Activity of carboxypeptidase a bound to a modified cellulosic matrix

Carboxypeptidase A immobilized on acid chloride of oxidized cellulose showed the following features: (a) as indicated by the linearity of reaction kinetics, the immobilized enzyme action is not diffusion controlled; (b) greater flow rates are achievable with less clogging during continual usage since the enzyme is attached to a porous screen; (c) ease of handling; and (d) no apparent electrostatic interaction with the support material that is uncharged. The immobilized enzyme retained 60% of the original activity. The half-life of free enzyme was only 20 min, whereas for immobilized enzyme it was enhanced up to 2 h 48 min. It could be recovered and repeatedly used.     

Suzuki Reaction of Aryl Bromides Using a Phosphine-Free Magnetic Nanoparticle-Supported Palladium Catalyst

A palladium catalyst immobilized on superparaganetic nanoparticles was prepared with a palladium loading of 0.30 mmol/g. The catalyst was characterized using X-ray diffraction, scanning electron microscopy, transmission electron microscopy, vibrating sample magnetometry, thermogravimetric analysis, Fourier transform infrared, atomic absorption spectrophotometry, and nitrogen adsorption. The immobilized palladium catalyst was an efficient catalyst without added phosphine ligands for the Suzuki cross-coupling reaction of several aryl bromides with phenylboronic acid. The recovery of catalyst was simply by magnetic decantation in the presence of a magnet. The immobilized palladium catalyst can be reused many times without significant degradation in catalytic activity. No leaching of active palladium species into the reaction solution was detected.     

固定化酶催化合成CCK-8C-端三肽衍生物

报道胆囊收缩素（CCK-8）C-末端片段三肽衍生物外Hpac-Met_Asp(Cam为起始 原料，采用三种固定化酶--α-糜蛋白酶／Celite-545、木瓜蛋白酶／VA-Epoxy、 步酶促反应得到目标三肽化合物．对酶的专一性、酶的固定化、溶剂选择和合成条 件等进行了研究，比较了自由酶法与固定化酶法的结果．     

Amplified Detection of NAD+ and NADH by the Enzymatic Cycling with the Use of Immobilized Enzymes in a Flow System

Abstract

The enzymatic cycling for the detection of NAD⁺ and NADH in low level was carried out in the flow system with immobilized enzymes. Alcohol dehydrogenase and glutamate dehydrogenase immobilized on Sepharose 4B were used for the cycling reaction. The compound produced in the enzymatic cycling reaction was subjected to an enzymatic reaction to yield NADH, which was detected fluorometrically.     

Flow-through chemiluminescence sensor using immobilized oxidases for the selective determination of L-glutamate in a flow-injection system.

A selective and sensitive chemiluminometric flow sensor for the determination of L-glutamate in serum, based on immobilized oxidases such as glutamate oxidase (GOD), uricase (UC) and peroxidase (POD), is described herein. The principle for the selective chemiluminometric detection for L-glutamate is based on coupled reactions of four sequentially aligned immobilized oxidases, UC/POD/GOD/POD in a flow cell. The immobilized UC was employed to decompose urate, which is one of the major interfering components in serum for a luminol-H2O2 chemiluminescence reaction. The H2O2 produced from the UC reaction readily reacted with reducing components, such as ascorbate and glutathione, and then the excess H2O2 was decomposed by the immobilized POD. L-Glutamate in the sample plug was enzymatically converted to H2O2 with immobilized GOD. Subsequently, the peroxide reacts with luminol on the immobilized POD to produce chemiluminescence, proportional to glutamate concentration. The enzymes were immobilized on tresylated poly(vinyl alcohol beads). The immobilized enzymes were packed into TPFE tube (1.0 mm i.d. x 60 cm), in turn, and used as a flow cell. The sampling rate was 30 h-1. The calibration graph for L-glutamate is linear for 20 nM-5 microM; the detection limit (signal-to-noise = 3) is 10 nM.     

Enzymatic Synthesis of a CCK-8 Tripeptide Fragment

A process for the synthesis of CCK-8 tripeptide H-Gly-Trp-Met-OH catalyzed by immobilized enzyme was reported. Enzymes were used for the formation of peptide bonds and the removal of protecting group. Starting with phenylacetyl (PhAc) glycin, N-protected dipeptide PhAc-Gly-Trp-OMe was obtained by coupling PhAc-protected glycine carboxamidomethyl ester (OCam) with Trp-OMe catalyzed by immobilized papain in buffered ethyl acetate. Then the condensation between PhAc-Gly-Trp-OMe and Met-OEtoHC1 was carried out by immobilized α-chymotrypsin catalysis in solvent free system. Basic hydrolysis was followed getting PhAc-Gly-Trp-Met-OH. The PhAc-group was removed with penicillin G amidase and H-Gly-Trp-Met-OH was obtained in an overall yield of 43.9%. The reaction conversion of tripeptide in solvent free system was strongly affected by the system of basic salts added. The influence of the support materials used to deposit enzymes and structures of acyl donor and nucleophile on the reaction was also investigated.     

Solid-phase synthesis of isoindolinones and naturally-occurring benzobutyrolactones (phthalides) using a cyclative-cleavage approach

Starting from Merrifield resin, 2-formylbenzoic acids were immobilized on solid supports. Reactions between immobilized 2-formylbenzoic acids and different organometallic reagents (Grignard reagents, zinc reagents, allyl silanes via Sakurai type reactions) furnished secondary alcohols which cyclized depending on the metal counter ion and reaction conditions, forming benzoannelated lactones. Asymmetric synthesis was possible on the resin using chiral [2.2]paracyclophane ligands. While the reaction of immobilized ortho-carboxy benzaldehydes with primary amines at elevated temperatures yielded 3-hydroxyisoindolinones, a reaction at ambient temperature allowed imine formation, which underwent 1,2-addition-cleavage reaction with various nucleophiles, yielding isoindolinones with three points of diversity.     

一种新型低密度脂蛋白吸附剂的制备

通过在环氧化的交联聚乙烯醇球上固载多乙烯多胺和磺酸基团的方法制备一种新型的低密度脂蛋白吸附剂.环氧化的交联聚乙烯醇球首先与乙二胺或二乙烯三胺、三乙烯四胺及四乙烯五胺等多乙烯多胺进行胺化反应,由此获得不同长度悬臂,而后将胺化的环氧化的交联聚乙烯醇球与DMF/ClSO₃H反应,从而固载磺酸基团.磺酸基团的固载量随交联度的减小和聚乙烯醇浓度的增大而增大.初步研究证实,该类吸附剂具有较大的吸附量和较好的选择性.     

Carbonylation reaction of aryl halides on a polymer support using in situ-generated carbon monoxide without the assistance of microwaves

Palladium-catalyzed carbonylation, which was based on a ligand exchange reaction, efficiently converted immobilized aryl halides to amides under mild reaction conditions using molybdenum hexacarbonyl [Mo(CO)(6)] as the carbon monoxide source. The method easily operates without irradiating with microwaves and yields a wide range of highly pure amides after cleaving from the resin. The method could also be applied to the carbonylation of immobilized amines with aryl halides and to construct heterocyclic systems via a carbonylative cyclization.     

壳聚糖固定化胰蛋白酶的研究

以壳聚糖为载体，戊二醛为交联剂，采用两种方法制备了固定化胰蛋白酶。考察了固定化反应中pH值，戊二醛的浓度，以及给酶量对固定化胰蛋白酶活力的影响，并研究了这两种固定化胰蛋白酶的性质。实验结果表明，以戊二醛预交联的网状壳聚糖为载体制备的固定化胰蛋白酶具有更加优良的性能，在最佳固定化反应条件下，酶的活性加收率可达56％。此固定化胰蛋白酶的最适pH为7．0－8．5，最适温度为60℃，Km值为2．52mol/L，固定化胰蛋白酶表现出较好的热稳定性，pH贮存稳定性，以及在乙醇水溶液中的稳定性。     

用嗜热菌蛋白酶催化合成天冬甜精并同时进行DL-苯丙氨酸甲酯的光学拆分

以DL-苯丙氨酸甲酯作原料,利用嗜热菌蛋白酶和固定化嗜热菌蛋白酶催化合成了天冬甜精,经拆分得到D-苯丙氨酸甲酯。实验结果表明,不仅天冬甜精产率高,而且D-苯丙氨酸甲酯的回收率好,光学纯度高。     

氨化大孔球状聚氯乙烯固定化木瓜蛋白酶的研究

以氨化大孔球状聚氯乙烯为载体,采用戊二醛载体交联的方法,将木瓜蛋白酶进行了固定化。以酪蛋白为底物,测定了固定化酶的活力回收。研究了固定化条件对固定化酶活力回收的影响。同时,对所得固定化酶的性质,如温度-活力关系、pH-活力关系、热稳定性以及重复使用性进行了考察。结果表明,所得固定化木瓜蛋白酶具有较好的稳定性和重复使用性。     

Determination of glutamate-pyruvate transaminase activity in blood serum with a pyruvate oxidase/poly(vinyl chloride) membrane sensor

Pyruvate oxidase (E.C. 1.2.3.3.) is immobilized by adsorption on a wet PVC membrane. Glutamate-pyruvate transaminase activity (5–1600 IU l^?1) in serum is determined by a pyruvate oxidase sensor consisting of the immobilized pyruvate oxidase coupled to a platinum electrode for measuring hydrogen peroxide, after an l-alanine—α-ketoglutarate reaction. The assay requires ?60 s, and has a precision of 2–3%. Endogenous pyruvate should not interfere if measurements are made > 30 s after starting the reaction.     

Preparation,characterization, and application of a novel immobilized carboxypeptidase B

Pig pancreas carboxypeptidase B has been immobilized by covalent attachment to a polyacrylamide-type bead support possessing carboxylic functional groups activated by water-soluble carbodiimide. The optimum conditions of immobilization were determined. The activation of the support and the coupling reaction were performed in 0.1 M sodium citrate/sodium phosphate buffer (pH 4.5) using a support-carbodiimide-enzyme weight ratio 4:8:1 at 0-4 degrees C. Under such conditions, the highest activity achieved was 6700 U/g solid. The catalytic properties and stability of immobilized carboxypeptidase B were studied and compared with the corresponding properties of the soluble enzyme. The specific activity of the immobilized enzyme calculated on bound protein basis was about 70% of that of soluble enzyme. The optimum pH for the catalytic activity of the immobilized carboxypeptidase B was practically identical with that of soluble enzyme (pH 7.6-7.7). The apparent optimum temperature of the immobilized carboxypeptidase B was about 7 degrees C higher than that of the soluble enzyme. With hippuryl-L-arginine as substrate, Kmapp value of the immobilized enzyme was tenfold higher than the Km value of the soluble enzyme. The conformational stability of the enzyme was markedly enhanced by the strongly hydrophylic microenvironment in a wide temperature and pH range. The immobilized carboxypeptidase B was used for stepwise digestion of cytochrome C.     

固定化木瓜蛋白酶的制备和性质研究

多孔硅球固定化木瓜蛋白酶具有热增活性 .本文在前文研究的基础上 ,用载体交联法制备了甲壳胺固定化木瓜蛋白酶和纤维素固定化木瓜蛋白酶 .考察了固定化pH值、戊二醛浓度和给酶量对固定化木瓜蛋白酶活力的影响 .研究了固定化木瓜蛋白酶的性质 ,特别是热稳定性和耐热性 ,并与溶液酶和多孔硅球固定化木瓜蛋白酶进行了比较 .所制得的甲壳胺固定化木瓜蛋白酶和纤维素固定化木瓜蛋白酶的最适反应温度均达到了 80℃ ;90℃温育 1h后固定化酶的活力保持在 95 %以上 ;70℃温育处理 5h和 6h后固定化酶的活力也仍能保持在 90 %以上 .固定化木瓜蛋白酶的热稳定性和耐热性得到了显著提高     

固定化嗜热菌蛋白酶催化合成二肽甜味剂Aspartame

以氨丙基多孔硅球作载体,以戊二醛作交联剂制备的固定化嗜热菌蛋白酶催化合成Aspartame前体,通过酸化脱盐、氢化等反应得到二肽甜味剂Aspartame。研究了反应条件对合成Aspartame前体产率的影响,考察了固定化酶的重复使用性能。结果表明,固定化酶在水相中能较好的催化合成Aspartame前体,且具有良好的重复使用性能。     

Investigations of the Enhancer Effect of a High-Salt Concentration Medium on the Luminol Chemiluminescent Reaction

The enhancer effect of a high-salt concentration medium on the luminol chemiluminescence reaction catalyzed by either soluble or immobilized peroxidase has been investigated. Some widely used salts were tested at high concentration (up to 3 mol L): potassium chloride, sodium chloride, ammonium sulfate and calcium chloride. The magnitude of the light intensity enhancement depends on the nature of the salt and on the form of the peroxidase, i.e. free in solution or immobilized. The enhancement is observed whether the catalyst of the chemiluminescence reaction is peroxidase or ferricyanide. Both the enhanced or nonenhanced luminol chemiluminescence spectra have a maximum wavelength emission at around 425 nm. The results reported in this study are in favor of an action of the salts on the nonenzymatic steps of the luminol chemiluminescence reaction rather than a modification of the enzymatic process.     

Synthesis of dopamine and serotonin derivatives for immobilization on a solid support

The two important neurotransmitters dopamine and serotonin are synthesized with short PEG tethers and immobilized on a magnetic solid support. The tether is attached to the aromatic moiety of the neurotransmitters to conserve their original functional groups. This approach causes minimal alteration of the original structure with the aim of optimizing the immobilized neurotransmitters for aptamer selection by SELEX. For the dopamine derivative, the tether is attached to the aromatic core of a dopamine precursor by the Sonogashira reaction. For serotonin, a link to the indole core is introduced by a Claisen rearrangement from the allylated phenol moiety of serotonin. The tethers are azide-functionalized, which enables coupling to alkyne-modified magnetic beads. The coupling to the magnetic beads is quantified by UV spectroscopy using Fmoc-monitoring of the immobilized dopamine and serotonin derivatives.     

固载Ru基催化剂上二氧化碳加氢合成甲酸Ⅱ反应条件对催化剂性能的影响

The synthesis of formic acid from carbon dioxide and hydrogen using a silica immobilized ruthenium catalyst as precursor has been studied in different reaction conditions. The results revealed that the TOF （turn over frequency） of HCOOH achieved 1481.5 h^-1 on immobilized ruthenium catalyst near the critical pressure point of CO2 with H2 pressure of 4.0 MPa, reaction temperature of 80℃ and PPh3/Ru molar ratio of 6：1. The reaction activity of immobilized catalyst was higher than that of homogeneous catalyst, and the immobilized catalyst also offered the practical advantages such as easy separation and reuse.     

Enhancing electron transfer at a cytochrome c-immobilized microelectrode and macroelectrode

The redox reaction of cytochrome c immobilized on the bare surfaces of microelectrodes and macroscopic electrodes (macroelectrodes) composed of different planes of highly oriented pyrolytic graphite has been investigated using cyclic voltammetry. The protein-immobilized microelectrodes were fabricated using a simple masking method. For both macroelectrodes and microelectrodes, the redox reaction of immobilized cytochrome c needs to be activated by increasing the electrochemical potential maximum of cyclic voltammetry to a high positive value. The redox currents of this protein-electrode system can be enhanced using two approaches. The oxidation and reduction currents of cytochrome c adsorbed on microelectrodes that are composed of the edge plane show an anomalous enhancement compared to those for macroelectrodes composed of the basal plane. The difference in the surface chemical properties of the two kinds of electrodes results in the current anomaly. The oxidation current of the macroelectrode can be selectively enhanced by decreasing the potential minimum.