3-氨基苯硼酸为功能单体在壳聚糖上印迹牛血清白蛋白的研究

以壳聚糖为载体, 3-氨基苯硼酸为功能单体对牛血清白蛋白进行了分子印迹的研究, 并对吸附过程进行Langmuir等温吸附模型的数据处理. 结果表明, 印迹聚合物上形成了对于模板分子有较高的吸附容量和选择性的识别位点, Langmuir等温吸附平衡常数为49.5 mL/mg, 结合位点的最大表观结合量为16.3 mg/g, 证明了该印迹聚合物对于牛血红蛋白和溶菌酶这些非模板蛋白的吸附不具有选择性.     

牛血清白蛋白和溶菌酶为双模板蛋白质的表面印迹聚合物的制备及吸附性能

采用反应条件温和的原子转移自由基聚合法(ATRP),以N-异丙基丙烯酰胺(NIPAAm)和丙烯酰胺(AAm)为功能单体,以N-(3-二甲氨基丙基)甲基丙烯酰胺(DMAPMA)为辅助功能单体,制备了以牛血清白蛋白(BSA)和溶菌酶(Lyz)为双模板蛋白质的表面印迹聚合物(Bi-MIP)。对印迹过程中辅助功能单体的量进行了考察,结果表明,在单一蛋白质溶液和混合蛋白质溶液中,当DMAPMA为20 μL时,制备的Bi-MIP对模板蛋白质BSA和Lyz有较好的吸附容量与选择性。通过静态吸附实验考察了Bi-MIP的吸附性能,并结合Langmuir吸附模型得到聚合物对模板蛋白质BSA和Lyz的最大吸附容量分别为10.2 mg/g和19.2 mg/g。且该印迹聚合物在实际样品中对模板蛋白质也表现出较强的吸附能力和较高的选择性。该方法将为复杂生物样品中同时对双/多种目标蛋白质的识别提供一种新的途径。     

不同功能单体合成的谷胱甘肽分子印迹聚合物的研究

采用分子印迹技术, 以谷胱甘肽为模板分子, 以丙烯酰胺、甲基丙烯酸为功能单体制备分子印迹聚合物; 通过静态吸附试验, 探讨了合成分子印迹聚合物时模板分子与功能单体的物质的量比、上样液pH 值、吸附平衡时间、上样液浓度对聚合物吸附性能的影响; 实验结果表明: 以丙烯酰胺、甲基丙烯酸为功能单体制备谷胱甘肽分子印迹聚合物时,谷胱甘肽与丙烯酰胺、甲基丙烯酸的最适摩尔比分别为1:5 和1:4, 以及最适静态吸附条件为: 上样液pH 值分别为3.0 和5.0 左右; 上样液浓度分别为1.50～2.00 g/L 和1.00～1.50 g/L; 静态吸附平衡时间为18 和20 h 左右. 同时也探讨了分子印迹聚合物对谷胱甘肽结构类似物的吸附性能, 结果表明, 所合成的分子印迹聚合物对谷胱甘肽具有良好的选择性吸附能力. 同时也研究了分子印迹聚合物对酵母抽提物中谷胱甘肽的吸附性能, 以丙烯酰胺和甲基丙烯酸为功能单体制备的分子印迹聚合物对混合体系中谷胱甘肽的一次性提取率分别为41%和77%. 分子印迹聚合物均表现出了较好的吸附特性, 为分离提纯谷胱甘肽提供一种可选择的途径.     

葡萄球菌肠毒素B分子印迹聚合物的制备及其与蛋白质的结合性能

以葡萄球菌肠毒素B(SEB)蛋白为模板分子,以聚苯乙烯微球为基质,采用表面分子印迹法制备了SEB分子印迹聚合物.利用平衡吸附试验分析了SEB聚合物对目标蛋白的吸附能力及对类似底物的选择性;分析了该聚合物的吸附动力学,并利用扫描电镜观察了其形貌特征和颗粒尺寸.结果表明,经Scatchard模型分析求得的标题聚合物的最大表观结合量Qmax为3.23mg/g;所制备的SEB分子印迹聚合物呈微球形,粒径约为1²μm,对SEB蛋白具有较好的吸附性和特异选择性.     

己烯雌酚印迹共价有机骨架材料的制备及其性能探究

采用一步法制备己烯雌酚印迹共价骨架材料(MICOFs),将其作为固相萃取填料,结合高效液相色谱法,用于实际样品中己烯雌酚的分离与检测。以己烯雌酚为模板分子,三醛基间苯三酚(Tp)、对苯二胺(Pa-1)为功能单体,通过席夫碱反应合成印迹共价骨架材料。通过傅里叶变换红外光谱(FT-IR)、扫描电镜(SEM)、X-射线粉末衍射(XRD)对聚合物进行了表征,动力学和选择性吸附实验对MICOFs的吸附性能进行评价。结果表明:聚合物具有规则的形貌、良好的晶型,对己烯雌酚具有较高的吸附量(89.05 mg/g),能够快速达到吸附平衡(25 min),同时对模板分子具有良好的选择性。为己烯雌酚的分离提供一种新材料。     

磁性胰蛋白酶分子印迹聚合物的制备及性能评价

以壳聚糖修饰的四氧化三铁为载体,利用壳聚糖表面的氨基与戊二醛结合,丙烯酰胺为功能单体和交联剂,胰蛋白酶为模板蛋白,制备了磁性胰蛋白酶分子印迹聚合物。通过静态平衡结合法研究了磁性分子印迹聚合物的吸附能力、选择性。结果表明,与磁性分子非印迹聚合物相比,磁性分子印迹聚合物对模板蛋白具有高选择性和高特异性吸附,最大吸附量为162.2mg·g-1;Scatchard分析表明,存在两类不同的吸附结合位点,其离解常数分别为96.5μg·mL-1(高结合位点)和2.41mg.mL-1(低结合位点)。     

TNT分子印迹聚合物微球的合成与性能研究

以三硝基甲苯(TNT)为模板分子,EDMA为交联剂,采用沉淀聚合法制备了TNT分子印迹微球.讨论了溶剂用量、模板分子用量、功能单体种类等对分子印迹微球的形貌及吸附性能的影响;利用紫外吸收光谱和BET表征了印迹聚合物微球的结合位点相互作用与印迹孔穴结构;通过平衡吸附和选择性吸附实验,研究了印迹聚合物微球的吸附性能和选择性识别性能.结果表明,以丙烯酰胺为功能单体制备的分子印迹聚合物为规则的球形,内部含有分子印迹孔穴,微球的粒径为1～2μm.印迹聚合物微球可在30 min内达到吸附平衡,在1 mmol/L的TNT乙醇溶液中,印迹聚合物微球的平衡吸附量为32.5 mmol/kg,对TNT分离系数为25.19,具有较好的特异性吸附能力,并可选择性识别TNT分子.     

新型荧光分子印迹膜特异性识别和检测目标蛋白质

制备了一种新型荧光分子印迹膜(L-半胱氨酸修饰的量子点嵌入的分子印迹膜(QDs@MIM)),并将其作为荧光人工受体用于目标蛋白质(溶菌酶)的特异性识别和检测。QDs@MIM以溶菌酶为模板分子、丙烯酰胺为功能单体、L-半胱氨酸修饰的量子点为辅助单体、N,N′-亚甲基双丙烯酰胺为交联剂,在预硅烷化的玻璃板上制备而成。在最佳条件下,QDs@MIM对溶菌酶检测的线性范围为0.1~1.0μmol/L,吸附平衡时间为4 min,选择性因子为6.2。该方法操作简单、吸附平衡时间短、选择性高,具备作为生物传感器快速分析样品中目标蛋白质的潜力。     

头孢氨苄分子印迹聚合物制备及其性能研究

采用不同合成方法制备了头孢氨苄分子的印迹聚合物,考察了模板分子与功能单体之间的结合作用,测定了其吸附性能,用扫描电镜对其表面做了表征.结果表明:在甲醇体系中,用丙烯酰胺作功能单体,采用本体聚合法制备的印迹聚合物的吸附能力更好,对模板的单位结合量达到29.6mg/g,特异因子达3.29.     

双酚A分子印迹材料的制备及其识别特性研究

以双酚A为模板分子,α-甲基丙烯酸为功能单体,乙二醇二甲基丙烯酸酯为交联剂,偶氮二异丁腈为引发剂制备了双酚A印迹聚合物。采用动态和静态两种方法研究了该印迹材料对双酚A的结合性能与分子识别特性。印迹材料对模板分子双酚A具有良好的特异性识别作用,经过Scatchard模型分析,双酚A印迹聚合物上有两类不同性质的结合位点,两种结合位点的解离常数分别为1.36和44.78 m L/g,对双酚A的最大表观吸附量分别为24.56μmol/g和312.6μmol/g。将该聚合物应用于固相萃取中,以食品包装材料为样品的加标回收实验表明,此印迹材料可以对痕量双酚A进行富集分离测定,且可重复使用。     

复合分子印迹聚合物体系选择性富集蛋白质样品中的溶菌酶

考察了功能单体与模板蛋白的反应摩尔比、溶液pH值及离子强度对功能单体与模板蛋白之间相互作用的影响, 得出制备分子印迹聚合物的最佳条件. 在最佳条件下, 以溶菌酶(Lyz)为模板分子, 丙烯酰胺(AA)和N,N’-亚甲基双丙烯酰胺(BisAA)为聚合基质, 二氧化硅为固体制孔剂, 制备了复合分子印迹聚丙烯酰胺凝胶, 并用平衡吸附实验研究了其吸附性能和识别选择性. 研究结果表明, 该聚合物对模板蛋白有较高的亲和性、选择性和吸附容量,可以从蛋白质混合溶液中分离富集模板分子.     

Coating lysozyme molecularly imprinted thin films on the surface of microspheres in aqueous solutions

The polymerization of 3‐aminophenylboronic acid in an aqueous environment was used for the first time to modify polystyrene microspheres for protein (lysozyme) molecular imprinting. Polystyrene microspheres were prepared by styrene polymerization in an aqueous emulsion with poly(vinyl alcohol) as a surfactant. Poly(3‐aminophenylboronic acid) was then grafted onto the surface of the polystyrene microspheres through oxidation by ammonium persulfate in an aqueous solution in the presence or absence of lysozyme or hemoglobin. Rebinding experiments were conducted to establish the equilibrium time and to detect the specific binding capacity and selective recognition. The results indicated that the microspheres, imprinted by the template protein lysozyme or hemoglobin, possessed specific recognition sites on the shells and had a high specific binding capacity for template proteins. The imprinted particles did not need to be ground or sieved and could easily reach the adsorption equilibrium, thus avoiding some problems of the bulk polymer. All these results demonstrate that the particles have potential applications as substitutes for bulk polymers in biological macromolecular affinity studies. © 2006 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem 45: 1911–1919, 2007     

Recognition of Staphylococcus enterotoxin via molecularly imprinted beads

The synthesis of molecularly imprinted beads for the recognition of the protein Staphylococcus enterotoxin B (SEB) is described. Two kinds of organic silane (3-aminopropyltrimethoxysilane (APTMS) and octyltrimethoxysilane (OTMS)) were polymerized on the surface of polystyrene microspheres after the SEB template was covalently immobilized by forming imine bonds. The resulting imprinted beads were selective for SEB. The Langmuir adsorption models were applied to describe the equilibrium isotherms. The results showed that an equal class of adsorption was formed in the molecularly imprinted polymer (MIP) with the maximum adsorption capacity of 3.86 mg SEB/g imprinted beads. The MIP has much higher adsorption capacity for SEB than the nonimprinted polymer, and the MIP beads have a higher selectivity for the template molecule.     

尼卡地平分子聚合物的制备及识别性能研究

采用分子印迹技术合成了以尼卡地平为模板分子,甲基丙烯酸为功能单体的分子印迹聚合物(MIP).运用平衡结合实验研究了聚合物的吸附特性和选择识别能力.通过Scatchard方程分析,结合位点的离解常数Kd=1.03 mmol·L-1,最大表观结合常数Qmax=18.76 μmol·g-1.结果表明,分子印迹聚合物对尼卡地平呈现出较高的吸附性和选择识别性,对尼卡地平药物的分离富集和检测具有实际临床意义.     

双甘氨肽分子印迹聚合物微球的吸附性能研究

以双甘氨肽(Gly-Gly)为印迹分子,丙烯酰胺(AM)、二甲基丙烯酸乙二醇酯(EDMA)分别作为功能单体和交联剂,在低温条件下采用乳液聚合于水相中制备了双甘氨肽分子印迹聚合物微球(Gly-Gly-MIPMs)。通过静态、动态平衡吸附和薄层色谱(TLC)分离实验,研究了Gly-Gly-MIPMs的选择吸附性能,并进行了Scatchard模型分析。结果表明,Gly-Gly-MIPMs对Gly-Gly分子具有较好的特异性吸附,最大单位饱和吸附量0.428mmol/g,印迹因子2.19。     

Superparamagnetic lysozyme surface-imprinted polymer prepared by atom transfer radical polymerization and its application for protein separation

Molecular imprinting as a promising and facile separation technique has received much attention because of their high selectivity for target molecules. In this study, the superparamagnetic lysozyme surface-imprinted polymer was prepared by a novel fabricating protocol, the grafting of the imprinted polymer on magnetic particles in aqueous media was done by atom transfer radical polymerization (ATRP), and the properties of the imprinted polymer were characterized in detail. Its high selective adsorption and recognition to lysozyme demonstrated the separation ability of the magnetic imprinted material to template molecule, and it has been used for quick and direct separation of lysozyme from the mixture of standard proteins and real egg white samples under an external magnetic field. Furthermore, the elution of lysozyme from the imprinted material was achieved by PEG/sulphate aqueous two-phase system, which caused lysozyme not only desorption from the imprinted materials but also redistribution in the top and bottom phase of aqueous two-phase system. The aqueous two-phase system exhibited some of the extraction and enrichment effect to desorbed lysozyme. Our results showed that ATRP is a promising method for the protein molecularly imprinted polymer preparation.     

Poly(amino acid)-based thermoresponsive molecularly imprinted magnetic nanoparticles for specific recognition and release of lysozyme

In this study, poly(amino acid)-based thermoresponsive molecularly imprinted magnetic nanoparticles for recognition and release of lysozyme was prepared via surface imprinting method. For constructing the molecularly imprinted polymer (MIP) layer, amino acid-based thermoresponsive monomer (N-methacryloyl-l-alanine methyl ester, MA-L-Ala-OMe) was mainly selected for the functional monomer along with N,N′-methylenebis(acrylamide) as the crosslinker. The resultant magnetic MIP nanoparticles were characterized in detail. Meanwhile, the dynamic light scattering studies and swelling ratios measurements were carried out for demonstrating the thermoresponsive property of the imprinted nanoparticles. The prepared magnetic MIP nanoparticles showed good adsorption capacity and selective recognition properties to lysozyme. Moreover, the fast adsorption process could reach equilibrium within 15 min. Importantly, the capture and release of lysozyme could be easily realized simply by altering the temperature of aqueous solution. Furthermore, the prepared imprinted nanoparticles were applied to separate lysozyme from the real egg white samples. The results proved that the thermoresponsive MIPs based on MA-L-Ala-OMe have great potential for selectively enriching target proteins in real samples.