Poly(vinyl alcohol) Ultrafiltration Membranes: Synthesis,Characterization, the Use for Enzyme Immobilization

An enzymatic hydrolysis in a symmetric membrane, combining reaction and separation, has been studied. PVA hydrogel was chosen because of its hydrophilicity expecting to minimize membrane fouling and concentration polarization. The membrane pores containing covalently bound enzymes serve as catalyst support. The membrane immobilization of the enzyme and the filtration mode of operating the process were chosen in order to avoid product inhibition of the enzyme. The properties of cross‐linked PVA hydrogel were investigated. The conversion of the hydrolysis of p‐nitrophenyllaurate with two different loadings of Cr lipase was evaluated. The conversion of the reaction decreased with both increasing substrate flux and initial concentration. The kinetic parameters were obtained. Compared to the free lipase, the K_m of the membrane bonded enzyme was lower and its R_max approximately the same.     

聚乙烯醇降解酶研究进展

聚乙烯醇是一种广泛应用的水溶性聚合物,尤其作为纺织浆料。由于其生物难降解性,对水体会造成较大的污染,因此得到较多的关注。对聚乙烯醇生物处理的研究主要集中在生物降解酶和生物降解机理上,特别是随着对环境友好的酶加工纤维技术的不断发展,利用聚乙烯醇降解酶进行纺织脱浆已引起较大的兴趣。已发现的聚乙烯醇降解酶主要包括:聚乙烯醇氧化酶(仲醇氧化酶)、聚乙烯醇脱氢酶、β双酮水解酶(氧化型聚乙烯醇水解酶)。聚乙烯醇降解酶催化聚乙烯醇的生物降解主要分为两步进行。聚乙烯醇酶脱浆技术不仅节省了脱浆能耗,而且提高了脱浆废水的生物可降解性。     

聚乙烯醇的生物降解

聚乙烯醇(PVA)是较少的可溶于水并被生物降解的乙烯聚合物之一。研究表明,在受PVA污染的自然环境中存在着能降解PVA的微生物,并从中提取出了PVA降解酶。介绍了国内外研究聚乙烯醇生物降解的情况。分别讨论了聚乙烯醇被单一菌种、共生细菌和真菌降解过程中的生物化学和生理学特性,以及结构因素对聚乙烯醇生物降解的影响。这些研究促进了可有效生物降解的PVA类材料产品项目的发展。     

Ion-Conductive Poly(vinyl alcohol)-Based IPMCs

Partially crosslinked and sulfonated poly(vinyl alcohol) (s-PVA) membranes were prepared as ion-conductive matrices of Ionic Polymer-Metal Composite (IPMC) and a new IPMC based on the s-PVA membrane was fabricated via an electroless plating procedure of platinum. PVA was reacted with sulfosuccinic acid (SSA) as a crosslinking agent with a sulfonic group and 4-(2-hydroxyethyl)piperazine-1-propanesulfonic acid (EPPS) as a side chain with a sulfonic group. The crosslinked s-PVA membranes were characterized using a FT-IR spectroscope and a scanning electron microscope-combined energy-dispersive X-ray spectrometer and were assessed in terms of water absorption, proton conductivity, and the feasibility of electroless plating. Among the prepared ionomers, the s-PVA membrane obtained at 20 wt.% SSA and 10 wt.% EPPS (S20E10 membrane) registered the highest proton conductivity of 2.9 × 10^?2 S·cm^?1, which corresponds to one third of that of Nafion series, and only the S20E10 membrane was successfully plated via the electroless plating method without any crack and broken part. The s-PVA-based IPMC showed the one-directional displacement with 1-minute-long time-lapse comparable to typical Nafion-based IPMCs. However, the displacement under an AC potential was very limited due to its slow deformation response and the actuation performance was severely varied with actuation time including the short service life of several minutes in air. The short and variable actuation of the s-PVA-based IPMC was attributed to its large variation of surface and ionic resistances during air-operation, which is induced by the low ratio of bound to free water.     

Modeling of a Catalyzed Reaction Using Lipase Immobilized in a Poly(vinyl alcohol) Membrane

A mathematical model for the hydrolysis reaction of p‐nitro phenol laurate catalyzed by a lipase immobilized in a membrane was developed. In an earlier study this model reaction was found to show very different reaction rates when it was performed in aqueous micellar solution with free enzyme and with membrane immobilized enzyme. It was assumed that a local accumulation of substrate in the membrane is responsible for the observed rate enhancement. The conversion of p‐nitro phenol ester within the membrane was modeled by considering a combination of the convective flow through poly(vinyl alcohol) membrane pores, concentration polarization of substrate containing micelles at the membrane surface and the kinetics of the reaction with free enzymes. It was demonstrated that the model offered a comprehensive understanding of the interaction of the involved phenomena. The modeling results are in good agreement with the experimental data from 10 runs with different enzyme and substrate concentrations. The substrate concentration at the membrane surface increased by up to a factor of 3 compared to the feed concentration. This effect explains the observed rate enhancement. Moreover, the model was used to determine the unknown parameters, i.e., the intrinsic retention and the mass transfer coefficient, by fitting the model to the experimental data. The model may also be used to calculate the optimum operating conditions and design parameters of such a reactor.     

Immobilization of biocatalysts with poly(vinyl alcohol) supports.

Two polymer materials, poly(vinyl alcohol) (PVA) superfine fibers and photocrosslinkable PVA bearing styrylpyridinium groups, have been developed to immobilize biocatalysts. The former has a large surface consisting of relatively large-size pores and the fibers can immobilize a large amount of biocatalyst on their surface by ionic interaction. The latter entraps many kinds of biocatalysts by cyclodimerization caused by visible light irradiation. The biocatalysts on/in these supports maintain high activity and thermal stability. These materials can easily be formed into various shapes suitable for various applications. A new bioreactor system was constructed for evaluating a variety of biocatalysts and supports.     

Poly(vinyl alcohol) functionalized poly(dimethylsiloxane) solid surface for immunoassay

In this communication, we describe a simple and robust method for the covalent bonding of poly(vinyl alcohol) (PVA) on a silanized poly(dimethylsiloxane) (PDMS) surface. Nonspecific adsorption of proteins via hydrophobic-hydrophobic interactions of the PVA-coated surface is greatly reduced, and biomolecules can be rapidly anchored on the PVA-coated surface with high loading and uniformity. On the basis of a sandwich immunoassay with the anti-rabbit IgG and IgG pair as a model, the detection limit for IgG is down to 1 pg/mL with linearity up to 11 microg the levels often encountered in biological, forensic, and environmental samples.     

Poly(vinyl alcohol) acetoacetate-based tissue adhesives are non-cytotoxic and non-inflammatory

Polymer-based tissue adhesives composed of poly(vinyl alcohol) acetoacetate (PVOH acac) and cross-linking amines were investigated for their effects on cell survival and inflammatory cell activation using in vitro mouse cell cultures. Cytotoxicity of tissue adhesives was evaluated by placing adhesives in direct contact with 3T3 fibroblast cells. Tissue adhesives formulated from PVOH acac and 3-aminopropyltrialkoxysilane (APS) were non-cytotoxic to fibroblasts; adhesives formulated from PVOH acac and aminated poly(vinyl alcohol) (PVOH amine) were also non-cytotoxic to fibroblasts. In contrast, a commercial adhesive composed of 2-octyl cyanoacrylate was highly cytotoxic to fibroblasts. The inflammatory potential of tissue adhesives was evaluated by exposing J774 macrophage cells to adhesives, and measuring TNF-α release from macrophages. PVOH acac-based tissue adhesives did not elicit inflammatory TNF-α release from macrophages. These results suggest that PVOH acac-based tissue adhesives are non-cytotoxic and non-inflammatory. Such tissue adhesives represent a promising technology for a variety of medical applications, including surgical wound closure and tissue engineering, and the results are also significant in the design of in vitro cell culture systems to study biomaterials.     

Immobilization of maltogenase onto polyurethane microparticles from poly(vinyl alcohol) and hexamethylene diisocyanate

A series of porous polyurethane (PU) microparticles from poly(vinyl alcohol) (PVA) and hexamethylene diisocyanate (HMDI) using different ratios of components were obtained by one step method. Molar compositions of PU microparticles were estimated by determination of nitrogen, isocyanate and hydroxyl groups. PU carriers which were synthesized using optimal initial molar ratios of PVA and HMDI were applied for immobilization of maltogenase (MG) from Bacillus stearothermophilus. Immobilized enzyme exhibited higher catalytic activity and enhanced temperature stability in comparison with the native MG. Maximal loading 7.78 mg/g wet carrier was reached when PU microparticles with initial molar ratio of PVA and HMDI = 1:3 was used as a carrier for immobilization. The high efficiency of immobilization (EI) was obtained using PU microparticles when initial molar ratio of HMDI and PVA was 1:1–1:10. High stability of MG immobilized onto PU microparticles during storage was demonstrated. Immobilized starch hydrolyzing enzyme was successfully tested in batch and column type reactors for hydrolysis of potato starch. MG immobilized onto PU enables easy separation from the reaction medium and reuse of the immobilized preparation over seven reaction cycles in bath operation and at least three cycles in column type reactor.     

Immobilization of hydrocarbon-oxidizing bacteria in poly(vinyl alcohol) cryogels hydrophobized using a biosurfactant

A simple biosurfactant-based hydrophobization procedure for poly(vinyl alcohol) (PVA) cryogels was developed allowing effective immobilization of hydrocarbon-oxidizing bacteria. The resulting partially hydrophobized PVA cryogel granules (granule volume 5 microl) contained sufficient number (6.5 x 10(3)) of viable bacterial cells per granule, possessed high mechanical strength and spontaneously located at the interface in water-hydrocarbon system. Such interfacial location of PVA granules allowed high contact of immobilized biocatalyst with hydrophobic substrate and water phase, thus providing bacterial cells with mineral and organic nutrients. As a result, n-hexadecane oxidation efficiency of 51% after 10-day incubation was achieved using immobilized biocatalyst. PVA cryogels with increased hydrophobicity can be used for immobilization of bacterial cultures performing oxidative transformations of water-immiscible organic compounds. Immobilization of in situ biosurfactant producing Rhodococcus bacteria into PVA cryogel is discussed. PVA cryogel granules with entrapped alkanotrophic rhodococcal cells were stable after 10-month storage at room temperature.     

Immobilization of tyrosinase and alcohol oxidase in conducting copolymers of thiophene functionalized poly(vinyl alcohol) with pyrrole

Immobilization of tyrosinase and alcohol oxidase is achieved in the copolymer of pyrrole with vinyl alcohol with thiophene side groups (PVATh-co-PPy) which is a newly synthesized conducting polymer. PVATh-co-PPy/alcohol oxidase and PVATh-co-PPy/tyrosinase electrodes are constructed by the entrapment of enzyme in conducting copolymer matrix during electrochemical copolymerization. For tyrosinase and alcohol oxidase enzymes, catechol and ethanol are used as the substrates, respectively. Kinetic parameters: maximum reaction rates (V(max)) and Michaelis-Menten constants (K(m)) are obtained. V(max) and K(m) are found as 2.75 micromol/(minelectrode) and 18 mM, respectively, for PVATh-co-PPy/alcohol oxidase electrode and as 0.0091micromol/(minelectrode) and 40 mM, respectively, for PVATh-co-PPy/tyrosinase electrode. Maximum temperature and pH values are investigated and found that both electrodes have a wide working range with respect to both temperature and pH. Operational and storage stabilities show that although they have limited storage stabilities, the enzyme electrodes are useful with respect to operational stabilities.     

Enzyme reactor with knitted fabric made of poly(vinyl alcohol) superfine filaments

Various supports and bio-reactors have been proposed. Packed bed reactors with polymer material in granular shape are most often employed in both laboratory and industry. But they have a disadvantage related to an increase in pressure drop. We already developed filter paper composed of short cut pieces of superfine filaments (SFF). It shows high performance, but its hydrodynamic resistance increases when substrate solution passes through it. A new type of enzyme reactor equipped with knitted SFF has been proposed. In this reactor, substrate does not pass through the support but flows along the thin channel and parallel to the support. Therefore, it is able to maintain flow rate constant during a considerable period. The productivity of the reactor fairly increases by reducing the thickness of the channel because linear velocity increases with the reduction of the thickness and that contributes to the decrease in mass transfer resistance.     

Poly(vinyl alcohol) hydrogel as a biocompatible viscoelastic mimetic for articular cartilage

The prevalence of suboptimal outcome for surgical interventions in the treatment of full-thickness articular cartilage damage suggests that there is scope for a materials-based strategy to deliver a more durable repair. Given that the superficial layer of articular cartilage creates and sustains the tribological function of synovial joints, it is logical that candidate materials should have surface viscoelastic properties that mimic native articular cartilage. The present paper describes force spectroscopy analysis by nano-indentation to measure the elastic modulus of the surface of a novel poly(vinyl alcohol) hydrogel with therapeutic potential as a joint implant. More than 1 order of magnitude decrease in the elastic modulus was detected after adsorption of a hyaluronic acid layer onto the hydrogel, bringing it very close to previously reported values for articular cartilage. Covalent derivatization of the hydrogel surface with fibronectin facilitated the adhesion and growth of cultured rat tibial condyle chondrocytes as evidenced morphologically and by the observance of metachromatic staining with toluidine blue dye. The present results indicate that hydrogel materials with potential therapeutic benefit for injured and diseased joints can be engineered with surfaces with biomechanical properties similar to those of native tissue and are accepted as such by their constituent cell type.     

Ion-Conductive Poly(vinyl alcohoi)-Based IPMCs

Partially crosslinked and sulfonated poly(vinyl alcohol) (s-PVA) membranes were prepared as ion-conductive matrices of Ionic Polymer-Metal Composite (IPMC) and a new IPMC based on the s-PVA membrane was fabricated via an electroless plating procedure of platinum. PVA was reacted with sulfosuccinic acid (SSA) as a crosslinking agent with a sulfonic group and 4-(2-hydroxyethyl)piperazine-1-propanesulfonic acid (EPPS) as a side chain with a sulfonic group. The crosslinked s-PVA membranes were characterized using a FT-IR spectroscope and a scanning electron microscope-combined energy-dispersive X-ray spectrometer and were assessed in terms of water absorption, proton conductivity, and the feasibility of electroless plating, Among the prepared ionomers, the s-PVA membrane obtained at 20 wt.% SSA and 10 wt.% EPPS (S20E10 membrane) registered the highest proton conductivity of 2.9 × 10~(-2) S·m~(-1), which corresponds to one third of that of Nafion series, and only the S20E10 membrane was successfully plated via the electroless plating method without any crack and broken part. The s-PVA-based IPMC showed the one-directional displacement with 1-minute-long time-lapse comparable to typical Nafion-based IPMCs. However, the displacement under an AC potential was very limited due to its slow deformation response and the actuation performance was severely varied with actuation time including the short service life of several minutes in air. The short and variable actuation of the s-PVA-based IPMC was attributed to its large variation of surface and ionic resistances during air-operation, which is induced by the low ratio of bound to free water.     

Immobilization of porcine pancreatic lipase on glycidyl methacrylate grafted poly vinyl alcohol

Graft copolymerization of glycidyl methacrylate (GMA) on to polyvinyl alcohol (PVA) using benzophenone (BP) as initiator was carried out. Grafted PVA was used as carrier for pancreatic lipase immobilization. The effects of GMA and BP concentrations as well as grafting reaction times on grafting yields and activities of the immobilized lipase were determined. The influence of enzyme concentrations was also studied. The optimal conditions for the grafting reaction were: 1 h at 15 mM BP and 2.3 M GMA, the optimum enzyme concentration for immobilization was 1 mg/ml. After optimization of the immobilization process a physical and chemical characterization of the immobilized enzyme was performed. Furthermore, the thermal, pH, storage and operational stability of the immobilized enzyme in comparison to the free form was tested.     

Purification and Characterization of an Esterase Involved in Poly(vinyl alcohol) Degradation by Pseudomonas vesicularis PD

An esterase catalyzing the hydrolysis of acetyl ester moieties in poly(vinyl alcohol) was purified 400-fold to electrophoretic homogeneity from the cytoplasmic fraction of Pseudomonas vesicularis PD, which was capable of assimilating poly(vinyl alcohol) as the sole carbon and energy source. The purified enzyme was a homodimeric protein with a molecular mass of 80 kDa and the isoelectric point was 6.8. The pH and temperature optima of the enzyme were 8.0 and 45°C. The enzyme catalyzed the hydrolysis of side chains of poly(vinyl alcohol), short-chain p-nitrophenyl esters, 2-naphthyl acetate, and phenyl acetate, and was slightly active toward aliphatic esters. The enzyme was also active toward the enzymatic degradation products, acetoxy hydroxy fatty acids, of poly(vinyl alcohol). The K _m and V _max of poly(vinyl alcohol) (degree of polymerization, 500; saponification degree, 86.5-89.0 mol%) and p-nitrophenyl acetate were 0.381% (10.6 mM as acetyl content in the polymer) and 2.56 μM, and 6.52 and 12.6 μmol/min/mg, respectively. The enzyme was strongly inhibited by phenylmethylsulfonyl fluoride and diisopropyl fluorophosphate at a concentration of 5 mM, which indicated that the enzyme was a serine esterase. The pathway for the metabolism of poly(vinyl alcohol) is also discussed.     

聚乙烯醇/葡聚糖复合凝胶的制备及药物释放规律的研究

目的:采用冷冻-解冻物理交联方法制备聚乙烯醇(PVA)和葡聚糖(Dextran)混合凝胶.并考察复合凝胶药物释放规律.方法:含有胰岛素的PVA/Dextran溶液置于-20℃条件下冷冻8 h,在室温下解冻4 h,反复冷冻-解冻数次制备得到胰岛素PVA/Dextran复合凝胶,反相高效液相色谱法考察了胰岛素的体外释放行为.结果:胰岛素复合凝胶体外释放模式符合Higuchi扩散方程.当PVA/Dextran比例从100/0降到80/20,胰岛素释放速率明显增加,最大释放率从45%增加到65%.当冷冻-解冻循环次数从2增加到6,胰岛素达到最大释放的时间从24 h增加到45 h,最大释放率从70%降到50%.释放介质的温度的升高能显著增加胰岛素的释放速率.结论:PVA/Dextran制备的胰岛素复合凝胶具有良好的缓释效果.PVA/Dextran复合凝胶是一种较有前景的水凝胶药物载体.     

Immobilization of hog pancreas lipase in macroporous poly(vinyl alcohol)-cryogel carrier for the biocatalysis in water-poor media

Hog pancreas lipase was covalently attached to the beads of poly(vinyl alcohol)-cryogel – a macroporous hydrogel prepared by means of freeze-thaw technique. The immobilized biocatalyst thus obtained was examined in the reaction of enantioselective hydrolysis of the ethyl ester of N-benzylidene derivative of DL-phehylalanine in the medium of acetonitrile (contained 5 vol.% of water without any buffers). Eighty-three %-enantiomeric excess of the l-amino acid was reached after 144 h. Virtually the same result was obtained in the repeated use of the same immobilized biocatalyst after its 6-months-storing in a refrigerator.     

Immobilization of enzyme onto poly(ethylene-vinyl alcohol) membrane

Invertase was ionically bound to the poly(ethylene-vinyl alcohol) membrane surface modified with two aminoacetals with different molecular length, 2-dimethyl-aminoacetoaldehyde dimethylacetal (AAA) and 3-(N, N-dimethylamino-n-propanediamine) propionaldehyde dimethylacetal (APA). Immobilization conditions were determined with respect to enzyme concentration in solution, pH value, ionic strength in immobilization solution, and immobilization time. Various properties of immobilized invertase were evaluated, and thermal stability was found especially to be improved by immobilization. The apparent Michaelis constant, K(m), was smaller for invertase bound by APA with longer molecular lengths than for invertase bound by AAA. We attempted to bind glucoamylase of Rhizopus delemar origin in the same way. The amount and activity of immobilized glucoamylase were much less than of invertase.