22 research outputs found

    Situación de la agricultura actual en Andalucía: el olivar de Jaén

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    MEDIO RURAL Y SOSTENIBILIDAD IV CONGRESO ANDALUZ DE DESARROLLO SOSTENIBLE VIII CONGRESO ANDALUZ DE CIENCIAS AMBIENTALE

    Eliminación de Cu2+ de efluentes acuosos

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    Se presenta un estudio de eliminación de Cu2+ por adsorción sobre pasta de celulosa al sulfato. Se han obtenido las isotermas de equilibrio a la temperatura de 30'0° C y pH 4,5 y 6, respectivamente. En los tres casos las curvas se ajustan a funciones del tipo Koble-Corrigan, con n = 2. Para los mismos pH y concentraciones de 1, 3, 5, 7 y 10 ppm de Cu2+ se han trazado los frentes de adsorción. Finalmente, siguiendo el tratamiento de Michaels se han calculado, a partir de dichos frentes, las distintas características del proceso: LUB, V, f, G, Ntoc, y Htoo, respectivamente

    Elimination of 4-chlorophenol from Water Solutions Using Commercial Peroxidases

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    A comparative study of the two most widely used commercial peroxidases (E.C. 1.11.1.7) for removing 4-chlorophenol from aqueous industrial effluents is presented. Both the peroxidases tested, horseradish peroxidase (HRP) and soybean peroxidase (SBP), showed maximal removal efficiency in a neutral pH medium although they maintained more than 70 % of their activity in a pH range of between 6.0 and 8.0. The influence of temperature on the elimination levels was negligible between T = 25 and 40 °C for both enzymes. To minimize the treatment period and enzyme dose, the effect of adding different amounts of a protective agent (polyethylene glycol, PEG) was explored. The final choice of the peroxidase source will depend on the convenience of using such protective agents, SBP being the most suitable when the addition of PEG is not possible or desirable

    Hydrogel coated monoliths for enzymatic hydrolysis of penicillin G

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    The objective of this work was to develop a hydrogel-coated monolith for the entrapment of penicillin G acylase (E. coli, PGA). After screening of different hydrogels, chitosan was chosen as the carrier material for the preparation of monolithic biocatalysts. This protocol leads to active immobilized biocatalysts for the enzymatic hydrolysis of penicillin G (PenG). The monolithic biocatalyst was tested in a monolith loop reactor (MLR) and compared with conventional reactor systems using free PGA, and a commercially available immobilized PGA. The optimal immobilization protocol was found to be 5 g l−1 PGA, 1% chitosan, 1.1% glutaraldehyde and pH 7. Final PGA loading on glass plates was 29 mg ml−1 gel. For 400 cpsi monoliths, the final PGA loading on functionalized monoliths was 36 mg ml−1 gel. The observed volumetric reaction rate in the MLR was 0.79 mol s−1 m−3monolith. Apart from an initial drop in activity due to wash out of PGA at higher ionic strength, no decrease in activity was observed after five subsequent activity test runs. The storage stability of the biocatalysts is at least a month without loss of activity. Although the monolithic biocatalyst as used in the MLR is still outperformed by the current industrial catalyst (immobilized preparation of PGA, 4.5 mol s−1 m−3catalyst), the rate per gel volume is slightly higher for monolithic catalysts. Good activity and improved mechanical strength make the monolithic bioreactor an interesting alternative that deserves further investigation for this application. Although moderate internal diffusion limitations have been observed inside the gel beads and in the gel layer on the monolith channel, this is not the main reason for the large differences in reactor performance that were observed. The pH drop over the reactor as a result of the chosen method for pH control results in a decreased performance of both the MLR and the packed bed reactor compared to the batch system. A different reactor configuration including an optimal pH profile is required to increase the reactor performance. The monolithic stirrer reactor would be an interesting alternative to improve the performance of the monolith-PGA combination

    Decolorization and partial mineralization of a polyazo dye by Bacillus firmus immobilized within tubular polymeric gel

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    The degradation of C.I. Direct red 80, a polyazo dye, was investigated using Bacillus firmus immobilized by entrapment in tubular polymeric gel. This bacterial strain was able to completely decolorize 50 mg/L of C.I. Direct red 80 under anoxic conditions within 12 h and also degrade the reaction intermediates (aromatic amines) during the subsequent 12 h under aerobic conditions. The tubular gel harboring the immobilized cells consisted of anoxic and aerobic regions integrated in a single unit which was ideal for azo dye degradation studies. Results obtained show that effective dye decolorization (97.8%), chemical oxygen demand (COD) reduction (91.7%) and total aromatic amines removal were obtained in 15 h with the immobilized bacterial cell system whereas for the free cells, a hydraulic residence time of 24 h was required for an equivalent performance in a sequential anoxic and aerobic process. Repeated-batch experiments indicate the immobilized cells could decolorize C.I. Direct red 80 and reduce medium COD in five successive batch runs with enhanced activity obtained after each consecutive run, thus suggesting its stability and potential for repeated use in wastewater treatment. UV–visible spectrophotometry and HPLC analysis were used to confirm the partial mineralization of the dye. Data from this study could be used as a reference for the development of effective industrial scale biotechnological process for the removal of dyes and their metabolites in textile wastewater

    Characterization of an Aminoacylase from the Hyperthermophilic Archaeon Pyrococcus furiosus

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    Aminoacylase was identified in cell extracts of the hyperthermophilic archaeon Pyrococcus furiosus by its ability to hydrolyze N-acetyl-l-methionine and was purified by multistep chromatography. The enzyme is a homotetramer (42.06 kDa per subunit) and, as purified, contains 1.0 ± 0.48 g-atoms of zinc per subunit. Treatment of the purified enzyme with EDTA resulted in complete loss of activity. This was restored to 86% of the original value (200 U/mg) by treatment with ZnCl(2) (and to 74% by the addition of CoCl(2)). After reconstitution with ZnCl(2), the enzyme contained 2.85 ± 0.48 g-atoms of zinc per subunit. Aminoacylase showed broad substrate specificity and hydrolyzed nonpolar N-acylated l amino acids (Met, Ala, Val, and Leu), as well as N-formyl-l-methionine. The high K(m) values for these compounds indicate that the enzyme plays a role in the metabolism of protein growth substrates rather than in the degradation of cellular proteins. Maximal aminoacylase activity with N-acetyl-l-methionine as the substrate occurred at pH 6.5 and a temperature of 100°C. The N-terminal amino acid sequence of the purified aminoacylase was used to identify, in the P. furiosus genome database, a gene that encodes 383 amino acids. The gene was cloned and expressed in Escherichia coli by using two approaches. One involved the T7 lac promoter system, in which the recombinant protein was expressed as inclusion bodies. The second approach used the Trx fusion system, and this produced soluble but inactive recombinant protein. Renaturation and reconstitution experiments with Zn(2+) ions failed to produce catalytically active protein. A survey of databases showed that, in general, organisms that contain a homolog of the P. furiosus aminoacylase (≥50% sequence identity) utilize peptide growth substrates, whereas those that do not contain the enzyme are not known to be proteolytic, suggesting a role for the enzyme in primary catabolism
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