230 research outputs found
Introduction â RicĆur and the Problem of Space. Perspectives on a RicĆurian âSpatial Turnâ
Introduction to special issue "Ricoeur and the Problem of Space"English introduction to the special issue "RicĆur and the Problem of Space
RNomics: a computational search for box C/D snoRNA genes in the D. melanogaster genome.
Motivation: In eukaryotes, the family of non-coding RNA
genes includes a number of genes encoding small nucleolar
RNAs (mainly C/D and H/ACA snoRNAs), which act as
guides in the maturation or post-transcriptional modifications
of target RNA molecules. Since in Drosophila melanogaster
(Dm) only few examples of snoRNAs have been identified so
far by cDNA libraries screening, integration of the molecular
data with in silico identification of these types of genes could
throw light on their organization in the Dm genome.
Results: We have performed a computational screening of
the Dm genome for C/D snoRNA genes, followed by experimental validation of the putative candidates. Few of the
26 confirmed snoRNAs had been recognized by cDNA library
analysis. Organization of the Dm genome was also
found to be more variegated than previously suspected, with
snoRNA genes nested in both the introns and exons of
protein-coding genes. This finding suggests that the presence
of additional mechanisms of snoRNA biogenesis based
on the alternative production of overlapping mRNA/snoRNA
molecules.
Availability: Additional information is available at http://www.
bioinformatica.unito.it/bioinformatics/snoRNA
Linking pseudouridine synthases to growth, developmentand cell competition
Eukaryotic pseudouridine synthases direct RNA pseudouridylation and bind HâACA small nucleolar RNA (snoRNAs), which, in turn, may act as precursors of microRNA-like molecules. In humans, loss of pseudouridine
synthase activity causes dyskeratosis congenita (DC), a complex systemic disorder characterized by cancer susceptibility, failures in ribosome biogenesis
and telomere stability, and defects in stem cell formation. Considering the significant interest in deciphering the various molecular consequences of pseudouridine synthase failure, we performed a loss of function analysis of minifly (mfl), the pseudouridine synthase gene of Drosophila, in the wing
disc, an advantageous model system for studies of cell growth and differentiation.
In this organ, depletion of the mfl-encoded pseudouridine synthase causes a severe reduction in size by decreasing both the number and the size of wing cells. Reduction of cell number was mainly attributable to cell death rather than reduced proliferation, establishing that apoptosis plays a
key role in the development of the loss of function mutant phenotype.
Depletion of Mfl also causes a proliferative disadvantage in mosaic tissues that leads to the elimination of mutant cells by cell competition. Intriguingly, mfl silencing also triggered unexpected effects on wing patterning and cell differentiation, including deviations from normal lineage
boundaries, mingling of cells of different compartments, and defects in the formation of the wing margin that closely mimic the phenotype of reduced Notch activity. These results suggest that a component of the pseudouridine
synthase loss of function phenotype is caused by defects in Notch signalling
In vitro and ex vivo substrate stiffness effects on endothelial monolayer permeability in response to TNF-[alpha]
Hypertension affects 67 million American adults and is a major risk factor for atherosclerosis. While hypertension was once thought to lead to adaptive vascular stiffening, recent studies suggest that reversible vascular stiffening precedes hypertension development. In addition, increased inflammation, such as elevated inflammatory cytokine tumor necrosis factor-α (TNF-α), is associated with hypertension. Both stiff substrates and TNF-α increase endothelial cell permeability, which contributes to atherosclerotic plaque development; however, the impact of substrate stiffness on endothelial cell permeability with TNF-α has not previously been investigated. In this project, we developed an assay to measured endothelial cell permeability with TNF-α on different stiffness polyacrylamide (PA) gels. We also created an ex vivo tissue chamber to enable en face fluorescent imaging of live mouse aortae for real time quantification of endothelial cell permeability in intact vessels exposed to flow. Our data confirms the increase in permeability with TNF-α treatment and substrate stiffness and suggests an interaction between inflammation and stiffness on endothelial cell permeability. This research enhanced our understanding of the integrated impact of substrate stiffness and inflammatory molecules on endothelial barrier loss. This can lead to a greater understanding of how hypertension contributes to atherosclerosis. By improving our knowledge of the interactions between biomechanical and biochemical stimuli, we can develop targeted hypertension therapies.M.S., Biomedical Engineering -- Drexel University, 201
The coding/non-coding overlapping architecture of the gene encoding the Drosophila pseudouridine synthase
BACKGROUND: In eukaryotic cells, each molecule of H/ACA small nucleolar RNA (snoRNA) assembles with four evolutionarily conserved core proteins to compose a specific ribonucleoprotein particle. One of the four core components has pseudouridine synthase activity and catalyzes the conversion of a selected uridine to pseudouridine. Members of the pseudouridine synthase family are highly conserved. In addition to catalyzing pseudouridylation of target RNAs, they carry out a variety of essential functions related to ribosome biogenesis and, in mammals, to telomere maintenance. To investigate further the molecular mechanisms underlying the expression of pseudouridine synthase genes, we analyzed the transcriptional activity of the Drosophila member of this family in great detail. RESULTS: The Drosophila gene for pseudouridine synthase, minifly/Nop60b (mfl), encodes two novel mRNAs ending at a downstream poly(A) site. One species is characterized only by an extended 3'-untranslated region (3'UTR), while a minor mRNA encodes a variant protein that represents the first example of an alternative subform described for any member of the family to date. The rare spliced variant is detected mainly in females and is predicted to have distinct functional properties. We also report that a cluster comprising four isoforms of a C/D box snoRNA and two highly related copies of a small ncRNA gene of unknown function is intron-encoded at the gene-variable 3'UTRs. Because this arrangement, the alternative 3' ends allow mfl not only to produce two distinct protein subforms, but also to release different ncRNAs. Intriguingly, accumulation of all these intron-encoded RNAs was found to be sex-biased and quantitatively modulated throughout development and, within the ovaries, the ncRNAs of unknown function were found not ubiquitously expressed. CONCLUSION: Our results expand the repertoire of coding/non-coding transcripts derived from the gene encoding Drosophila pseudouridine synthase. This gene exhibits a complex and interlaced organization, and its genetic information may be expressed as different protein subforms and/or ncRNAs that may potentially contribute to its biological functions
Introduction â RicĆur et la question de lâespace. Les perspectives dâun « tournant spatial » Ă partir de RicĆur
Introduction au numĂ©ro spĂ©cial " RicĆur et la question de l'espace"Introduction française au numĂ©ro spĂ©cial "RicĆur et la question de l'espace
Drosophila dyskerin is required for somatic stem cell homeostasis
Drosophila represents an excellent model to dissect the roles played by the evolutionary conserved
family of eukaryotic dyskerins. These multifunctional proteins are involved in the formation of H/
ACA snoRNP and telomerase complexes, both involved in essential cellular tasks. Since fly telomere
integrity is guaranteed by a different mechanism, we used this organism to investigate the specific
role played by dyskerin in somatic stem cell maintenance. To this aim, we focussed on Drosophila
midgut, a hierarchically organized and well characterized model for stemness analysis. Surprisingly,
the ubiquitous loss of the protein uniquely affects the formation of the larval stem cell niches, without
altering other midgut cell types. The number of adult midgut precursor stem cells is dramatically
reduced, and this effect is not caused by premature differentiation and is cell-autonomous. Moreover,
a few dispersed precursors found in the depleted midguts can maintain stem identity and the ability to
divide asymmetrically, nor show cell-growth defects or undergo apoptosis. Instead, their loss is mainly
specifically dependent on defective amplification. These studies establish a strict link between dyskerin
and somatic stem cell maintenance in a telomerase-lacking organism, indicating that loss of stemness
can be regarded as a conserved, telomerase-independent effect of dyskerin dysfunction
HSP90 and pCREB alterations are linked to mancozeb-dependent behavioral and neurodegenerative effects in a marine teleost
The pesticide mancozeb (mz) is recognized as a potent inducer of oxidative stress due to its ability to catalyze the production of reactive oxygen species plus inhibiting mitochondrial respiration thus becoming an environmental risk for neurodegenerative diseases. Despite numerous toxicological studies on mz have been directed to mammals, attention on marine fish is still lacking. Thus, it was our intention to evaluate neurobehavioral activities of ornate wrasses (Thalassoma pavo) exposed to 0.2mg/l of mz after a preliminary screening test (0.07-0.3mg/l). Treated fish exhibited an evident (p1000%) while exploratory attitudes (total arm entries) diminished (-50%; p<0.05) versus controls during spontaneous exploration tests. Moreover, they showed evident enhancements (+111%) of immobility in the cylinder test. Contextually, strong (-88%; p<0.01) reductions of permanence in light zone of the Light/Dark apparatus along with diminished crossings (-65%) were also detected. Conversely, wrasses displayed evident enhancements (160%) of risk assessment consisting of fast entries in the dark side of this apparatus. From a molecular point of view, a notable activation (p<0.005) of the brain transcription factor pCREB occurred during mz-exposure. Similarly, in situ hybridization supplied increased HSP90 mRNAs in most brain areas such as the lateral part of the dorsal telencephalon (Dl; +68%) and valvula of the cerebellum (VCe; +35%) that also revealed evident argyrophilic signals. Overall, these first indications suggest a possible protective role of the early biomarkers pCREB and HSP90 against fish toxicit
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