Your search keyword '"Mayer Kimberly M"' showing total 8 results

1. Exploring the diversity of marine-derived fungal polyketide synthases.

Author

Mayer, Kimberly M., Ford, Jermaine, Macpherson, Gordon R., Padgett, David, Volkmann-Kohlmeyer, Brigitte, Kohlmeyer, Jan, Murphy, Colleen, Douglas, Susan E., Wright, Jonathan M., and Wright, Jeffrey L. C.

Subjects

*POLYMERASE chain reaction, *POLYKETIDES, *MARINE fungi, *GENES, *DNA polymerases, *BIOINFORMATICS

Abstract

Using an approach based on polymerase chain reaction (PCR), we examined the diversity of polyketide synthase (PKS) genes present in 160 marine fungal isolates, representing 142 species. We obtained ketosynthase (KS) domain PCR products from 99 fungal isolates, representing Dothideomycetes, Sordariomycetes, Eurotiomycetes, and incertae sedis. Sequence similarity searches and phylogenetic analysis of 29 marine partial-KS-encoding sequences revealed domains predicted to encode reducing, nonreducing, and 6-methylsalicylic acid PKSs. Bioinformatic analysis of an alignment of the KS sequences from marine-derived fungi revealed no unique motifs in this region. However, several specificity-determining positions were apparent between fungal 6-methylsalicylic acid PKSs as compared with either reducing or nonreducing PKSs. Evaluation of these positions in the context of a modelled three-dimensional protein structure highlighted their potential use as PKS classification markers. Evaluating primer-binding sites was necessary to obtain KS domain fragments from putative PKSs while maintaining a level of sequence information adequate to properly classify and characterize them. [ABSTRACT FROM AUTHOR]

Published

2007

2. Identification of amino acid residues involved in substrate specificity of plant acyl-ACP thioesterases using a bioinformatics-guided approach.

Author

Mayer, Kimberly M. and Shanklin, John

Subjects

*PLANT genetics, *AMINO acids, *MUTAGENESIS, *BIOINFORMATICS, *FATTY acids, *PLANT mutation, *GENETIC mutation

Abstract

Background: The large amount of available sequence information for the plant acyl-ACP thioesterases (TEs) made it possible to use a bioinformatics-guided approach to identify amino acid residues involved in substrate specificity. The Conserved Property Difference Locator (CPDL) program allowed the identification of putative specificity-determining residues that differ between the FatA and FatB TE classes. Six of the FatA residue differences identified by CPDL were incorporated into the FatB-like parent via site-directed mutagenesis and the effect of each on TE activity was determined. Variants were expressed in E. coli strain K27 that allows determination of enzyme activity by GCMS analysis of fatty acids released into the medium. Results: Substitutions at four of the positions (74, 86, 141, and 174) changed substrate specificity to varying degrees while changes at the remaining two positions, 110 and 221, essentially inactivated the thioesterase. The effects of substitutions at positions 74, 141, and 174 (3-MUT) or 74, 86, 141, 174 (4-MUT) were not additive with respect to specificity. Conclusion: Four of six putative specificity determining positions in plant TEs, identified with the use of CPDL, were validated experimentally; a novel colorimetric screen that discriminates between active and inactive TEs is also presented. [ABSTRACT FROM AUTHOR]

Published

2007

3. A Structural Model of the Plant Acyl-Acyl Carrier Protein Thioesterase FatB Comprises Two Helix/4-Stranded Sheet Domains, the N-terminal Domain Containing Residues...

Author

Mayer, Kimberly M. and Shanklin, John

Subjects

*CARRIER proteins, *BIOLOGICAL transport, *PROTEIN binding, *FATTY acids, *CARBOXYLIC acids, *BIOSYNTHESIS

Abstract

Plant acyl-acyl carrier protein thioesterases (TEs) terminate the acyl-acyl carrier protein track of fatty acid biosynthesis and play an essential role in determining the amount and composition of fatty acids entering the storage lipid pool. A combination of bioinformatics tools was used to predict a three-dimensional model for Arabidopsis FatB (AtFatB), which comprises a fold similar to that of Escherichia coli TEII, an enzyme that is functionally similar to plant TEs but lacks significant sequence similarity and displays different inhibitor sensitivity. The catalytic residues in AtFatB, Cys-264 and His229, localize to the same region of the model as catalytic residues found in other enzymes with helix/multistranded sheet motifs (hot dog folds). Based on the model, we identified Asn-227 as a possible third member of the proposed papain-like catalytic triad. The conversion of Asn-227 to Ala resulted in a loss of detectable activity (>200-fold reduction), similar to the result seen for the equivalent mutation in papain. Mapping of plant TE specificity-affecting mutations onto the structural model showed that these mutations all cluster around the catalytic triad. Also, superposition of the crystallographically determined structures of the complexes of 4-hydroxybenzoyl-CoA TE with substrate and β-hydroxydecanoyl thiol ester dehydrase with inhibitor onto the AtFatB model showed that the substrate and inhibitor localize to the same region as the AtFatB catalytic triad in their respective structures. Together these data corroborate the structural model and show that the hot dog fold is common to enzymes from both prokaryotes and eukaryotes and that this fold supports at least three different catalytic mechanisms. [ABSTRACT FROM AUTHOR]

Published

2005

4. Linking enzyme sequence to function using conserved property difference locator to identify and annotate positions likely to control specific functionality.

Author

Mayer, Kimberly M., McCorkle, Sean R., and Shanklin, John

Subjects

*BIOINFORMATICS, *ENZYMES, *PROTEINS, *ALGORITHMS, *COMPUTERS in biology, *INFORMATION science

Abstract

Background: Families of homologous enzymes evolved from common progenitors. The availability of multiple sequences representing each activity presents an opportunity for extracting information specifying the functionality of individual homologs. We present a straightforward method for the identification of residues likely to determine class specific functionality in which multiple sequence alignments are converted to an annotated graphical form by the Conserved Property Difference Locator (CPDL) program. Results: Three test cases, each comprised of two groups of funtionally-distinct homologs, are presented. Of the test cases, one is a membrane and two are soluble enzyme families. The desaturase/hydroxylase data was used to design and test the CPDL algorithm because a comparative sequence approach had been successfully applied to manipulate the specificity of these enzymes. The other two cases, ATP/GTP cyclases, and MurD/MurE synthases were chosen because they are well characterized structurally and biochemically. For the desaturase/hydroxylase enzymes, the ATP/GTP cyclases and the MurD/MurE synthases, groups of 8 (of ~400), 4 (of ~150) and 10 (of >400) residues, respectively, of interest were identified that contain empirically defined specificity determining positions. Conclusion: CPDL consistently identifies positions near enzyme active sites that include those predicted from structural and/or biochemical studies to be important for specificity and/or function. This suggests that CPDL will have broad utility for the identification of potential class determining residues based on multiple sequence analysis of groups of homologous proteins. Because the method is sequence, rather than structure, based it is equally well suited for designing structure-function experiments to investigate membrane and soluble proteins. [ABSTRACT FROM AUTHOR]

Published

2005

5. Identification of Single Nucleotide Mutations That Prevent Developmentally Programmed DNA Elimination in Paramecium tetraurelia.

Author

Matsuda, Atsushi, Mayer, Kimberly M., and Forney, James D.

Subjects

*PARAMECIUM, *GENOMES, *NUCLEOTIDE sequence, *NUCLEOTIDE analysis, *PROTOZOA

Abstract

Describes the isolation and characterization of two additional Paramecium mutants that fail to excise an internal eliminated sequences (IES) due to a single base change. Differentiation of a new somatic macronuclear genome in ciliated protozoa; Analysis of many IES; Functional importance of nucleotides within the consensus sequence in Paramecium.

Published

2004

6. A mutation in the flanking 5'-TA-3' dinucleotide prevents excision of an internal eliminated...

Author

Mayer, Kimberly M. and Forney, James D.

Subjects

*PARAMECIUM, *MICROBIAL mutation, *MICROBIAL genetics

Abstract

Reveals that a mutation in the dinucleotide prevents excision of an internal eliminated sequence (IES) from the Paramecium tetraurelia genome. Relationship between the Paramecium IES and mariner; Mechanism of IES excision; Sequence requirements of IES excision; Inheritance of phenotypes in the F2 generation from a representative AIM-2 mutant.

Published

1999

7. A mutation in Paramecium tetraurelia reveals functional and structural features of...

Author

Mayer, Kimberly M., Mikami, Kazuyuki, and Forney, James D.

Subjects

*PARAMECIUM

Abstract

Presents a study which examines the internal eliminated sequences (IES) in Paramecium tetraurelia in relation to deoxyribonucoeic acid (DNA) sequences. Materials and methods used to conduct the study; Determination of the macronuclear and micronuclear DNA sequences for different variable surface protein genes; Results and discussion of the study.

Published

1998

8. Long-Distance Translocation of Protein during Morphogenesis of the Fruiting Body in the Filamentous Fungus, Agaricus bisporus.

Author

Woolston, Benjamin M., Schlagnhaufer, Carl, Wilkinson, Jack, Larsen, Jeffrey, Shi, Zhixin, Mayer, Kimberly M., Walters, Donald S., Curtis, Wayne R., and Romaine, C. Peter

Subjects

*BETA-glucuronidase genes, *AGARICUS, *GENETIC polymorphisms, *FILAMENTOUS fungi, *OXIDOREDUCTASES, *MORPHOGENESIS

Abstract

Commercial cultivation of the mushroom fungus, Agaricus bisporus, utilizes a substrate consisting of a lower layer of compost and upper layer of peat. Typically, the two layers are seeded with individual mycelial inoculants representing a single genotype of A. bisporus. Studies aimed at examining the potential of this fungal species as a heterologous protein expression system have revealed unexpected contributions of the mycelial inoculants in the morphogenesis of the fruiting body. These contributions were elucidated using a dual-inoculant method whereby the two layers were differientially inoculated with transgenic β-glucuronidase (GUS) and wild-type (WT) lines. Surprisingly, use of a transgenic GUS line in the lower substrate and a WT line in the upper substrate yielded fruiting bodies expressing GUS activity while lacking the GUS transgene. Results of PCR and RT-PCR analyses for the GUS transgene and RNA transcript, respectively, suggested translocation of the GUS protein from the transgenic mycelium colonizing the lower layer into the fruiting body that developed exclusively from WT mycelium colonizing the upper layer. Effective translocation of the GUS protein depended on the use of a transgenic line in the lower layer in which the GUS gene was controlled by a vegetative mycelium-active promoter (laccase 2 and β-actin), rather than a fruiting body-active promoter (hydrophobin A). GUS-expressing fruiting bodies lacking the GUS gene had a bonafide WT genotype, confirmed by the absence of stably inherited GUS and hygromycin phosphotransferase selectable marker activities in their derived basidiospores and mycelial tissue cultures. Differientially inoculating the two substrate layers with individual lines carrying the GUS gene controlled by different tissue-preferred promoters resulted in up to a ∼3.5-fold increase in GUS activity over that obtained with a single inoculant. Our findings support the existence of a previously undescribed phenomenon of long-distance protein translocation in A. bisporus that has potential application in recombinant protein expression and biotechnological approaches for crop improvement. [ABSTRACT FROM AUTHOR]

Published

2011