Your search keyword '"Kolling DJ"' showing total 5 results

1. Development of plasmid DNA reference material for the quantification of genetically modified common bean embrapa 5.1.

Author

Brod FC, Dinon AZ, Kolling DJ, Faria JC, and Arisi AC

Subjects

Brazil, Calibration, Genetic Engineering legislation & jurisprudence, Limit of Detection, Real-Time Polymerase Chain Reaction standards, DNA, Plant analysis, DNA, Plant genetics, Phaseolus genetics, Plants, Genetically Modified genetics, Plasmids genetics

Abstract

The genetically modified (GM) common bean Embrapa 5.1 was recently approved for commercialization. The reliable detection and quantification of GM organisms is strongly dependent on validated methods as well as calibration systems. This work presents the development of a calibrant plasmid for Embrapa 5.1 common bean detection. The reaction parameters were determined and compared for both the plasmid DNA (pDNA) and the genomic DNA (gDNA). PCR efficiencies for pDNA were 81% for the construction-specific assays and 76% for the taxon-specific assay, whereas for gDNA efficiencies were 94 and 93%, respectively. The limits of detection (LOD) in both qPCR assays were 10(2) and 10(3) copies of gDNA and pDNA per PCR reaction, respectively. This is sufficient to detect 0.067 and 0.67% of GM common bean in 100 ng of DNA, respectively, which is in agreement with detecting the 1% GM content required by the Brazilian legislation.

Published

2013

2. Immobilization of a recombinant esterase from Lactobacillus plantarum on polypropylene Accurel MP1000.

Author

Kolling DJ, Suguino WA, Brod FC, and Arisi AC

Subjects

Adsorption, Enzymes, Immobilized chemistry, Escherichia coli, Esterases genetics, Gene Expression, Hydrogen-Ion Concentration, Lactobacillus plantarum enzymology, Polypropylenes chemistry, Recombinant Proteins genetics, Temperature, Butyrates metabolism, Enzymes, Immobilized metabolism, Esterases metabolism, Recombinant Proteins metabolism

Abstract

A recombinant esterase from Lactobacillus plantarum was immobilized on hydrophobic support polypropylene Accurel MP1000 by adsorption. Adsorption efficiency was 83%, and the immobilized protein was 12.4 mg/g of support. Esterase activity was determined using p-nitrophenyl butyrate as substrate, and highest activities were observed at 50 °C for immobilized enzyme and 30 °C for free enzyme extract. Concerning thermal stability, after enzyme incubation at 80 °C for 30 min, immobilized and free enzyme retained 91% and 56% of initial activity, respectively. Immobilized enzyme presented lower V(max) and higher K(m) than free enzyme. Protein was not released from the support, and esterase activity increased after 3 cycles of reuse.

Published

2011

3. Biochemical and structural characterization of two site-directed mutants of Staphylococcus xylosus lipase.

Author

Kolling DJ, Bertoldo JB, Brod FC, Vernal J, Terenzi H, and Arisi AC

Subjects

Amino Acid Substitution, Bacterial Proteins biosynthesis, Bacterial Proteins genetics, Enzyme Stability, Escherichia coli, Hydrogen-Ion Concentration, Mutagenesis, Site-Directed, Mutation, Point Mutation, Protein Structure, Secondary, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Temperature, Bacterial Proteins chemistry, Lipase chemistry, Lipase genetics, Recombinant Proteins chemistry, Staphylococcus enzymology

Abstract

Staphylococcus xylosus AF208229 lipase was expressed in E. coli containing an histidine-tag (WT-Val). In the present work, in order to check the importance of the residue 309 in the specific activity, the amino acid side chain residue valine 309 was substituted by aspartate or lysine through site-directed mutagenesis. Both mutant lipases (MUT-Lys and MUT-Asp) were expressed in E. coli and the recombinant histidine-tagged lipases were purified by immobilized metal ion affinity chromatography. The enzyme activity was determined using p-nitrophenyl butyrate as substrate and secondary structure content was evaluated by circular dichroism. MUT-Lys and MUT-Asp presented significant increase of lipase activity (P < 0.05) in comparison to WT-Val, although highest activities for the three enzymes were observed at the same pH and temperature (pH 9.0 and 42 degrees C). The wild type and mutant lipases presented high thermal stability, after 30 min of incubation at 80 degrees C all enzymes retained their initial activities.

Published

2010

4. Anti-HSV-1 and anti-HIV-1 activity of gallic acid and pentyl gallate.

Author

Kratz JM, Andrighetti-Fröhner CR, Kolling DJ, Leal PC, Cirne-Santos CC, Yunes RA, Nunes RJ, Trybala E, Bergström T, Frugulhetti IC, Barardi CR, and Simões CM

Subjects

Animals, Anti-HIV Agents pharmacology, Cattle, Chlorocebus aethiops, Humans, Leukocytes, Mononuclear drug effects, Vero Cells, Virus Replication drug effects, Antiviral Agents pharmacology, Gallic Acid analogs & derivatives, Gallic Acid pharmacology, HIV-1 drug effects, Herpesvirus 1, Human drug effects

Abstract

The synthetic n-alkyl esters of gallic acid (GA), also known as gallates, especially propyl, octyl and dodecyl gallates, are widely employed as antioxidants by food and pharmaceutical industries. The inhibitory effects of GA and 15 gallates on Herpes Simplex Virus type 1 (HSV-1) and Human Immunodeficiency Virus (HIV-1) replication were investigated here. After a preliminary screening of these compounds, GA and pentyl gallate (PG) seemed to be the most active compounds against HSV-1 replication and their mode of action was characterized through a set of assays, which attempted to localize the step of the viral multiplication cycle where impairment occurred. The detected anti-HSV-1 activity was mediated by the inhibition of virus attachment to and penetration into cells, and by virucidal properties. Furthermore, an anti-HIV-1 activity was also found, to different degrees. In summary, our results suggest that both compounds could be regarded as promising candidates for the development of topical anti-HSV-1 agents, and further studies concerning the anti-HIV-1 activity of this group of molecules are merited.

Published

2008

5. Atomic resolution structures of rieske iron-sulfur protein: role of hydrogen bonds in tuning the redox potential of iron-sulfur clusters.

Author

Kolling DJ, Brunzelle JS, Lhee S, Crofts AR, and Nair SK

Subjects

Amino Acid Substitution, Bacterial Proteins genetics, Crystallography, X-Ray, Electron Transport Complex III genetics, Hydrogen Bonding, Iron-Sulfur Proteins genetics, Mutation, Oxidation-Reduction, Protein Conformation, Serine chemistry, Serine genetics, Structure-Activity Relationship, Tyrosine chemistry, Tyrosine genetics, Bacterial Proteins chemistry, Electron Transport Complex III chemistry, Iron-Sulfur Proteins chemistry, Rhodobacter sphaeroides metabolism

Abstract

The Rieske [2Fe-2S] iron-sulfur protein of cytochrome bc(1) functions as the initial electron acceptor in the rate-limiting step of the catalytic reaction. Prior studies have established roles for a number of conserved residues that hydrogen bond to ligands of the [2Fe-2S] cluster. We have constructed site-specific variants at two of these residues, measured their thermodynamic and functional properties, and determined atomic resolution X-ray crystal structures for the native protein at 1.2 A resolution and for five variants (Ser-154-->Ala, Ser-154-->Thr, Ser-154-->Cys, Tyr-156-->Phe, and Tyr-156-->Trp) to resolutions between 1.5 A and 1.1 A. These structures and complementary biophysical data provide a molecular framework for understanding the role hydrogen bonds to the cluster play in tuning thermodynamic properties, and hence the rate of this bioenergetic reaction. These studies provide a detailed structure-function dissection of the role of hydrogen bonds in tuning the redox potentials of [2Fe-2S] clusters.

Published

2007