Isolamento e identificação de Klebsiella de solo de cerrado e o uso de suas enzimas para modificação química de fungicidas / Isolation and identification of Klebsiella in cerrado soil and its use of enzymes for chemical modification of fungicides

AUTOR(ES)

Flavio Marques Lopes

DATA DE PUBLICAÇÃO

2008

RESUMO

In this research, open ground samples (Brazilian Savannah Cerrado) proceeding from treated cultures of soy with Opera (epoxiconazol and piraclostrobin) had been used as source of resistant microorganisms to fungicide. The sample were collected in July 2006, in three points of planted area and two depths, 0 to 20 cm, and from 80 cm to 1m, next to the state highway GO-139, in the towns of São Miguel do Passa Quatro, in a producing farm model of soy seeds, where Opera was used since its launching in 2002. The collection point was characterized as a risk place for ecological accidents, presenting area with extensive agriculture activity, intense use of pest management, soil with good level of infiltration and storage of water, and areas of declivity. The microorganisms selection was carried through using selective solid J.E. supplemented with 0.1% of Opera with microorganisms collected in depth of 80cm. In a previous selection, 9 microorganisms were isolated, and from these, the one that showed a better growth within the selective J.E. liquid supplemented with 0.03% of Opera (1805) was chosen for the development of this research. The analysis for coloration of Gram-negative showed that the isolated microorganism is one bacillococcus Gram-negative with poliphormic characteristics, being sensible to all the tested antibiotics. Biochemical identification made through the method of Bactray, presented a correlaction of 99% with the genus Klebsiella. Through molecular identification by the gene 16S rDNA, it was possible to find a correlaction of 99% of similarity with the species K.pneumoniae and K. oxytoca. The proteins released by the Klebsiella in a supplemented environment with 0.03% of Opera had been precipitated with acetone, obtaining two proteinic fractions, a soluble (FS) and the other insoluble (FI) in a 0,1 mol L-1 phosphate buffer, pH 6.0. In the soluble solution (FS), it was found an oxirredutase from the peroxidases family, which uses hydrogen peroxide as an agent and several substrates as reducing agents, presenting greater activity for pyrogallol, TMB, o-dianisidine and catechol. In a chromatogram obtained through separation by molecular exclusion in Sephadex G- 100, two peaks with peroxidasic activities had been observed. Peak 1 presented two bands in SDS-PAGE, one with39.3 kDa and another one with 24.6 kDa. In the FI, it was possible to determine the presence of one hydrolysis with capacity to break the bonds between the ester molecule, from the family of carboxylesterases esterase B. The esterase B presented activity against casein substrates (9.3 UE), BApNA (1.31 UE), pNPP (0.01), presenting 5,4% activity of inhibition after incubation with E64, 6.5% activity of inhibition after incubation with protease inhibitors cocktail containing AEBSF and 7.5% of inhibition after incubation with TLCK. The electrophoreses of FI presented two protein bands with molecular mass of approximately 61.7 kDa for superior band and 60.7 kDa for the inferior band. The enzymatic characterization using pNPP showed high activity in pH 5.0 and pH 7.0. Esterase B kept 100% of activity after 120 minutes of incubation at 60oC. The presence of ZnCl2, EDTA, MgSO4 and CuSO4 had presented an inhibition effect of 16%, 16%, 23.2% and 40.8% respectively, within the enzyme activity. Esterase B slightly presented higher activity in the presence of DMSO and acetone, and a reduction of up to 87% comparing to isopropyl alcohol (lower polarity). The vale of Km using pNPP as substratum was of 3.4 mmol L-1, with a Vmax of 0.019 UE. When the selective J.E. supplemented with 0.03% Opera was treated with Klebsiella for 120 h, it had a reduction of 43.7% in the absorbance of the compounds with a peak of 200 nm, 55.7% - 220 nm and 28.7% - 260 nm. Using released enzymes by Klebsiella for treatment of the epoxiconazol standards in the reduction of the absorbance 200, 220 and 260 nm the observed results were 99.7%, 95.7% and 99.5% respectively. Whereas for the pyraclostrobin, the observed reduction were 95.5% and 80.2% for the wave lengths 200 and 260 nm respectively

ASSUNTO(S)

epoxiconazol peroxidase klebsiella, opera, pyraclostrobin, epoxiconazole, peroxidase, esterase b esterase b klebsiella biologia molecular opera piraclostrobin

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