聚脲多孔材料的简单制备及在酶固定和手性拆分中的应用

以甲苯二异氰酸酯(TDI)为单体,在水与丙酮混合溶剂中通过沉淀聚合一步法制备了富含胺基的聚脲多孔材料(PPU),通过扫描电镜和压汞法对其表面形貌和孔结构进行了表征.PPU经戊二醛(GA)活化后用于荧光假单胞菌脂肪酶(PFL)的固定,考察了GA活化过程中GA浓度对酶固定量及固定酶活性的影响.结果表明,PPU是一种粒子尺寸分布在30~50μm范围的形状不规则的多孔粒子,孔径在2 nm~100μm之间呈连续分布.在pH=8.0的缓冲溶液中用0.17 mol/L的GA对PPU进行改性,将改性后的PPU用于PFL的固定,当酶溶液浓度为2.56 mg/m L时,得到酶的最大固定量为95.2 mg/g,固定酶的活性为375 U/mg,相对活性为76%.将此固定酶作为催化剂,用于1-苯乙醇外消旋化合物的手性拆分,并与游离酶催化的结果相比较.结果表明,固定酶的反应活性和立体选择性都明显优于游离酶.通过沉淀聚合制备的聚脲多孔材料在酶固定及手性分子拆分方面具有应用前景.     

Amination of Poly(ethylene-terephthalate) polymer surface for biochemical applications

Amine functionalization of Poly(ethylene-terephthalate) (PET) films for covalent binding of peptides is described. Ammonia plasma treatments have been used to graft nitrogen-containing functional groups onto the PET surface. The samples were then analyzed by X-ray photoelectron spectroscopy (XPS) and a parametric study was performed to define the best plasma grafting conditions. For biological tests, samples were sterilized by steam autoclaving: this induces a four to fivefold loss of the nitrogen functional groups on the polymer surface. XPS does not differentiate easily between the various nitrogen groups present on the surface so it is difficult to estimate the amount of surface amine groups available for direct coupling of bioactive molecules (proteins, peptides, nucleic acids, ...). To obtain a direct measurement of the amines present, we assayed for cysteine fixation through its carboxylic group by detection of the thiolaminoacid by XPS. We obtained cysteine fixation, showing the presence of grafted primary amine functions on PET surface after ammonia plasma treatment. Radiochemical assays were also made to quantify the amount of amine groups on plasma treated PET. XPS, cysteine fixation and radiochemical assays all show the presence of amine functions on ammonia plasma treated PET.     

Conductive AFM patterning on oligo(ethylene glycol)-terminated alkyl monolayers on silicon substrates: proposed mechanism and fabrication of avidin patterns

Micro- and nanopatterns of biomolecules on inert, ultrathin platforms on nonoxidized silicon are ideal interfaces between silicon-based microelectronics and biological systems. We report here the local oxidation nanolithography with conductive atomic force microscopy (cAFM) on highly protein-resistant, oligo(ethylene glycol) (OEG)-terminated alkyl monolayers on nonoxidized silicon substrates. We propose a mechanism for this process, suggesting that it is possible to oxidize only the top ethylene glycol units to generate carboxylic acid and aldehyde groups on the film surface. We show that avidin molecules can be attached selectively to the oxidized pattern and the density can be varied by altering the bias voltage during cAFM patterning. Biotinylated molecules and nanoparticles are selectively immobilized on the resultant avidin patterns. Since one of the most established methods for immobilization of biomolecules is based on avidin-biotin binding and a wide variety of biotinylated biomolecules are available, this approach represents a versatile means for prototyping any nanostructures presenting these biomolecules on silicon substrates.     

Immobilized streptavidin gradients as bioconjugation platforms

Surface density gradients of streptavidin (SAV) were created on solid surfaces and demonstrated functionality as a bioconjugation platform. The surface density of immobilized streptavidin steadily increased in one dimension from 0 to 235 ng cm(-2) over a distance of 10 mm. The density of coupled protein was controlled by its immobilization onto a polymer surface bearing a gradient of aldehyde group density, onto which SAV was covalently linked using spontaneous imine bond formation between surface aldehyde functional groups and primary amine groups on the protein. As a control, human serum albumin was immobilized in the same manner. The gradient density of aldehyde groups was created using a method of simultaneous plasma copolymerization of ethanol and propionaldehyde. Control over the surface density of aldehyde groups was achieved by manipulating the flow rates of these vapors while moving a mask across substrates during plasma discharge. Immobilized SAV was able to bind biotinylated probes, indicating that the protein retained its functionality after being immobilized. This plasma polymerization technique conveniently allows virtually any substrate to be equipped with tunable protein gradients and provides a widely applicable method for bioconjugation to study effects arising from controllable surface densities of proteins.     

Development of an efficient amine-functionalized glass platform by additional silanization treatment with alkylsilane

Aminosilane-treated molecular layers on glass surfaces are frequently used as functional platforms for biosensor preparation. All the amino groups present on the surface are not available in reactive forms, because surface amino groups interact with remaining unreacted surface silanol groups. Such nonspecific interactions might reduce the efficiency of chemical immobilization of biomolecules such as DNA, enzymes, antibodies, etc., in biosensor fabrication. To improve immobilization efficiency we have used additional surface silanization with alkylsilane (capping) to convert the remaining silanol groups into Si–O–Si linkages, thereby liberating the amino groups from nonspecific interaction with the silanol groups. We prepared different types of capped amine surface and evaluated the effect of capping on immobilization efficiency by investigating the fluorescence intensity of Cy3-NHS (N-hydroxysuccinimide) dye that reacted with amino groups. The results indicate that most of the capped amine surfaces resulted in enhanced efficiency of immobilization of Cy3-NHS compared with the untreated control amine surface. We found a trend that trialkoxysilanes had greater capping effects on immobilization efficiency than monoalkoxysilanes. It was also found that the aliphatic chain of alkylsilane, which does not participate in the capping of the silanol, had an important function in enhancing immobilization efficiency. These results would be useful for preparation of an amine-modified surface platform, with enhanced immobilization efficiency, which is essential for developing many kinds of biosensors on a silica matrix. Enhancement of amine funtionality by capping with alkylsilane     

Expedient generation of patterned surface aldehydes by microfluidic oxidation for chemoselective immobilization of ligands and cells

An expedient and inexpensive method to generate patterned aldehydes on self-assembled monolayers (SAMs) of alkanethiolates on gold with control of density for subsequent chemoselective immobilization from commercially available starting materials has been developed. Utilizing microfluidic cassettes, primary alcohol oxidation of tetra(ethylene glycol) undecane thiol and 11-mercapto-1-undecanol SAMs was performed directly on the surface generating patterned aldehyde groups with pyridinium chlorochromate. The precise density of surface aldehydes generated can be controlled and characterized by electrochemistry. For biological applications, fibroblast cells were seeded on patterned surfaces presenting biospecifc cell adhesive (Arg-Glyc-Asp) RGD peptides.     

Chemical modifications of inert organic monolayers with oxygen plasma for biosensor applications

In this paper we present a study of using oxygen plasma for chemically modifying inert hydrocarbon self-assembled monolayers of octadecyltrichlorosilane (OTS-SAMs) and rendering active surfaces for protein immobilization. Detailed surface modification and protein immobilization were characterized by using ellipsometry, X-ray photoelectron spectroscopy (XPS), Fourier transform infrared-attenuated total reflectance spectroscopy, and fluorescence microscopy. Our XPS results showed that the surface reaction between OTS-SAMs and oxygen plasma can generate new surface functional groups such as alcohol (C-O), aldehyde (C=O), and carboxylic acid (O-C=O), and their compositions can be controlled by using different treatment times and powers. A short treatment time ( approximately 1 s) and high power (10 W) can lead to a higher density of aldehyde groups, which can serve as linker groups for protein immobilization through the formation of Schiff bases with the amine groups of proteins. By using the fluorescence immunostaining method, we confirmed that human immunoglobulin (IgG) can be immobilized on a glass slide, only if the surface was decorated with OTS-SAMs and if the OTS-SAMs were pretreated with oxygen plasma. The protein immobilized on the oxygen-plasma-treated surface can only be recognized by using a highly specific antibody, FITC-anti-IgG, but not FITC-anti-biotin.     

Tuning the Surface Properties of Oxygen-Rich and Nitrogen-Rich Plasma Polymers: Functional Groups and Surface Charge

Controlling the concentration and nature of functional groups in plasma polymer films by adjusting the flow ratio of constituent precursor gases can be exploited to tune the surface charge of the resulting coating. Plasma polymer films containing various concentrations of nitrogen and oxygen functional groups were deposited in a low-pressure capacitively-coupled glow discharge reactor by plasma polymerization of binary gas mixtures of a hydrocarbon (ethylene or butadiene) and a heteroatom source gas (ammonia and/or carbon dioxide). Increasing the flow ratio of heteroatom to hydrocarbon gases increased the concentration of bonded nitrogen or oxygen, including that of primary amine or carboxylic groups as determined by X-ray photoelectron spectroscopy and chemical derivatization procedures. The zeta potential of samples was measured using an electro-kinetic analyser in a diluted sodium chloride solution. The deposition parameters controlled the composition of the coatings, allowing to tune the surface charge to either positive (ammonia based films)—or negatively (carbon dioxide base films) values at physiological pH.     

Determination of accessible amino groups on surfaces by chemical derivatization with 3,5-bis(trifluoromethyl)phenyl isothiocyanate and XPS/NEXAFS analysis

The determination of amino groups on surfaces capable of binding biomolecules is important for the understanding and optimization of technologically relevant coupling processes. In this study, three different types of amino-functionalized model surfaces, amino thiolate on Au, amino siloxane on Si, and polyethylene (PE) foils and films reacted with 1,2-diaminoethane (DAE) were derivatized with 3,5-bis(trifluoromethyl)phenyl isothiocyanate. Subsequently, these samples were analyzed by chemical derivatization X-ray photoelectron spectroscopy (CD-XPS) and near-edge X-ray absorption fine structure spectroscopy (NEXAFS). The determination of amino groups by this analytical approach allows gaining insight into the availability of groups on surfaces that can actually serve as attachment sites for biomolecules in technical applications. In the case of the amino thiolate on Au, almost 90% of the expected amino groups were detected by CD-XPS. Investigation of the amino siloxane films revealed lower yields for the derivatization reaction in the order of 30%. The lowered reaction yields are thought to be due to interactions between the amino siloxane’s amino and silanol groups or the underlying substrate, making them inaccessible to the derivatization agent. The aminated PE samples are characterized by a complex surface chemistry and structure, and reaction yields of the derivatization reaction cannot be unequivocally derived. However, 1–3% of the total carbon atoms in the surface layer were found to be bound to amino groups accessible to the derivatization agent. It can be concluded that, depending on the detailed character of the investigated amino-terminated surface, the amount of amino groups accessible to CD-XPS can be substantially lower than the total amount of amino groups present at the surface.     

Poly(phenylene oxide) films modified with allylamine plasma as a support for invertase immobilization

The paper describes a method for preparation of polymer support suitable for covalent invertase immobilization. Modification of poly(phenylene oxide) films by plasma polymerization of allylamine has been applied to introduce amine functionality on the polymer surface. It has been observed that the polymer surface became covered in plasma by a loosely fixed, moderately hydrophilic layer that should be removed before the immobilization process. The chemical character of the stable sub-layer has been related to several modification parameters: geometry of reactor, mode of plasma action and composition of gaseous mixture. Methods for determination of surface concentration of amine groups have also been presented and discussed from the immobilization point of view.     

聚丙烯表面的生物相容性修饰: 表面氨基放大还原胺化接枝磷酰胆碱

在氨气氛中对聚丙烯薄膜表面进行等离子处理, 获得了不同浓度的表面氨基. 表面氨基的数量经1,6-己二异氰酸酯键合三(2-氨乙基)胺可成倍增加. 用还原胺化法将磷酰胆碱醛共价接枝到表面氨基上获得了磷酰胆碱改性的聚丙烯薄膜. X射线光电子能谱(XPS)测定结果表明, 接枝磷酰胆碱基团的表面覆盖率可达20%～40%. 衰减全反射傅立叶变换红外(ATR-FTIR)和动态接触角测定结果也都说明磷酸胆碱基团被成功地接枝于聚丙烯表面. 还原胺化法结合等离子处理及表面氨基放大技术, 有望成为获取新型生物材料的一种有效途径.     

Bio‐Orthogonal Polymer Coatings for Co‐Presentation of Biomolecules

Controlled presentation of biomolecules on synthetic substrates is an important aspect for biomaterials development. If the immobilization of multiple biomolecules is required, highly efficient orthogonal surface chemistries are needed to ensure the precision of the immobilization. In this communication, chemical vapor deposition (CVD) copolymerization is used to fabricate polymer coatings with controlled ratio of alkyne and pentafluorophenyl ester (Pfp‐ester) groups. Cyclic argine‐glycine‐aspartic acid (cRGD) adhesion peptide and epidermal growth factor (EGF) are immobilized through alkyne–azide cycloaddtion (“click” chemistry) and active ester–amine reaction, respectively. Cell studies with human umbilical vein endothelial cells (HUVEC) and A431 cell lines demonstrate the biological activity of the coimmobilized biomolecules.     

A Comparison of PE Surfaces Modified by Plasma Generated Neutral Nitrogen Species and Nitrogen Ions

The surface modification of polyethylene (PE) by neutral nitrogen species (ground and excited state N₂ as well as atomic N; modified nitrogen plasma treatment) has been compared to the effect of nitrogen ion bombardment using X-ray Photoelectron Spectroscopy (XPS) and contact angle measurements. XPS results indicate that a greater nitrogen concentration was grafted during the modified nitrogen plasma treatment of PE, an effect that was attributed to surface sputtering during ion beam modification. The distribution of nitrogen-containing functionalities was strongly dependent upon the treatment strategy; the modified nitrogen plasma treatment lead predominantly to imine groups being formed at the PE surface, while amine groups were the dominant species produced during ion beam modification. The presence of electron irradiation during the modified nitrogen plasma treatment of PE did not modify the rate of nitrogen incorporation or change the nature of N-containing functional groups produced but did lead to a systematic decrease in contact angle.     

Photo-oxidative degradation of polyethylene: Effect of polymer characteristics on chemical changes and mechanical properties. Part 1—Quenched polyethylene

Photo-oxidative degradation of quenched samples of linear low density (LLD), medium density (MD) and two kinds of high density (HD) polyethylene (PE) films was studied using a medium-pressure mercury lamp. Greater amounts of crosslinking and build up of oxidation products were noticed in LLDPE than the other samples. The primary products of interaction between dienes and oxygen are considered to participate in the initiation of the photo-oxidation reactions. Using the FT-IR difference spectrum technique, the amount of branch concentration in the photo-irradiated PE samples was determined. Oxidation damage at the boundary region between crystalline and amorphous phases is considered to be important in determining the embrittlement time.     

Immobilization of Heparin and Highly-Sulphated Hyaluronic Acid onto Plasma-Treated Polyethylene

Heparin and highly-sulphated hyaluronic acid have been successfully immobilized onto plasma-processed polyethylene via a diamine polyethyleneglycol (PEG) spacer molecule. Two different plasma-processes have been utilized, i.e. a treatment and a deposition process, for providing polyethylene surface with the COOH groups necessary for the immobilization reactions. XPS integrated with derivatization procedures, ATR-FTIR and Water Contact Angle measurements have been carried out for characterizing each modification step: 1) the plasma-process, 2) the immobilization of the spacer molecule and 3) the immobilization of the biomolecules. The thrombin time of the modified surfaces has been measured, and their platelet activation characteristics evaluated. The results indicate a certain nonthrombogenic character of the biomolecule-immobilized polyethylene samples.     

Novel synthetic route for covalent coupling of biomolecules on super‐paramagnetic hybrid nanoparticles

The immobilization of biomolecules on magnetic nanoparticles is an issue with high potential in different fields. We describe herein a new strategy to immobilize biomolecules on super‐paramagnetic nanoparticles based on the reactivity of vinyl sulfone groups with naturally occurring functional groups present in biomolecules (amine and thiol). A new monomer containing a polymerizable methacryloyl group and a secondary amine group was synthesized and used to prepare super‐paramagnetic hybrid nanoparticles (SP‐HNPs) by two‐step miniemulsion polymerization. The Michael addition reaction of divinyl sulfone (DVS) to the secondary amine groups localized on the nanoparticles surface allows the introduction of the vinyl sulfone function in the SP‐HNPs (SP‐HNPs‐VS). The morphology of the functionalized SP‐HNPs was characterized by transmission electron microscopy (TEM), high‐resolution transmission electron microscopy (HRTEM), dynamic light scattering, and magnetic susceptibility. The capacity of SP‐HNPs‐VS for the immobilization of biomolecules was evaluated with three model proteins: avidin, invertase, and horseradish peroxidase (HRP). The model proteins were successfully immobilized in mild aqueous conditions compatible with the biological nature of the enzymes. © 2012 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem, 2012     

Well-defined micropatterns of polymers prepared by controlled crystallization process

Surface confined recrystallization of highly-oriented polyethylene (PE) thin films realized by carbon-coating was utilized to control the morphological structure of ultrathin PE films. Selective carbon-coating with the help of a mask and subsequent recrystallization of the pre-oriented PE thin film lead to a partially structural control of the PE thin film in the coated domains. A fully structural control of the PE film is then fulfilled through a combination of surface confinement and heteroepitaxy of PE on the oriented poly(tetrafluroethylene) (PTFE) thin film. The thus obtained structure can serve as a template to induce pattern structures of a variety of other polymers through epitaxial growth. The poly(ε-caprolactone) (PCL) and poly(butylenes adipate) (PBA) micropattern thin films are shown in this paper as examples. These thin films exhibit different birefringence in different regions depending on the molecular orientation and may find potential applications in the fields of polarization-dependent display or storage.     

Natural weathering test for films of various formulations of low density polyethylene (LDPE) and linear low density polyethylene (LLDPE)

Natural (outdoor) weathering test was performed to investigate the UV stability of thin films (0.06 mm) of linear low density polyethylene (LLDPE) and low density polyethylene (LDPE). The PE films were prepared from various formulations of LLDPE and LDPE resins. Some of these films contained a single high molecular mass HALS only, along with a primary antioxidant (i.e. Irganox 1010) and a secondary antioxidant (i.e. Irgafos 168 or Alkanox TNPP), while others contained HALS and UVA (i.e. Chimassorb 81 or Tinuvin P or Tinuvin 326) along with these antioxidants. The HALS used was either an oligomeric or a synergistic mixture of a high molecular mass (HMM) hindered amine stabilizer and co-additives. The UV stability was investigated by exposing the prepared films at 45° towards south in the direct sunshine up to 365 days. Fifty percent of tensile strength retention was determined for all these exposed films and it was found that the films containing a single HALS gained improved UV stability by about two to 12 fold over the pure films. On the other hand, films that contained a combination of HALS and UVA obtained further improved UV stability over the films containing a single HALS (both have antioxidants). Films containing a single HALS reached 50% TS retention within 205 days, whereas, films containing a combination of HALS and UVA reached 50% TS retention within 590 days, which is about three times further improvement in UV stability.     

HDPE,LLDPE或LDPE高取向薄膜微结构的电子显微学研究

木工作用透射电子显微术及电子衍射技术研究3种PE(HDPE,LLDPE或LDPE)均聚物高取向薄膜的微结构。定量测定了它们的结晶尺寸。通过倾斜样品电子显微学研究确定了不同种PE纤维结构的对称性。     

Immobilization of amine-modified oligonucleotides on aldehyde-terminated alkanethiol monolayers on gold

Chemistry is described for the fabrication of DNA arrays on gold surfaces. Alkanethiols modified with terminal aldehyde groups are used to prepare a self-assembled monolayer (SAM). The aldehyde groups of the monolayer may be reacted with amine-modified oligonucleotides or other amine-bearing biomolecules to form a Schiff base, which may then be reduced to a stable secondary amine by treatment with sodium cyanoborohydride. The surface modifications and reactions are characterized by polarization modulation Fourier transform infrared reflection absorption spectroscopy (PM-FTIRRAS), and the accessibility, binding specificity, and stability of the DNA-modified surfaces are demonstrated in hybridization experiments.