固化条件对环氧树脂/丙烯酸酯橡胶共混体系结构与性能的影响

利用丙烯酸酯橡胶(ACM)提高热固性环氧树脂(EP)的韧性,系统研究共混体系固化条件对材料结构和性能的影响.研究表明,固化前环氧树脂与丙烯酸酯橡胶在整个组成范围内为均相体系,固化过程中两组份分子量不断增大,部分组成环氧树脂/丙烯酸酯橡胶共混体系(80/20及50/50)发生反应诱导相分离现象(RIPS).在发生反应诱导相分离的体系中,分相后的环氧树脂和丙烯酸酯橡胶两相彼此包含对方的组分,是一种不彻底的相分离.同时,固化后材料的结构与性能强烈依赖于所用固化条件(包括固化时间、固化温度及固化剂含量等).因此,可以通过调节体系固化条件实现对环氧树脂/丙烯酸酯橡胶共混体系结构和性能的调控.     

UV-光固化光纤涂料的研制

本文采用环氧丙烯酸酯与聚氨酯丙烯酸酯共混聚合的方法制备出新型的UV-光固化光纤涂料,其主要性能较好.研究了基体组成、引发剂、稀释剂以及固化工艺对UV-固化光纤涂料的光固化速度的影响.通过实验发现,环氧丙烯酸酯与聚氨酯丙烯酸酯的配比为 4:6～6:4、稀释剂的含量不大于20%时固化速度较快、性能较好,同时固化时灯距与固化膜厚度对固化速度的影响较大.     

一类高速固化光敏树指的合成及表征

光敏树脂具有节约能源、污染小、固化速度快、生产效率高、适宜流水线生产等优点,近年来得到了快速发展[1 4]。对于光敏树脂,固化速度是最重要的指标之一,它直接关系到生产效率、能源消耗以及固化树脂的性能。本文采用多元脂肪胺及含多元双键的丙烯酸酯通过迈克尔加成反应合成了一类UV快速固化光敏树脂,粘度较低,成膜性好,成本较低,在实际生产中有广阔的应用前景。1　实验部分1 1　试剂仪器乙二胺(AR,中国医药上海化学试剂公司);三乙烯四胺(AR,宜兴试剂三厂);三丙二醇二丙烯酸酯(TPGDA,工业品);三羟甲基丙烷三丙烯酯酯(TMPTA,工…     

紫外光固化涂料及其发展状况

紫外光固化涂料具有高效率、低消耗的特点,是一种新型环保节能型涂料。文章综述了紫外光固化涂料的特点、固化原理、主要组成包括齐聚物、活性稀释剂、光引发剂和助剂以及紫外光固化涂料的发展前景。     

紫外光固化水性树脂的研究与应用

介绍了紫外光固化水性树脂的分类,着重从引入的亲水基团种类的不同介绍了阴离子型、阳离子型以及非离子型三种水性UV固化自乳化型聚氨酯丙烯酸酯树脂的分类与制备,以及国内外的最新研究进展;并对水性UV固化聚氨酯丙烯酸酯树脂的其它相关研究进行了概述,简要介绍了水性UV固化树脂的相关应用.     

电子束固化含氟聚氨酯丙烯酸酯的制备与性能

以六亚甲基二异氰酸酯三聚体、丙烯酸羟乙酯及羟基含氟丙烯酸酯为原料制备了电子束固化含氟聚氨酯丙烯酸酯预聚物. 通过傅里叶变换红外光谱(FTIR)和核磁共振氢谱(¹H NMR)对产物进行了表征. 研究了产物与溶剂组成的两相混合体系的流变性能、电子束固化行为及固化后涂层性能. 结果表明, 产物与溶剂混合体系具有正触变性, 绝对黏度变化符合Sedden公式, 黏流活化能约为44.8 kJ/mol. 电子束固化后涂层性能(如热稳定性、硬度、附着力和光泽度)优良.     

光/潮气双重固化聚氨酯涂层的制备及性能研究

以甲苯-2,4-二异氰酸酯(TDI)和二乙醇胺(DEOA)为原料一步法合成了超支化聚氨酯,对其改性制备了光固化超支化聚氨酯丙烯酸酯(HPUA)和一系列双重固化(UV/潮气)超支化聚氨酯丙烯酸酯(DHPUA),使用傅立叶红外光谱(FT-IR)、核磁共振氢谱(1H-NMR)和碳谱(13C-NMR)以及凝胶色谱(GPC)对其分子结构进行了表征.并以其为预聚物制备光固化涂层,通过对双重固化涂层的表面形貌、热性能和物理性能的研究,结果表明,超支化双重固化涂层经过潮气固化后,涂层表面的粗糙度随着树脂中硅氧烷端基的含量的增加先下降后上升;超支化双重固化涂层的物理性能和热稳定性都随着树脂中硅氧烷端基的含量的增加而提升.     

树枝状多氨基环氧树脂固化剂的合成及其固化行为

树枝状多氨基环氧树脂固化剂的合成及其固化行为;树枝状大分子;丙烯酸酯双键;乙二胺(EDA)     

紫外光固化聚氨酯丙烯酸树脂的研究进展

综述了紫外光固化聚氨酯丙烯酸酯树脂的研究,讨论了其合成方法、固化机理以及性能。     

氨酯丙烯酸酯树脂的合成及其固化反应动力学研究

用不同分子量的聚氧化丙烯二元醇合成了一系列氨酯丙烯酸酯齐聚物（ＵＡＯ）以及含硬段／软段结构的ＵＡＯ，并用ＦＴ－ＩＲ跟踪了这类ＵＡＯ的合成过程。通过ＵＡＯ的链端双键测定，以及ＧＰＣ、ＶＰＯ测定的分子量，表征了ＵＡＯ的数均官能团度。进一步通过ＦＴ－ＩＲ研究了由ＵＡＯ与甲基丙烯酸甲酯形成的氨酯丙烯酸酯树脂（ＵＡＲ）固化时的共聚反应动力学，发现其共聚反应速率与体系中的扩散效应密切相关。在这类ＵＡＯ中引入硬段后，共聚合体系呈现出反常的动力学行为，与网络结构形成过程中材料的形态发展有关。     

Self-assembly of Acridine Orange into H-aggregates at the air/water interface: tuning of orientation of headgroup

The surface active derivative of the organic dye Acridine Orange (N-10-dodecyl-acridine orange (DAO)) has been included in mixed Langmuir monolayers with stearic acid (SA). The maximum relative content on DAO for a stable mixed monolayer is a molar ratio of X(DAO) = 0.5. Brewster angle microscopy (BAM) reveals a high homogeneity at the micrometer level for the mixed monolayer in equimolar proportion (X(DAO) = 0.5), whereas the appearance of domains occurs for lower content of DAO, i.e., X(DAO) = 0.2 and 0.1. The aggregation of the DAO headgroup leads to well-defined H-aggregates at the air/water interface for those mixed monolayers with a low content of DAO. However, for the mixed monolayers enriched in DAO, e.g., X(DAO) = 0.5, the molecular crowding prevents the formation of defined supramolecular structures. Molecular organization and tilting of the DAO headgroup is quantitatively analyzed by in situ UV-visible reflection spectroscopy. The formation of H-aggregates of the DAO headgroup can be reversibly tuned with the applied surface pressure. A molecular mechanism for the conformational rearrangement of the DAO molecule is proposed using RM1 quantum semiempirical calculations.     

Human D-amino acid oxidase: an update and review

The flavoprotein D-amino acid oxidase (DAO) degrades the gliotransmitter D-Ser, a potent activator of N-methyl-D-aspartate-type glutamate receptors. A body of evidence suggests that DAO, together with its activator, G72 protein, may play a key role in the pathophysiology of schizophrenia. It has also been suggested that 3,4-dihydroxy-D-phenylalanine (D-DOPA), the stereoisomer of 3,4-dihydroxy-L-phenylalanine (L-DOPA), is oxidized by DAO and converted to dopamine via an alternative biosynthetic pathway. We determined the crystal structures of human DAO in complex with the reaction products of two clinically important substrates, D-Ser and D-DOPA. Kinetic data show that the maximum velocity is much greater for D-DOPA than that for D-Ser, which strongly supports the proposed alternative pathway for dopamine biosynthesis in the treatment of Parkinson's disease. In addition, biochemical characterization of human DAO indicates that it binds FAD more weakly than does porcine D-amino acid oxidase (pDAO) and exists as a stable homodimer, even in the apoprotein form. Determination of the structures of human DAO in various states reveals that, in contrast to pDAO, the hydrophobic-Val-Ala-Ala-Gly-Leu (VAAGL) stretch (residues 47-51, structurally ambivalent peptide) located at the si-face of the flavin ring assumes a uniquely stable conformation, which provides a structural basis for the unique kinetic features of human DAO.     

In vitro determination of diamine oxidase activity in food matrices by an enzymatic assay coupled to UHPLC-FL

Intestinal diamine oxidase (DAO) acts as a protective barrier against exogenous histamine. A deficit of DAO activity can lead to the appearance of histamine intolerance, a clinical condition that may be treated by a low-histamine diet and oral DAO supplementation to enhance intestinal histamine degradation. As sources of DAO, porcine kidneys and certain legume seedlings are suitable components for the formulation of a DAO supplement. The aim of this work was to develop a rapid and reliable methodology for the in vitro determination of DAO activity in food matrices based on an enzymatic assay coupled to UHPLC-FL. The proposed method showed a satisfactory linearity and sensitivity and provided a relative standard deviation lower than 3%, guaranteeing method precision, and a mean recovery greater than 99% both for lyophilized pea sprouts and porcine kidney protein extracts. A high specificity is a key attribute of this method due to the use of histamine as the reaction substrate and the direct quantification of its degradation. Moreover, the lack of interference of catalase and hydrogen peroxide is another advantage in comparison with previously published methods. Lyophilized pea sprouts showed the greatest histamine-degrading activity (0.40 ± 0.01 mU/mg), followed by porcine kidney protein extracts (0.23 ± 0.01 mU/mg) and commercial DAO supplements (0.09 ± 0.06 mU/mg). This technique could be used as a tool to validate the DAO activity of food matrices of potential interest for the treatment of histamine intolerance.

     

Zymographic assay of plant diamine oxidase on entrapped peroxidase polyacrylamide gel electrophoresis. A study of stability to proteolysis

A zymographic assay of diamine oxidase (DAO, histaminase, EC 1.4.3.6), based on a coupled peroxidase reaction, and its behavior at proteolysis in simulated gastric and intestinal conditions, are described. The DAO activity from a vegetal extract of Lathyrus sativus seedlings was directly determined on sodium dodecyl sulfate polyacrylamide electrophoretic gels containing entrapped horseradish peroxidase, with putrescine as substrate of histaminase and ortho-phenylenediamine as co-substrate of peroxidase. The accumulation of azo-aniline, as peroxidase-catalyzed oxidation product, led to well-defined yellow-brown bands on gels, with intensities corresponding to the enzymatic activity of DAO. After image analysis of gels, a linear dependency of DAO content (Coomassie-stained protein bands) and of its enzymatic activity (zymographic bands) with the concentration of the vegetal extract was obtained. In simulated gastric conditions (pH 1.2, 37 °C), the DAO from the vegetal extract lost its enzymatic activity before 15 min of incubation, either in the presence or absence of pepsin. The protein pattern (Coomassie-stained) revealed that the DAO content from the vegetal extract was kept almost constant in the simulated intestinal fluid (containing pancreatin or not), with a slight diminution in the presence of pancreatic proteases. After 10 h of incubation at 37 °C, the DAO enzymatic activity from the vegetal extract was 44.7% in media without pancreatin and 13.6% in the presence of pancreatin, whereas the purified DAO retained only 4.65% of its initial enzymatic activity in the presence of pancreatin.      

Highly Sensitive Determination of DAO Activity by Oxidation of a Luminescence Reagent

A highly sensitive method for measuring the activity of the enzyme diamine oxidase (DAO) independent of the type of substrate is described. The principle of the assay is to determine the amount hydrogen peroxide generated as a reaction product during oxidation of diamines by DAO. PSatto™, a highly sensitive luminescence reagent, was used to generate a signal depending on the hydrogen peroxide concentration based on the action of horseradish peroxidase. DAO is specifically captured from a sample by an antibody immobilized to microwell plates, and the substrate is added to the bound enzyme. Various diamines were used as substrates; the peroxide produced is directly proportional to the amount of DAO bound to the specific antibodies. With this very sensitive method, it is possible to detect pmol amounts of generated hydrogen peroxide in plasma matrix corresponding to the biological activity of DAO.     

Studies of the Polymerization of Diallyl Compounds. XL. Correlation between Addition Modes and Evolution of Carbon Dioxide in the Polymerization of Diailyl Oxalate

The occurrence of head-to-head (HH) addition in the radical polymerization of diallyl oxalate (DAO) was examined under various polymerization conditions. The content of HH linkage in poly (DAO) was reduced in comparison with allyl acetate and diallyl succinate; this may be ascribed to the high polarity of DAO inducing a polar effect on the intermolecular propagation of the growing polymer radical, resulting in reduced HH addition. The correlation between addition modes and evolution of carbon dioxide characteristic of DAO polymerization at elevated temperatures is mechanistically discussed in detail, with special focus on the solvent effect and the reduced dismutation of the cyclized radical compared to the uncyclized one.     

辽河稠油减渣深度戊烷脱沥青的研究

以戊烷为溶剂,在脱沥青实验装置上对辽河稠油减渣进行梯级分离,得到轻脱油、重脱油和脱油沥青。在温度155℃~170℃、压力为4.0 MPa~7.0 MPa,考察了温度、压力变化对脱沥青油收率及性质的影响。用超临界萃取分馏的实验结果关联了脱沥青油残炭、N元素、Ni元素的脱除率。结果表明,压力升高、温度降低,脱沥青油收率增加,轻、重脱油的残炭值及S、N、Ni、V等元素含量升高,脱沥青油性质变差。在脱沥青油收率最高为74.23%时,Ca、Ni元素的脱除率分别为92.75%、74.50%;残炭的脱除率为62.13%;N、S元素的脱除率分别为40.17%、24.10%。超临界萃取馏分油的杂质脱除率与脱沥青油的杂质脱除率有较好的相关性。     

Polyurethane acrylate-stabilized cholesteric liquid crystal dispersions

Polymer stabilized cholesteric liquid crystals (PSCLCs) have been fabricated based on various structures of polyurethane acrylate (PUA) as well as conventional acrylate polymer, namely poly(1,6-hexanediol diacrylate). For PUA stabilized films, the transmittance spectra of cured films were essentially identical to those of uncured films, with no 'dead' reaction; whereas, using acrylate polymer; reflection greatly decreased upon curing and showed significant 'dead' reaction after the cessations of irradiation. The structure of PUA also had significant effects on the electro-optic performance, and these effects are interpreted in terms of elasticity and interfacial interaction between the polymer and LC.     

A high‐performance liquid chromatography assay with a triazole‐bonded column for evaluation of d‐amino acid oxidase activity

Elution profiles of kynurenic acid (KYNA) and 7‐chlorokynurenic acid (Cl‐KYNA) were examined by high‐performance liquid chromatography (HPLC) using a triazole‐bonded stationary phase column (Cosmosil® HILIC) under isocratic elution of a mobile phase consisting of CH₃CN–aqueous 10 mm ammonium formate between pH 3.0 and 6.0. The capacity factors of KYNA and Cl‐KYNA varied with both the CH₃CN content and the pH of the mobile phase. The elution order of KYNA and Cl‐KYNA was reversed between the CH₃CN‐ and H₂O‐rich mobile phases, suggesting that hydrophilic interactions and anion‐exchange interactions caused retention of KYNA and Cl‐KYNA in the CH₃CN‐ and H₂O‐rich mobile phases, respectively. The present HPLC method using a triazole‐bonded column and fluorescence detection (excitation 250 nm, emission 398 nm) was applied to monitor in vitro production of KYNA from d ‐kynurenine (d ‐KYN) by d ‐amino acid oxidase (DAO) using Cl‐KYNA as an internal standard. A single KYNA peak was clearly observed after enzymatic reaction of d ‐KYN with DAO. Production of KYNA from d ‐KYN was suppressed by the addition of commercial DAO inhibitors. The present HPLC method can be used to evaluate DAO activity and DAO inhibitory effects in candidate drugs for the treatment of schizophrenia. Copyright © 2015 John Wiley & Sons, Ltd.     

Catalytic, asymmetric aza-Baylis-Hillman reaction of N-sulfonated imines with activated olefins by quinidine-derived chiral amines

The chiral nitrogen Lewis base, tricyclic cinchona alkaloid derivative TQO, is an effective promoter in the catalytic, asymmetric aza‐Baylis–Hillman reaction of N‐sulfonated imines Ar? CH?NR′ 1 (R′ = Ts, Ms, Ns, SES) with various activated olefins such as methyl vinyl ketone (MVK), ethyl vinyl ketone (EVK), acrolein, methyl acrylate, phenyl acrylate, or α‐naphthyl acrylate to give the corresponding adducts in moderate to good yields with good to high ee (up to 99 %) at ?30 °C or 45 °C in various solvents, including DMF/MeCN (1:1, v/v). The first such reaction of 1 with the simplest Michael acceptor MVK and methyl acrylate has been achieved with excellent enantioselectivity. The adducts derived from MVK and EVK had the opposite absolute configuration to those from acrolein, methyl acrylate, phenyl acrylate, and α‐naphthyl acrylate. A plausible mechanism has been proposed on the basis of previous reports and the authors’ investigations. An effective bifunctional chiral nitrogen Lewis base–Brønsted acid system has been revealed in this type of aza‐Baylis–Hillman reaction.