Your search keyword '"Beneš, Helen"' showing total 4 results

1. Sex-, stage- and tissue-specific regulation by a mosquito hexamerin promoter.

Author

Jinwal, U. K., Zakharkin, S. O., Litvinova, O. V., Jain, S., and Beneš, Helen

Subjects

DROSOPHILA, GENETIC regulation, FRUIT flies, TRANSCRIPTION factors, DROSOPHILA melanogaster, DNA, GENES

Abstract

A portion of the 5′-flanking region of the female-specific hexamerin gene, Hex-1.2, from the mosquito Ochlerotatus atropalpus was used to drive expression of the luciferase reporter gene in Drosophila melanogaster. The proximal 0.7 kb of 5′-flanking DNA were sufficient to partially repress reporter gene activity in males and to drive tissue- and stage-specific expression comparable with that of the endogenous O. atropalpus Hex-1.2 gene. The Drosophila doublesex transcription factor (DSX), expressed in Escherichia coli, bound putative DSX sites of the Hex-1.2 gene differentially in vitro. Blocking expression of the female isoform of the Doublesex transcription factor in transgenic female flies resulted in reduction of luciferase expression to levels comparable with those in males, suggesting that Doublesex could contribute to regulation of female-specific expression of the O. atropalpus Hex-1.2 gene. [ABSTRACT FROM AUTHOR]

Published

2006

2. Increased glutathione S-transferase activity rescues dopaminergic neuron loss in a Drosophila model of Parkinson's disease.

Author

Whitworth, Alexander J., Theodore, Dorothy A., Greene, Jessica C., Beneš, Helen, Wes, Paul D., and Pallanck, Leo J.

Subjects

PARKINSON'S disease, GENETIC mutation, DROSOPHILA, NEURONS, PHENOTYPES, BRAIN diseases

Abstract

Loss-of-function mutations of the parkin gene are a major cause of early-onset parkinsonism. To explore the mechanism by which loss of parkin function results in neurodegeneration, we are using a genetic approach in Drosophila. Here, we show that Drosophila parkin mutants display degeneration of a subset of dopaminergic (DA) neurons in the brain. The neurodegenerative phenotype of parkin mutants is enhanced by loss-of-function mutations of the glutathione S-transferase S1 (GstS1) gene, which were identified in an unbiased genetic screen for genes that modify parkin phenotypes. Furthermore, overexpression of GstSl in DA neurons suppresses neurodegeneration in parkin mutants. Given the previous evidence for altered glutathione metabolism and oxidative stress in sporadic Parkinson's disease (PD), these data suggest that the mechanism of DA neuron loss in Drosophila parkin mutants is similar to the mechanisms underlying sporadic PD. Moreover, these findings identify a potential therapeutic approach in treating PD. [ABSTRACT FROM AUTHOR]

Published

2005

3. Catalytic function of Drosophila melanogaster glutathione S-transferase DmGSTS1-1 (GST-2) in conjugation of lipid peroxidation end products.

Author

Singh, Sharda P., Coronella, Julia A., Beneš, Helen, Cochrane, Bruce J., and Zimniak, Piotr

Subjects

GLUTATHIONE transferase, DROSOPHILA melanogaster, LIPIDS, BIOCONJUGATES, BIOCHEMICAL mechanism of action, PEROXIDATION, PHYSIOLOGY

Abstract

Drosophila melanogaster glutathione S-transferase DmGSTS1-1 (earlier designated as GST-2) is related to sigma class GSTs and was previously described as an indirect flight muscle-associated protein with no known catalytic properties. We now report that DmGSTS1-1 isolated from Drosophila or expressed in Escherichia coli is essentially inactive toward the commonly used synthetic substrate 1-chloro-2,4-dinitrobenzene (CDNB), but has relatively high glutathione-conjugating activity for 4-hydroxynonenal (4-HNE), an electrophilic aldehyde derived from lipid peroxidation. 4-HNE is thought to have signaling functions and, at higher concentrations, has been shown to be cytotoxic and involved in the etiology of various degenerative diseases. Drosophila strains carrying P-element insertions in the GstS1 gene have a reduced capacity for glutathione conjugation of 4-HNE. In flies with both, one, or none of the GstS1 alleles disrupted by P-element insertion, there is a linear correlation between DmGSTS1-1 protein content and 4-HNE-conjugating activity. This correlation indicates that in adult Drosophila 70 ± 6% of the capacity to conjugate 4-HNE is attributable to DmGSTS1-1. The high abundance of DmGSTS1-1 (approximately 2% of the soluble protein in adult flies) and its previously reported localization in tissues that are either highly aerobic (indirect flight muscle) or especially sensitive to oxidative damage (neuronal tissue) suggest that the enzyme may have a protective role against deleterious effects of oxidative stress. Such function in insects would be analogous to that carried out in mammals by specialized alpha class glutathione S-transferases (e.g. GSTA4-4). The independent emergence of 4-HNE-conjugating activity in more than one branch of the glutathione S-transferase superfamily suggests that 4-HNE catabolism may be essential for aerobic life. [ABSTRACT FROM AUTHOR]

Published

2001

4. The <em>Drosophila</em> Lsp-1β gene.

Author

Massey Jr., Holman C., Kejzlarová-Lepesant, Jana, Willis, Rebecca L., Castleberry, Alecia B., and Beneš, Helen

Subjects

GENES, MOLECULAR evolution, DROSOPHILA, FRUIT flies, DIPTERA, INSECT larvae, BLOOD proteins, PROTEINS

Abstract

In Drosophila melanogaster, metamorphosis and reproduction are thought to be supported in large by two immunologically distinct hexameric storage proteins (hexamerins), larval serum protein 1 (LSP-1), a mixed hexamer of three closely related subunits, Lsp-l(alpha;, β and γ) and larval serum protein 2 (LSP-2), a homohexamer of Lsp-2 subunits. To understand the structural and functional differences between these two storage hexamers, the nucleotide sequence of the coding region of the Lsp-1β gene was determined for comparison with LSP-2 and a number of other arthropod hexamerins. The G+C content of the coding sequence is 55 %, with 92.8 % of the codons containing G or C in the third position. Conceptual translation of the Lsp-1β open reading frame revealed a 789-amino-acid polypeptide of 94465 Da. The amino acid sequence of Lsp-1β is 65.8 % identical to that of calliphorin, the major hexamerin of the blowfly, Calli phora vicina, and only 35.2% identical to Drosophila Lsp-2. This greater similarity to calliphorin is also reflected in high aromatic amino acid and methionine contents, in contrast to LSP-2 which is enriched to a lesser extent only in aromatic amino acids. Lsp-1β is also more closely related to calliphorin with respect to the protein domain structure, the presence of a single intron in its gene, and the absence of glycosylation sites. However, phylogenetic analysis based on multiple alignments revealed that LSP-1/calliphorin and LSP-2 form a distinct dipteran clade whose members are more similar to each other than to any previously sequenced lepidopteran hexamerin or arthropod hemocyanin. [ABSTRACT FROM AUTHOR]

Published

1997