热敏性磁性高分子微球同蛋白质的相互作用

热敏性磁性微球被用于人血清白蛋白（ｈｕｍａｎ ｓｅｒｕｍ ａｌｂｕｍｉｎ ,ＨＳＡ） 的吸附／ 解吸研究,考察了温度、ｐＨ 值、蛋白质浓度以及保温时间等因素对蛋白质吸附／ 解吸的影响,结果显示微球对蛋白质的吸附／ 解吸具有明显的温度依赖性;ｐＨ 值增大使蛋白质的吸附量减小;延长保温时间和增大蛋白质的初始浓度均有利于增加蛋白质的吸附量．     

表面图案化的CdS-P(AM-co-10%MAA)复合微球对BSA的吸附性能研究

以微米级的P(AM-co-10%MAA)共聚物为模板,在反相悬浮体系中,通过外源沉积的方法合成了硫化镉复合微球CdS-P(AM-co-10%MAA)。以牛血清白蛋白为主要目标蛋白,研究微球对蛋白质的吸附性能。结果表明,牛血清白蛋白在CdS复合微球上的最大吸附量为35.84mg/g,其吸附模式符合Langmuir吸附定律。在20～50℃范围内,随着温度的升高,复合微球对蛋白质的吸附量增大。在磷酸缓冲溶液体系中,CdS-P(AM-co-10%MAA)复合微球对蛋白质的吸附量在蛋白质等电点时达到最大;此外,复合微球不仅对BSA具有一定的吸附能力,对其它蛋白质同样具有一定的吸附能力,说明该微球具有开发为分离材料的潜力。     

双硫腙改性的聚(二甲基丙烯酸乙二醇酯-甲基丙烯酸羟乙酯)微球的制备及其对铜离子的吸附研究

用悬浮聚合法由二甲基丙烯酸乙二醇酯(EGDMA)和甲基丙烯酸羟乙酯(HEMA)共聚制备得到聚(二甲基丙烯酸乙二醇酯-甲基丙烯酸羟乙酯)(PHEMA)微球,考察了NaOH浓度、反应时间等对用双硫腙进行PHEMA改性反应的影响以及铜离子水溶液浓度(5～500mg/L)、pH(2.0～6.5)、吸附时间等对改性后的微球对铜离子吸附性能影响的因素.改性的PHEMA微球对铜离子的最大吸附量为65.6mg铜离子/g双硫腙;而且,吸附有铜离子的改性PHEMA微球用0.1mol/L的硝酸的解吸率可达到90%以上,经过3次吸附-解吸循环后,解吸率仍基本不变,这表明双硫腙改性的PHEMA微球可以多次反复使用,具有良好的应用前景.     

单宁微球对Cr（Ⅵ）的吸附性能

利用单宁微球吸附Cr（Ⅵ）,探讨了温度、pH值、Cr（Ⅵ）初始质量浓度等因素对单宁微球吸附性能的影响,并分析了其吸附等温曲线。结果表明,单宁微球对Cr（Ⅵ）具有很好的吸附效果,吸附量可达到45.5 mg/g。单宁微球对Cr（Ⅵ）的去除率随吸附时间的延长而增大,5 h后基本达到平衡。温度对单宁微球吸附Cr（Ⅵ）的影响比较...     

多孔苯乙烯-二乙烯基苯共聚物微球的磺化及其对牛血清蛋白的吸附

在不同反应温度下对多孔苯乙烯-二乙烯基苯共聚物微球进行磺化亲水性修饰,采用扫描电镜与氮气吸附法,研究多孔微球的孔结构。结果显示,磺化反应修饰后,微球的孔容与比表面积变小,且随着磺化温度升高,比表面积与孔容递减。交换容量则随着磺化温度升高而递增。用牛血清蛋白作为模型蛋白质,研究了亲水性修饰后的多孔苯乙烯-二乙烯基苯共聚物微球对蛋白质大分子吸附性能的影响。实验结果表明,牛血清蛋白在磺化微球上的吸附主要由孔容与比表面积决定,孔容与比表面积越大,蛋白质吸附量也越大。吸附速率表现为疏水作用快于静电作用。吸附动力学研究表明,Kannan-Sundaram模型可较好地描述牛血清蛋白的吸附动力学行为。     

功能化PVA-g-PSt微球对牛血清蛋白的吸附研究

由大分子单体法制得了聚醋酸乙烯酯接枝聚苯乙烯(PVAc-g-PSt)微球,使该微球在碱性条件下醇解形成了聚乙烯醇接枝聚苯乙烯(PVA-g-PSt)微球.经X射线光电子能谱对PVA-g-PSt微球表层组成的表征,发现微球具有以PVA为壳、PSt为核的核壳结构.进而利用汽巴蓝F3GA(CB)与PVA-g-PSt微球进行亲核反应,制得了CB功能化的PVA-g-PSt微球,由元素分析定量出了固定在微球表面的CB含量.用透射电子显微镜对微球的粒径与形态进行了表征,发现微球表面在CB功能化后变得相对粗糙,粒径大小基本保持不变,但形态更加规整.比较了3种不同微球对蛋白质的吸附,考察了吸附动力学和影响吸附的因素,发现起始牛血清蛋白(BSA)浓度、pH值、离子强度对微球吸附BSA有明显的影响,并利用Zeta电位探讨了微球与蛋白质间的相互作用机理.最后用硫氰酸钠(NaSCN)进行解吸,计算解吸率最高可达到95.7%,该CB功能化微球可以重复利用,吸附率仅减少5.3%.     

Cu(Ⅱ)印迹丙烯腈-co-苯乙烯微球的制备与对Cu(Ⅱ)的选择性吸附

以Cu(Ⅱ)为模板离子、丙烯腈为功能单体,苯乙烯(St)为骨架单体,偶氮二异丁腈为引发剂,二乙烯苯为交联剂制备了铜离子印迹丙烯腈-co-苯乙烯微球(Cu-I-AN-co-St);用UV、FTIR、SEM和FAAS表征了聚合物和分析了Cu-I-AN-co-St对Cu(Ⅱ)的选择性吸附;结果表明,在室温下溶液pH为5～6,吸附时间为60 min时吸附达到平衡,最佳吸附条件下,饱和吸附容量可达到49.1 mg/g;以1 mol/L HCl溶液作为解吸剂其解吸率可达98%;与相应非印迹微球(NI-AN-co-St)相比,Cu(Ⅱ)I-AN-co-St对Cu(II)的吸附量增大并具有选择性;与电荷相同及离子半径相近的Zn(Ⅱ)、Ni(Ⅱ)、Cd(Ⅱ)共存时,其相对选择性系数分别为28.2,24.8,44.4。     

改性木质素磺酸钠水凝胶对镉离子的吸附研究

研究了改性木质素磺酸钠水凝胶对水溶液中镉离子的吸附性能,考察了吸附时间、溶液p H值、温度及镉离子初始浓度对吸附的影响。实验结果表明,改性木质素磺酸钠水凝胶对镉离子的平衡吸附量随着温度的上升而增加;p H值小于7时,镉离子的平衡吸附量随着p H值的增加而增大;p H值等于7时,镉离子的平衡吸附量最大。在室温下,p H值为7的水溶液中,该水凝胶对镉离子的平衡吸附量随着镉离子浓度的增加而增大,最大可达到225.2mg/g;吸附过程满足准二级动力学方程,并能较好地符合Langmuir等温吸附模型。     

一种羧甲基葡甘聚糖钛凝胶球的吸附性能

用钛交联羧甲基葡甘聚糖制得羧甲基葡甘聚糖钛凝胶球,研究该凝胶球对十二烷基苯磺酸钠(SDBS)的吸附性能。分别探究了吸附时间、p H值、Ti(SO_4)_2浓度、羧甲基葡甘聚糖(CMKGK)浓度、SDBS浓度及温度对吸附的影响。结果表明:Ti(SO_4)_2浓度为2%、CMKGM浓度为2%时制得的凝胶球吸附效果最佳,吸附反应在8h达到平衡,当SDBS溶液的pH值为4、初始浓度为2 000 mg·L~(-1),温度为298K时,凝胶球对SDBS的吸附量达到493 mg·g~(-1),而且吸附量随着SDBS溶液初始浓度的增大而增大。钛交联羧甲基葡甘聚糖凝胶球对SDBS的吸附符合Freundlich等温方程,升高温度不利于吸附。动力学研究表明此吸附遵从准二级动力学方程。     

明胶包埋黑根霉菌丝体对水中Pb^2＋吸附性能的研究

本文研究了明胶包埋黑根霉菌丝体的包埋条件及包埋后对水中Ｐｂ~（２＋）的吸附作用。结果表明，包埋比例为６／１（Ｗ／Ｗ），交联剂甲醛用量为２５％，凝胶化温度为４０℃，ＰＨ＝１０．０为包埋反应的最佳条件。包埋后的饱和吸附量可达１２１．２ｍｇ／ｇ，比未包埋黑根霉下降１０．８％。吸附平衡时间延长至８００分钟。ｐＨ值对吸附量有较大影响，ＰＨ＝４．０时，吸附最佳。升高温度有利于吸附。流速对动态吸附有很大影响。ＨＮＯ３和ＮａＯＨ可以对吸附剂进行解吸与再生，解吸率在９４％以上。明胶包埋后黑根霉具有较好的物理性能，断裂压缩强度为１２８．１Ｎ／ｃｍ２。     

磁性壳聚糖微球的制备及对Cr(Ⅵ)的吸附性能研究

用壳聚糖包埋磁流体,用戊二醛交联制成磁性壳聚糖微球,并用红外光谱表征其结构。用制备的磁性壳聚糖微球吸附Cr(Ⅵ)离子,考察了其对Cr(Ⅵ)离子的吸附性能;探讨了吸附时间、溶液pH值、吸附剂用量、温度、Cr(Ⅵ)起始浓度以及其他离子存在对Cr(Ⅵ)离子去除率的影响。实验结果表明,磁性壳聚糖微球吸附Cr(Ⅵ)离子的最佳条件为:吸附平衡时间40 min,最佳吸附pH值6左右,磁性壳聚糖微球用量10 mg,温度升高有利于提高磁性壳聚糖微球的吸附效率,Cr(Ⅵ)离子起始质量浓度为12μg/mL,无机盐的存在引起磁性壳聚糖微球的吸附性能降低。并且考察了吸附剂的再生性能,实验结果表明磁性壳聚糖微球具有良好的重复使用性。     

Hydrogel microspheres III. Temperature-dependent adsorption of proteins on poly-N-isopropylacrylamide hydrogel microspheres

Precipitation polymerization of N-isopropylacrylamide (NIPAM) with methylenebisacrylamide (MBAAm) in water at 70°C gave thermosensitive hydrogel microspheres. The adsorbability of proteins on the poly-NIPAM microspheres was found to depend on temperature. Below the lower critical solution temperature (LCST) of poly-NIPAM in an aqueous medium, that is, around 32°C, the microspheres hold a large amount of water inside and their surface is hydrophilic enough to suppress the adsorption of proteins. On the contrary, above 32°C, the micropheres deswell and their surface becomes hydrophobic and, consequently, susceptible to adsorption of a large amount of proteins. Proteins once adsorbed on the microspheres at a high temperature could be desorbed more or less by lowering the temperature to below 32°C. The extent of desorption at low temperatures was found to depend on the incubation time for adsorption at high temperatures.     

Preparation of Functional Fluorescent Microspheres Used for HTS and Their Interaction with Biomolecules

There is considerable interest in protein adsorption onto microspheres because of its importance in a wide range of biomedical applications, such as artificial tissues and organs, drug delivery systems, biosensors, solid-phase immunoassays, immunomagnetic cell separation and immobilized enzymes or catalyst. It has been well known that the interaction between proteins and microspheres plays important roles in this process. Major interaction involved in the adsorption can be classified as electrostatic, hydrophobic and hydrogen-bonding. Indeed, adsorption of proteins onto microspheres is a complex process and often can involve many dynamic steps, from the initial attachment of the protein on the surface of microspheres to the equilibrium. Also the conformation of proteins probably occurs to a certain degree of deformation or structural change due to the large area of contact. Recently, much interest has been shown in sulfonated microspheres, since sulfonate-group itself is one of components in bio-bodies, as well as is sensitive to the change of pH or ionic strength. Indeed, so far, scanty investigations have been performed in the full range. Also few researches have involved the data on adsorption rate and the maximum amount of protein adsorbed, or the reversibility of the process and conformational change of protein adsorbed as well.In present study, BSA (bovine serum albumin) was chosen as the model protein and sulfonated PMMA [poly(methyl methacrylate)] microspheres as the matrix to investigate the adsorption process.The purpose is to show some information especially the intrinsic information involved by the adsorption process Adsorption of BSA onto sulfonated microspheres (MS) has been investigated as a function of time, protein concentration and pH. The adsorption appears to be a reversible process and the presence of sulfonate groups can play important roles in the adsorption process, so as to increase the amount of protein adsorbed and influences the interaction of BSA molecules. Fig. 1 also shows that the reciprocation between unadsorbed and adsorbed BSA or rearrangement of adsorbed BSA molecules does not produce visible change in the properties of the adsorbed protein. Close to the isoelectric point of BSA (pI 4.7), the amount of protein adsorbed exhibits a maximum. A higher or lower pH results in the significant decrease of the adsorption amount. This is related to the dependence of BSA conformations at different pH conditions.     

Preparation and Kinetic Modeling of Cross-Linked Chitosan Microspheres Immobilized Zn(II) for Urea Adsorption

The preparation of Zn(II)-immobilized glutaraldehyde-crosslinked chitosan microspheres which was modified with epichlorohydrin, tetraethylenepentamine, and bromoacetic acid was presented in this work. The Zn(II)-immobilized value of the microspheres (Ac-TEPA-CS) is 43.6 mg g^?1, which is higher than the blank microspheres. The adsorption of urea onto Zn-Ac-TEPA-CS was studied in a batch system. Langmuir and Freundlich adsorption models were applied to describe the experimental isotherm and isotherm constant, and the kinetic of adsorption process were estimated. These data fits well with Langmuir isotherm and also indicated that the adsorption process is exothermic and follow the pseudo-second-order kinetics. The adsorption capacity depends upon the pH, the temperature and the initial concentration of urea. It observed that Zn-Ac-TEPA-CS could be repeatedly used by elution and regeneration without significant loss of adsorption capacity.     

胺基化PGMA交联微球对胆红素的吸附机理

通过胺基与环氧键之间的开环反应, 用己二胺及多乙烯多胺等小分子胺化试剂对聚甲基丙烯酸缩水甘油酯(PGMA)交联微球进行了化学改性, 制得了胺基化的PGMA交联微球, 研究了该功能微球对胆红素的吸附特性, 考察了胺化试剂的分子结构、介质pH值、离子强度及温度等因素对其吸附性能的影响, 较深入地研究了吸附机理. 实验结果表明, 胺基化微球对胆红素具有强吸附作用, 吸附容量可达17.80 mg·g-1, 等温吸附服从Freundlich方程. 胺基化微球与胆红素分子之间的作用力以静电相互作用为主, 同时也存在氢键作用与疏水相互作用. 在pH 值为6 的介质中二者之间的静电作用最强, 胆红素吸附容量最高. 高离子强度不利于静电相互作用, 盐度增大使吸附容量减小. 温度升高有利于疏水相互作用而不利于氢键作用, 两种作用中占优势者主导温度对吸附容量的影响. 用己二胺改性的微球, 由于疏水相互作用的强化以及较长连接臂导致较小的空间位阻, 使其对胆红素的吸附能力明显高于多乙烯多胺改性的微球.     

A thermosensitive amphoteric microsphere and its potential application as a biological carrier

Thermosensitive poly(N-isopropylacrylamide) moieties were introduced onto amphoteric styrene/glycidyl methacrylate copolymer seed microspheres prepared by use of amphoteric initiators. The resulting microspheres exhibited thermosensitive and amphoteric behavior, so dual sensitivity to both pH and temperature was observed. The colloidal properties of the microspheres before and after seeded polymerization were characterized by varying the temperature and the pH. The results indicated that the specific surface structure emerged when the environmental conditions were changed. In addition, the reactive epoxy groups on the microsphere surface could be utilized to immobilize the protein molecules. The behavior of protein adsorption and immobilization onto the microspheres was examined in order to understand their potential applications in biological areas.     

壳聚糖微球负载的己二胺型聚酰胺-胺树状大分子的制备及对胆红素的吸附

通过反相悬浮反应制备了戊二醛交联的壳聚糖微球。以所制备的壳聚糖微球为载体,合成了己二胺型低代数聚酰胺-胺（Polyamidoamine,简称PAMAM）树枝状大分子（Genaration≤3）。考察了该微球在生理条件下对水溶液中胆红素的吸附行为,以及溶液的pH值,离子强度,温度,胆红素初始浓度,牛血清白蛋白等因素对吸附的影响。结果表明,吸附剂对胆红素具有良好的吸附性能,CS-G2.0,CS-G3.0,CS-G1.0,CS-G0和CS微球的平衡吸附率分别为94.61%,93.44%,92.97%,86.47%,52.38%,CS-G1.0-G3.0微球在0.5h吸附率已经超过70%,1h基本接近平衡,对胆红素的吸附量高达42.78mg/g。     

Study of interaction of proteins with fumed silica in aqueous suspensions by adsorption and photon correlation spectroscopy methods

The interaction of fumed silica A-300 (S(BET) = 297 m2 g(-1)) with bovine serum albumin (prepared by different methods), ovalbumin, human hemoglobin, and gelatin as a function of pH, salinity, and concentrations of components in aqueous medium was studied by adsorption and photon correlation spectroscopy (PCS) methods. Comparison of equilibrium (incubation time t(i) approximately 1 h) adsorption of proteins on A-300, minute (t(i) approximately 1 min) flocculation rate, and the particle size distributions measured by the PCS method shows different rearrangement of particle swarms depending on pH, salinity, and concentration of proteins, especially at pH close to IEP of silica or proteins. The electrokinetic mobility of protein/silica swarms is greater than that of individual components at pH far from the IEP of proteins. Changes in the Gibbs free energy (DeltaG) on protein adsorption depend on pH (-DeltaG is minimal at pH 2, close to the IEP of silica, and maximal at pH between the IEP of protein and silica), concentration (-DeltaG is maximal at C(p) between 1 and 6 mg/ml), type of proteins, and their preparation technique.