheres were prepared possessing monodispersity, uniform magnetic properties, and abundant surface amino groups. Then, the dendritic poly(amidoamine) (PAMAM) shells were coated on the magnetic particles on the basis of the Michael addition of methyl acrylate and the amidation of the resulting ester with a large excess of EDA, which could achieve generational growth under such uniform stepwise reactions. For improving the luminescence properties of the composite particles, fluorescein isothiocyanate, which is a popular organic dye, was reacted with the terminal -NH2 groups from the dendritic PAMAM shells, resulting in the formation of multifunctional microspheres with excellent photoluminescence, superparamagnetic, and pH-sensitive properties. In this case, it can be expected that an extension of the functionalization of these microspheres is to immobilize other target molecules onto the PAMAM shells to introduce other desired functions for potential chemical and biological applications.     

磁性二氧化硅微球的表面修饰及其在植物基因组核酸纯化中的应用

在利用自主研发的专利技术制备球形磁性硅胶微球的基础上,对磁性硅胶微球进行表面改性,使其表面分别键合硅羟基、环氧基、邻二醇基和羧基等官能团,并对表面官能团进行了定量研究。以小牛胸腺基因组脱氧核糖核酸(DNA)为模型化合物,研究了核酸在不同表面官能团的磁性硅胶上的吸附和脱附行为,发现表面具有硅醇基的磁球对DNA的回收率最高。将改性后磁性微球应用于玉米DNA的提取,得到了平均长度大于8kb的高纯度基因组DNA。与传统的有机溶剂抽提法相比,基于磁性微球的核酸固相萃取法具有快速简便、省时省力、易于自动化的特点,适合于大规模植物基因组DNA的样品制备。     

Poly(styrene-acrylic acid) magnetic polymer microspheres

Magnetic polymer microspheres have been considered as a kind of new biopolymer materials with great advantages in bioseparation engineering and biomedicine engineering because they have not only polymer functional groups but also magnetic characteristics. Styrene-acrylic acid copolymer (p(S-AA)) magnetic microspheres were synthesized by dispersion polymerization with Fe₃O₄ as core and p(S-AA) as shell. The microspheres were characterized by SEM, size analysis, molecular weight and solid content measurement. All of them indicate that the microspheres are small in size, narrow in distribution, stable in chemistry and rich in functional groups on their surface. __________ Translated from Journal of Beijing Union University (Natural Science) 2008, 21(3): 82–84     

磁性微球的制备及在细胞分离中的应用

总结评述了近年来磁性微球制备的研究工作,阐述了磁性微球用于细胞分离的基本原理和方法,指出了当前需要解决的问题。     

Boronic acid functionalized Fe3O4 magnetic microspheres for the specific enrichment of glycoproteins

Glycoproteins are useful biomarkers and therapeutic targets for a number of diseases, including infections and cancer. However, identification and isolation of low‐abundant glycoproteins remains a significant challenge that limits their application. Thus, methods of specific and selective glycoprotein enrichment are required. In this study, novel phenylboronic acid functionalized magnetic microspheres were successfully synthesized. Fe₃O₄ microspheres were synthesized by using a hydrothermal method and were coated with tetraethyl orthosilicate using an ultrasonic method to form a core‐shell structure. Compared to the conventional mechanical stirring for 12 h, the ultrasonic method saved about 7 h in processing time, and the home‐made magnetic microspheres had better dispersibility and homogeneity. Subsequently, the magnetic microspheres were modified by addition of an amino group and a carboxyl group, in sequence. Finally, 3‐aminophenylboronic acid, as the functional monomer, was linked to the magnetic microspheres for capturing glycoprotein/glycopeptides. The results of this study indicate that phenylboronic acid functionalized magnetic microspheres show excellent adsorption performance toward glycoprotein/glycopeptides. The maximum absorbing capacity of the microspheres for fetuin was 108 mg/g, and the enrichment efficiency reached 89.7%, indicating their potential to separate and enrich glycoproteins from the complex biological samples.