Your search keyword '"Bourett TM"' showing total 11 results

1. Cryo-Fixation and Gene Product Localization in Fungi

Author

Bourett, TM, Duncan, KE, Czymmek, KJ, Sweigard, JA, Dezwaan, TM, and Howard, RJ

Abstract

There are many strategies for documenting the distribution of gene products or other molecules within cells or tissues. Depending on the required information, techniques can range from cell fractionation to methods that employ electron microscopy: some preclude examination of living cells, and thus can not provide dynamic temporal information. Time sequence data are paramount when gene expression is transient, as is often the case during fungal-pathogen plant-host interactions. Fluorescent dyes and protein tags (e.g., green fluorescent protein, GFP) allow monitoring of specific molecules, organelles or cells over time, for simultaneous recording of both spatial and temporal information. in addition, fluorescent markers are amenable to powerful 3-D analysis using confocal or multi-photon imaging methods. We have achieved good expression of fluorescent proteins in the fungal blast pathogen Magnaporthe grisea, and have generated a functional fusion protein between GFP and P-tubulin (Figs. 1,2).

Published

2001

2. Light and Electron Microscope Immunocytochemistry in Freeze-Substituted Plant and Fungal Cells

Author

Czymmek, KJ, Bourett, TM, and Howard, RJ

Abstract

In efforts to better understand the cell biology of fungi and their pathogenic interactions with plants, we have pursued the use of cryo-preparative techniques for specimen preservation and immunocytochemistry at the light and electron microscope level. The chemically diverse composition of plant and fungal walls has proven very challenging for immunofluorescence using confocal microscopy. Typically, to allow probe access in these organisms, immunolabeling has required sectioning or enzymatic digestion of cell walls. The ideal method would preserve the spatial fidelity and antigenicity of the target molecule as well as maintain the integrity of the surrounding tissue. Our early work using methacrylate de-embedment, as described for sectioned plant material, was very effective for freeze-substituted fungi. Further improvements, using a combination of slow freezing and freeze-substitution followed by methacrylate de-embedment, permitted whole mount fluorescence antibody labeling of a variety of phylogenetically diverse fungi without enzymatic digestion or sectioning (Fig.l).

Published

2001

3. A vegetative storage protein improves drought tolerance in maize.

Author

Abbaraju HKR, Gupta R, Appenzeller LM, Fallis LP, Hazebroek J, Zhu G, Bourett TM, Howard RJ, Weers B, Lafitte RH, Hakimi SM, Schussler JR, Loussaert DF, Habben JE, and Dhugga KS

Subjects

Chloroplasts, Edible Grain genetics, Nitrogen metabolism, Plant Proteins genetics, Plant Proteins metabolism, Plants, Genetically Modified genetics, Droughts, Zea mays genetics

Abstract

Vegetative storage proteins (VSPs) are known to serve as nitrogen reserves in many dicot plants but remain undiscovered in grasses, most widely grown group of crops globally. We identified and characterized a VSP in maize and demonstrated that its overexpression improved drought tolerance. Nitrogen supplementation selectively induced a mesophyll lipoxygenase (ZmLOX6), which was targeted to chloroplasts by a novel N-terminal transit peptide of 62 amino acids. When ectopically expressed under the control of various tissue-specific promoters, it accumulated to a fivefold higher level upon expression in the mesophyll cells than the wild-type plants. Constitutive expression or targeted expression specifically to the bundle sheath cells increased its accumulation by less than twofold. The overexpressed ZmLOX6 was remobilized from the leaves like other major proteins during grain development. Evaluated in the field over locations and years, transgenic hybrids overexpressing ZmLOX6 in the mesophyll cells significantly outyielded nontransgenic sibs under managed drought stress imposed at flowering. Additional storage of nitrogen as a VSP in maize leaves ameliorated the effect of drought on grain yield., (© 2021 Pioneer Hi-Bred International, Inc (Corteva Agriscience). Plant Biotechnology Journal published by Society for Experimental Biology and The Association of Applied Biologists and John Wiley & Sons Ltd.)

Published

2022

4. Backscattered electron SEM imaging of resin sections from plant specimens: observation of histological to subcellular structure and CLEM.

Author

Rizzo NW, Duncan KE, Bourett TM, and Howard RJ

Subjects

Intracellular Space, Light, Microscopy, Electron, Transmission, Microtomy, Electrons, Microscopy, Electron, Scanning, Plant Cells ultrastructure, Resins, Synthetic

Abstract

We have refined methods for biological specimen preparation and low-voltage backscattered electron imaging in the scanning electron microscope that allow for observation at continuous magnifications of ca. 130-70 000 X, and documentation of tissue and subcellular ultrastructure detail. The technique, based upon early work by Ogura & Hasegawa (1980), affords use of significantly larger sections from fixed and resin-embedded specimens than is possible with transmission electron microscopy while providing similar data. After microtomy, the sections, typically ca. 750 nm thick, were dried onto the surface of glass or silicon wafer and stained with heavy metals-the use of grids avoided. The glass/wafer support was then mounted onto standard scanning electron microscopy sample stubs, carbon-coated and imaged directly at an accelerating voltage of 5 kV, using either a yttrium aluminum garnet or ExB backscattered electron detector. Alternatively, the sections could be viewed first by light microscopy, for example to document signal from a fluorescent protein, and then by scanning electron microscopy to provide correlative light/electron microscope (CLEM) data. These methods provide unobstructed access to ultrastructure in the spatial context of a section ca. 7 × 10 mm in size, significantly larger than the typical 0.2 × 0.3 mm section used for conventional transmission electron microscopy imaging. Application of this approach was especially useful when the biology of interest was rare or difficult to find, e.g. a particular cell type, developmental stage, large organ, the interface between cells of interacting organisms, when contextual information within a large tissue was obligatory, or combinations of these factors. In addition, the methods were easily adapted for immunolocalizations., (© 2015 The Author. Journal of Microscopy published by John Wiley & Sons, Ltd on behalf of the Royal Microscopical Society.)

Published

2016

5. A pair of homoeolog ClpP5 genes underlies a virescent yellow-like mutant and its modifier in maize.

Author

Xing A, Williams ME, Bourett TM, Hu W, Hou Z, Meeley RB, Jaqueth J, Dam T, and Li B

Subjects

Chloroplasts enzymology, Endopeptidase Clp genetics, Endopeptidase Clp metabolism, Gene Expression Regulation, Plant, Genes, Duplicate physiology, Plant Leaves genetics, Zea mays genetics, Genes, Duplicate genetics, Plant Leaves metabolism, Zea mays metabolism

Abstract

Gene-background interaction is a commonly observed phenomenon in many species, but the molecular mechanisms of such an interaction is less well understood. Here we report the cloning of a maize mutant gene and its modifier. A recessive mutant with a virescent yellow-like (vyl) phenotype was identified in an ethyl methanesulfonate-mutagenized population derived from the maize inbred line B73. Homozygous mutant maize plants exhibited a yellow leaf phenotype after emergence but gradually recovered and became indistinguishable from wild-type plants after approximately 2 weeks. Taking the positional cloning approach, the Chr.9_ClpP5 gene, one of the proteolytic subunits of the chloroplast Clp protease complex, was identified and validated as the candidate gene for vyl. When introgressed by backcross into the maize inbred line PH09B, the mutant phenotype of vyl lasted much longer in the greenhouse and was lethal in the field, implying the presence of a modifier(s) for vyl. A major modifier locus was identified on chromosome 1, and a paralogous ClpP5 gene was isolated and confirmed as the candidate for the vyl-modifier. Expression of Chr.1_ClpP5 is induced significantly in B73 by the vyl mutation, while the expression of Chr.1_ClpP5 in PH09B is not responsive to the vyl mutation. Moreover, expression and sequence analysis suggests that the PH09B Chr.1_ClpP5 allele is functionally weaker than the B73 allele. We propose that functional redundancy between duplicated paralogous genes is the molecular mechanism for the interaction between vyl and its modifier., (© 2014 The Authors The Plant Journal © 2014 John Wiley & Sons Ltd.)

Published

2014

6. Brittle stalk 2 encodes a putative glycosylphosphatidylinositol-anchored protein that affects mechanical strength of maize tissues by altering the composition and structure of secondary cell walls.

Author

Ching A, Dhugga KS, Appenzeller L, Meeley R, Bourett TM, Howard RJ, and Rafalski A

Subjects

Biomechanical Phenomena, Cell Wall physiology, DNA Transposable Elements, Exons, Gene Expression, Genes, Plant, Glycosylphosphatidylinositols metabolism, Mutation, Plant Proteins genetics, Plant Proteins metabolism, Zea mays genetics, Zea mays metabolism, Cell Wall metabolism, Plant Proteins physiology, Zea mays physiology

Abstract

A spontaneous maize mutant, brittle stalk-2 (bk2-ref), exhibits dramatically reduced tissue mechanical strength. Reduction in mechanical strength in the stalk tissue was highly correlated with a reduction in the amount of cellulose and an uneven deposition of secondary cell wall material in the subepidermal and perivascular sclerenchyma fibers. Cell wall accounted for two-thirds of the observed reduction in dry matter content per unit length of the mutant stalk in comparison to the wildtype stalk. Although the cell wall composition was significantly altered in the mutant in comparison to the wildtype stalks, no compensation by lignin and cell wall matrix for reduced cellulose amount was observed. We demonstrate that Bk2 encodes a Cobra-like protein that is homologous to the rice Bc1 protein. In the bk2-ref gene, a 1 kb transposon-like element is inserted in the beginning of the second exon, disrupting the open reading frame. The Bk2 gene was expressed in the stalk, husk, root, and leaf tissues, but not in the embryo, endosperm, pollen, silk, or other tissues with comparatively few or no secondary cell wall containing cells. The highest expression was in the isolated vascular bundles. In agreement with its role in secondary wall formation, the expression pattern of the Bk2 gene was very similar to that of the ZmCesA10, ZmCesA11, and ZmCesA12 genes, which are known to be involved in secondary wall formation. We have isolated an independent Mutator-tagged allele of bk2, referred to as bk2-Mu7, the phenotype of which is similar to that of the spontaneous mutant. Our results demonstrate that mutations in the Bk2 gene affect stalk strength in maize by interfering with the deposition of cellulose in the secondary cell wall in fiber cells.

Published

2006

7. Live-cell imaging of tubulin in the filamentous fungus Magnaporthe grisea treated with anti-microtubule and anti-microfilament agents.

Author

Czymmek KJ, Bourett TM, Shao Y, DeZwaan TM, Sweigard JA, and Howard RJ

Subjects

Actin Cytoskeleton drug effects, Actin Cytoskeleton ultrastructure, Antifungal Agents pharmacology, Bacterial Proteins genetics, Bacterial Proteins metabolism, Benomyl pharmacology, Bridged Bicyclo Compounds, Heterocyclic pharmacology, Fungicides, Industrial pharmacology, Griseofulvin pharmacology, Luminescent Proteins genetics, Luminescent Proteins metabolism, Magnaporthe genetics, Magnaporthe ultrastructure, Microscopy, Electron, Microtubules drug effects, Microtubules ultrastructure, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Thiazoles pharmacology, Thiazolidines, Transformation, Genetic, Tubulin genetics, Magnaporthe drug effects, Magnaporthe metabolism, Tubulin metabolism

Abstract

Microtubule dynamics were examined in live cells of the fungal plant pathogen Magnaporthe grisea transformed for constitutive expression of a fusion protein containing enhanced yellow-fluorescent protein and a Neurospora crassa benomyl-resistant allele of beta-tubulin. Transformants retained their ability to differentiate appressoria and cause disease but remained sensitive to benomyl. Linear microtubule arrays and low-level cytoplasmic fluorescence were observed in vegetative hyphae, conidia, germ tubes, and developing appressoria. Fluorescence within nuclei was conspicuously absent during interphase but increased rapidly at the onset of mitosis. Treatment with either benomyl or griseofulvin resulted in the appearance of prominent brightly fluorescent aggregates, including a large aggregate near the apex, with the concomitant disappearance of most cytoplasmic microtubules. Electron microscope imaging of treated cells indicated that the aggregates lacked any obvious profiles of intact microtubules. During these treatments, hyphal tip cells continued to elongate in a nonlinear and aerial fashion at a much slower rate than untreated cells. With subsequent removal of griseofulvin, distal aggregates disappeared rapidly but the apical aggregates persisted longer. Treatment with latrunculin A caused hyphal tip swelling without apparent effect on linear microtubule arrays. Simultaneous treatment with griseofulvin and latrunculin A resulted in depolymerization of microtubules and a cessation of growth, but near-apical fluorescent aggregates were not observed.

Published

2005

8. Reef coral fluorescent proteins for visualizing fungal pathogens.

Author

Bourett TM, Sweigard JA, Czymmek KJ, Carroll A, and Howard RJ

Subjects

Animals, Fusarium genetics, Fusarium metabolism, Hordeum microbiology, Luminescent Proteins genetics, Magnaporthe genetics, Magnaporthe metabolism, Microscopy methods, Microscopy, Confocal, Photons, Plant Diseases microbiology, Transformation, Genetic, Anthozoa metabolism, Fusarium pathogenicity, Fusarium ultrastructure, Luminescent Proteins metabolism, Magnaporthe pathogenicity, Magnaporthe ultrastructure

Abstract

The fluorescent proteins AmCyan, ZsGreen, ZsYellow, and AsRed, modified versions of proteins identified recently from several Anthozoa species of reef corals, were expressed for the first time in a heterologous system and used for imaging two different fungal plant pathogens. When driven by strong constitutive fungal promotors, expression of these reef coral fluorescent proteins yielded bright cytoplasmic fluorescence in Fusarium verticillioides and Magnaporthe grisea, and had no detectable effect on either growth rate or the ability to cause disease. Differential intracellular localization of the fluorescent proteins resulted in the discrimination of many subcellular organelles by confocal and multi-photon microscopy, and facilitated monitoring of such details as organelle dynamics and changes in the permeability of the nuclear envelope. AmCyan and ZsGreen were sufficiently excited at 855 and 880 nm, respectively, to allow for time-resolved in planta imaging by two-photon microscopy., (Copyright 2002 Elsevier Science (USA))

Published

2002

9. Utility of cytoplasmic fluorescent proteins for live-cell imaging of Magnaporthe grisea in planta.

Author

Czymmek KJ, Bourett TM, Sweigard JA, Carroll A, and Howard RJ

Abstract

The subcellular expression patterns and fluorescence intensities of cytoplasm-targeted, constitutively expressed blue-, cyano-, green-, yellow- and red-fluorescent protein were assessed in a number of transformants of the blast pathogen, Magnaporthe grisea. All transformants grew normally, remained pathogenic on barley, and, except for those expressing blue fluorescent protein, exhibited significant cytoplasmic fluorescence. The exceptionally intense brightness of some strains proved very useful for laser scanning confocal microscope imaging during invasion of host tissues. Acquisition of three-dimensional data sets from intact, individual, pathogen encounter sites in planta were generated during the time course of pathogenesis using non-invasive optical sectioning methods. Confocal and multiphoton microscopy imaging in conjunction with fluorescent protein expression allowed for the real time documentation of fungal colonization within plant cells and tissues with remarkable ease. These methods constitute valuable new tools for the investigation of plant disease.

Published

2002

10. An improved method for affinity probe localization in whole cells of filamentous fungi.

Author

Bourett TM, Czymmek KJ, and Howard RJ

Subjects

Affinity Labels, Cytoskeleton ultrastructure, Fluorescent Antibody Technique, Freezing, Immunoglobulin M, Lectins, Methacrylates, Microscopy, Confocal, Microtubules ultrastructure, Organelles ultrastructure, Fungi ultrastructure, Tissue Embedding methods, Tissue Fixation methods

Abstract

The fungal cell wall, though phylogenetically variable, acts universally as a potent barrier to probing intracellular structures. Thus, the use of high-molecular-weight probes such as antibodies and lectins has proven a formidable challenge. We have devised a preparative method for use with various affinity probes that can be applied to a broad spectrum of filamentous fungal species and used for imaging whole cells. In this study, confocal imaging of whole-mount fungal hyphae after freeze substitution, methacrylate embedment/de-embedment, and infiltration with affinity probes has yielded remarkably improved renderings of the three-dimensional distribution of both microtubules (using antibodies against both alpha- and beta-tubulin) and concanavalin A binding sites. Using this protocol we have been able to document: (1) the three-dimensional distribution of microtubules in all regions of hyphae, (2) the presence of apparent foci for cytoplasmic microtubules, (3) persistent cytoplasmic microtubules during mitosis, and (4) a three-dimensional view of many compartments of the endomembrane system including Golgi-equivalent organelles and apical vesicles. The last result represents the first direct confirmation of apical vesicles comprising the Spitzenkörper., (Copyright 1998 Academic Press.)

Published

1998

11. Control of leaf and chloroplast development by the Arabidopsis gene pale cress.

Author

Reiter RS, Coomber SA, Bourett TM, Bartley GE, and Scolnik PA

Subjects

Amino Acid Sequence, Arabidopsis growth & development, Base Sequence, Chloroplasts ultrastructure, Chromosome Mapping, Cloning, Molecular, Meristem genetics, Meristem growth & development, Meristem ultrastructure, Microscopy, Electron, Molecular Sequence Data, Arabidopsis genetics, Chloroplasts genetics, Gene Expression Regulation, Plant genetics, Genes, Plant genetics, Plant Leaves growth & development

Abstract

Leaf plastids of the Arabidopsis pale cress (pac) mutant do not develop beyond the initial stages of differentiation from proplastids or etioplasts and contain only low levels of chlorophylls and carotenoids. Early in development, the epidermis and mesophyll of pac leaves resemble those of wild-type plants. In later stages, mutant leaves have enlarged intercellular spaces, and the palisade layer of the mesophyll can no longer be distinguished. To study the molecular basis of this phenotype, we cloned PAC and determined that this gene is regulated by light and has the capacity to encode an acidic, predominantly alpha-helical protein. The PAC gene appears to be a novel component of a light-induced regulatory network that controls the development of leaves and chloroplasts.

Published

1994