Your search keyword '"Annette Plachetka"' showing total 7 results

1. 'Jump Start and Gain' Model for Dosage Compensation in Drosophila Based on Direct Sequencing of Nascent Transcripts

Author

Francesco Ferrari, Annette Plachetka, Artyom A. Alekseyenko, Youngsook L. Jung, Fatih Ozsolak, Peter V. Kharchenko, Peter J. Park, and Mitzi I. Kuroda

Subjects

Biology (General), QH301-705.5

Abstract

Dosage compensation in Drosophila is mediated by the MSL complex, which increases male X-linked gene expression approximately 2-fold. The MSL complex preferentially binds the bodies of active genes on the male X, depositing H4K16ac with a 3′ bias. Two models have been proposed for the influence of the MSL complex on transcription: one based on promoter recruitment of RNA polymerase II (Pol II), and a second featuring enhanced transcriptional elongation. Here, we utilize nascent RNA sequencing to document dosage compensation during transcriptional elongation. We also compare X and autosomes from published data on paused and elongating polymerase in order to assess the role of Pol II recruitment. Our results support a model for differentially regulated elongation, starting with release from 5′ pausing and increasing through X-linked gene bodies. Our results highlight facilitated transcriptional elongation as a key mechanism for the coordinated regulation of a diverse set of genes.

Published

2013

2. Correction: Sequence-Specific Targeting of Dosage Compensation in Favors an Active Chromatin Context.

Author

Artyom A. Alekseyenko, Joshua W. K. Ho, Shouyong Peng, Marnie Gelbart, Michael Y. Tolstorukov, Annette Plachetka, Peter V. Kharchenko, Youngsook L. Jung, Andrey A. Gorchakov, Erica Larschan, Tingting Gu, Aki Minoda, Nicole C. Riddle, Yuri B. Schwartz, Sarah C. R. Elgin, Gary H. Karpen, Vincenzo Pirrotta, Mitzi I. Kuroda, and Peter J. Park

Subjects

Genetics, QH426-470

Published

2014

3. Enrichment of HP1a on Drosophila chromosome 4 genes creates an alternate chromatin structure critical for regulation in this heterochromatic domain.

Author

Nicole C Riddle, Youngsook L Jung, Tingting Gu, Artyom A Alekseyenko, Dalal Asker, Hongxing Gui, Peter V Kharchenko, Aki Minoda, Annette Plachetka, Yuri B Schwartz, Michael Y Tolstorukov, Mitzi I Kuroda, Vincenzo Pirrotta, Gary H Karpen, Peter J Park, and Sarah C R Elgin

Subjects

Genetics, QH426-470

Abstract

Chromatin environments differ greatly within a eukaryotic genome, depending on expression state, chromosomal location, and nuclear position. In genomic regions characterized by high repeat content and high gene density, chromatin structure must silence transposable elements but permit expression of embedded genes. We have investigated one such region, chromosome 4 of Drosophila melanogaster. Using chromatin-immunoprecipitation followed by microarray (ChIP-chip) analysis, we examined enrichment patterns of 20 histone modifications and 25 chromosomal proteins in S2 and BG3 cells, as well as the changes in several marks resulting from mutations in key proteins. Active genes on chromosome 4 are distinct from those in euchromatin or pericentric heterochromatin: while there is a depletion of silencing marks at the transcription start sites (TSSs), HP1a and H3K9me3, but not H3K9me2, are enriched strongly over gene bodies. Intriguingly, genes on chromosome 4 are less frequently associated with paused polymerase. However, when the chromatin is altered by depleting HP1a or POF, the RNA pol II enrichment patterns of many chromosome 4 genes shift, showing a significant decrease over gene bodies but not at TSSs, accompanied by lower expression of those genes. Chromosome 4 genes have a low incidence of TRL/GAGA factor binding sites and a low T(m) downstream of the TSS, characteristics that could contribute to a low incidence of RNA polymerase pausing. Our data also indicate that EGG and POF jointly regulate H3K9 methylation and promote HP1a binding over gene bodies, while HP1a targeting and H3K9 methylation are maintained at the repeats by an independent mechanism. The HP1a-enriched, POF-associated chromatin structure over the gene bodies may represent one type of adaptation for genes embedded in repetitive DNA.

Published

2012

4. Sequence-specific targeting of dosage compensation in Drosophila favors an active chromatin context.

Author

Artyom A Alekseyenko, Joshua W K Ho, Shouyong Peng, Marnie Gelbart, Michael Y Tolstorukov, Annette Plachetka, Peter V Kharchenko, Youngsook L Jung, Andrey A Gorchakov, Erica Larschan, Tingting Gu, Aki Minoda, Nicole C Riddle, Yuri B Schwartz, Sarah C R Elgin, Gary H Karpen, Vincenzo Pirrotta, Mitzi I Kuroda, and Peter J Park

Subjects

Genetics, QH426-470

Abstract

The Drosophila MSL complex mediates dosage compensation by increasing transcription of the single X chromosome in males approximately two-fold. This is accomplished through recognition of the X chromosome and subsequent acetylation of histone H4K16 on X-linked genes. Initial binding to the X is thought to occur at "entry sites" that contain a consensus sequence motif ("MSL recognition element" or MRE). However, this motif is only ∼2 fold enriched on X, and only a fraction of the motifs on X are initially targeted. Here we ask whether chromatin context could distinguish between utilized and non-utilized copies of the motif, by comparing their relative enrichment for histone modifications and chromosomal proteins mapped in the modENCODE project. Through a comparative analysis of the chromatin features in male S2 cells (which contain MSL complex) and female Kc cells (which lack the complex), we find that the presence of active chromatin modifications, together with an elevated local GC content in the surrounding sequences, has strong predictive value for functional MSL entry sites, independent of MSL binding. We tested these sites for function in Kc cells by RNAi knockdown of Sxl, resulting in induction of MSL complex. We show that ectopic MSL expression in Kc cells leads to H4K16 acetylation around these sites and a relative increase in X chromosome transcription. Collectively, our results support a model in which a pre-existing active chromatin environment, coincident with H3K36me3, contributes to MSL entry site selection. The consequences of MSL targeting of the male X chromosome include increase in nucleosome lability, enrichment for H4K16 acetylation and JIL-1 kinase, and depletion of linker histone H1 on active X-linked genes. Our analysis can serve as a model for identifying chromatin and local sequence features that may contribute to selection of functional protein binding sites in the genome.

Published

2012

5. 'Jumpstart and gain' model for dosage compensation in Drosophila based on direct sequencing of nascent transcripts

Author

Peter V. Kharchenko, Youngsook L. Jung, Artyom A. Alekseyenko, Annette Plachetka, Mitzi I. Kuroda, Peter J. Park, Fatih Ozsolak, and Francesco Ferrari

Subjects

Male, X Chromosome, Transcription, Genetic, RNA polymerase II, General Biochemistry, Genetics and Molecular Biology, Article, 03 medical and health sciences, 0302 clinical medicine, Transcription (biology), MSL complex, Dosage Compensation, Genetic, Gene expression, Animals, Drosophila Proteins, lcsh:QH301-705.5, Gene, Polymerase, Cells, Cultured, 030304 developmental biology, Genetics, 0303 health sciences, Dosage compensation, biology, RNA, Nuclear Proteins, Drosophila melanogaster, lcsh:Biology (General), biology.protein, Female, 030217 neurology & neurosurgery, Transcription Factors

Abstract

Summary Dosage compensation in Drosophila is mediated by the MSL complex, which increases male X-linked gene expression approximately 2-fold. The MSL complex preferentially binds the bodies of active genes on the male X, depositing H4K16ac with a 3′ bias. Two models have been proposed for the influence of the MSL complex on transcription: one based on promoter recruitment of RNA polymerase II (Pol II), and a second featuring enhanced transcriptional elongation. Here, we utilize nascent RNA sequencing to document dosage compensation during transcriptional elongation. We also compare X and autosomes from published data on paused and elongating polymerase in order to assess the role of Pol II recruitment. Our results support a model for differentially regulated elongation, starting with release from 5′ pausing and increasing through X-linked gene bodies. Our results highlight facilitated transcriptional elongation as a key mechanism for the coordinated regulation of a diverse set of genes.

Published

2013

6. Sequence-Specific Targeting of Dosage Compensation in Drosophila Favors an Active Chromatin Context

Author

Sarah C. R. Elgin, Tingting Gu, Peter V. Kharchenko, Aki Minoda, Youngsook L. Jung, Nicole C. Riddle, Artyom A. Alekseyenko, Gary H. Karpen, Mitzi I. Kuroda, Peter J. Park, Michael Y. Tolstorukov, Erica Larschan, Andrey A. Gorchakov, Vincenzo Pirrotta, Yuri B. Schwartz, Annette Plachetka, Shouyong Peng, Joshua W. K. Ho, Marnie E. Gelbart, and Ferguson-Smith, Anne C

Subjects

Male, Cancer Research, Transcription, Genetic, Histones, 0302 clinical medicine, Genes, X-Linked, MSL complex, Drosophila Proteins, Genetics (clinical), X chromosome, Genetics, 0303 health sciences, Base Composition, Dosage compensation, biology, Biochemistry and Molecular Biology, Nuclear Proteins, RNA-Binding Proteins, Acetylation, Genomics, Protein-Serine-Threonine Kinases, Chromatin, Nucleosomes, Drosophila melanogaster, Dosage Compensation, RNA Interference, Transcription, Drosophila Protein, Research Article, X Chromosome, lcsh:QH426-470, 1.1 Normal biological development and functioning, Protein Serine-Threonine Kinases, 03 medical and health sciences, Genetic, Underpinning research, Dosage Compensation, Genetic, Nucleosome, Animals, Nucleotide Motifs, Molecular Biology, Transcription factor, Biology, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Binding Sites, Human Genome, fungi, Computational Biology, X-Linked, biology.organism_classification, lcsh:Genetics, Genes, Gene Expression Regulation, Generic health relevance, 030217 neurology & neurosurgery, Biokemi och molekylärbiologi, Developmental Biology, Transcription Factors

Abstract

The Drosophila MSL complex mediates dosage compensation by increasing transcription of the single X chromosome in males approximately two-fold. This is accomplished through recognition of the X chromosome and subsequent acetylation of histone H4K16 on X-linked genes. Initial binding to the X is thought to occur at “entry sites” that contain a consensus sequence motif (“MSL recognition element” or MRE). However, this motif is only ∼2 fold enriched on X, and only a fraction of the motifs on X are initially targeted. Here we ask whether chromatin context could distinguish between utilized and non-utilized copies of the motif, by comparing their relative enrichment for histone modifications and chromosomal proteins mapped in the modENCODE project. Through a comparative analysis of the chromatin features in male S2 cells (which contain MSL complex) and female Kc cells (which lack the complex), we find that the presence of active chromatin modifications, together with an elevated local GC content in the surrounding sequences, has strong predictive value for functional MSL entry sites, independent of MSL binding. We tested these sites for function in Kc cells by RNAi knockdown of Sxl, resulting in induction of MSL complex. We show that ectopic MSL expression in Kc cells leads to H4K16 acetylation around these sites and a relative increase in X chromosome transcription. Collectively, our results support a model in which a pre-existing active chromatin environment, coincident with H3K36me3, contributes to MSL entry site selection. The consequences of MSL targeting of the male X chromosome include increase in nucleosome lability, enrichment for H4K16 acetylation and JIL-1 kinase, and depletion of linker histone H1 on active X-linked genes. Our analysis can serve as a model for identifying chromatin and local sequence features that may contribute to selection of functional protein binding sites in the genome., Author Summary The genomes of complex organisms encompass hundreds of millions of base pairs of DNA, and regulatory molecules must distinguish specific targets within this vast landscape. In general, regulatory factors find target genes through sequence-specific interactions with the underlying DNA. However, sequence-specific factors typically bind only a fraction of the candidate genomic regions containing their specific target sequence motif. Here we identify potential roles for chromatin environment and flanking sequence composition in helping regulatory factors find their appropriate binding sites, using targeting of the Drosophila dosage compensation complex as a model. The initial stage of dosage compensation involves binding of the Male Specific Lethal (MSL) complex to a sequence motif called the MSL recognition element [1]. Using data from a large chromatin mapping effort (the modENCODE project), we successfully identify an active chromatin environment as predictive of selective MRE binding by the MSL complex. Our study provides a framework for using genome-wide datasets to analyze and predict functional protein–DNA binding site selection.

Published

2012

7. Enrichment of HP1a on drosophila chromosome 4 genes creates an alternate chromatin structure critical for regulation in this heterochromatic domain

Author

Youngsook L. Jung, Yuri B. Schwartz, Sarah C. R. Elgin, Annette Plachetka, Peter V. Kharchenko, Mitzi I. Kuroda, Artyom A. Alekseyenko, Dalal Asker, Peter J. Park, Tingting Gu, Nicole C. Riddle, Vincenzo Pirrotta, Michael Y. Tolstorukov, Hongxing Gui, Aki Minoda, Gary H. Karpen, and Lieb, Jason D

Subjects

melanogaster, Cancer Research, Euchromatin, Chromosomal Proteins, Non-Histone, Gene Expression, Animals, Genetically Modified, Histones, sequence count data, 0302 clinical medicine, position-effect variegation, Heterochromatin, Drosophila Proteins, Genetics (clinical), chip-chip, rna-polymerase, Regulation of gene expression, Genetics, 0303 health sciences, Chromosome Biology, Drosophila Melanogaster, 4th chromosome, Biochemistry and Molecular Biology, DNA-Directed RNA Polymerases, Genomics, Animal Models, Chromatin, Chromosomal Proteins, Drosophila melanogaster, differential expression analysis, Epigenetics, Biotechnology, Research Article, TBX1, lcsh:QH426-470, 1.1 Normal biological development and functioning, Genetically Modified, Biology, Methylation, Chromosomes, 03 medical and health sciences, Model Organisms, Underpinning research, dot chromosom, Animals, Humans, Molecular Biology, Gene, Ecology, Evolution, Behavior and Systematics, ChIA-PET, 030304 developmental biology, Human Genome, Non-Histone, Histone-Lysine N-Methyltransferase, lcsh:Genetics, Chromosome 4, Gene Expression Regulation, Chromobox Protein Homolog 5, Mutation, Generic health relevance, nascent rna, Genome Expression Analysis, protein, 030217 neurology & neurosurgery, Biokemi och molekylärbiologi, Developmental Biology

Abstract

Chromatin environments differ greatly within a eukaryotic genome, depending on expression state, chromosomal location, and nuclear position. In genomic regions characterized by high repeat content and high gene density, chromatin structure must silence transposable elements but permit expression of embedded genes. We have investigated one such region, chromosome 4 of Drosophila melanogaster. Using chromatin-immunoprecipitation followed by microarray (ChIP–chip) analysis, we examined enrichment patterns of 20 histone modifications and 25 chromosomal proteins in S2 and BG3 cells, as well as the changes in several marks resulting from mutations in key proteins. Active genes on chromosome 4 are distinct from those in euchromatin or pericentric heterochromatin: while there is a depletion of silencing marks at the transcription start sites (TSSs), HP1a and H3K9me3, but not H3K9me2, are enriched strongly over gene bodies. Intriguingly, genes on chromosome 4 are less frequently associated with paused polymerase. However, when the chromatin is altered by depleting HP1a or POF, the RNA pol II enrichment patterns of many chromosome 4 genes shift, showing a significant decrease over gene bodies but not at TSSs, accompanied by lower expression of those genes. Chromosome 4 genes have a low incidence of TRL/GAGA factor binding sites and a low Tm downstream of the TSS, characteristics that could contribute to a low incidence of RNA polymerase pausing. Our data also indicate that EGG and POF jointly regulate H3K9 methylation and promote HP1a binding over gene bodies, while HP1a targeting and H3K9 methylation are maintained at the repeats by an independent mechanism. The HP1a-enriched, POF-associated chromatin structure over the gene bodies may represent one type of adaptation for genes embedded in repetitive DNA., Author Summary How DNA is packaged into chromatin has profound implications for gene regulation. While certain chromatin conformations are accessible to RNA polymerase and allow expression, other chromatin structures prevent transcription. In many genomes, genes that need to be expressed and repetitive sequences that need to be silenced are interspersed at close intervals. We use Drosophila melanogaster chromosome 4 as one example of such a complex domain and ask how the genes on this chromosome are packaged and regulated. While the transcription start sites of active genes on chromosome 4 exhibit the expected pattern of chromatin marks, we see an unusual combination of marks over expressed gene bodies, including enrichment of HP1a and H3K9me3. Deposition of HP1a over the gene bodies is dependent on POF (painting of fourth), while its association with intergenic repeat clusters is accomplished by a different mechanism. In this environment, promoter proximal RNA polymerase pausing is largely absent, despite the fact that genome-wide, approximately 10%–15% of all active genes display pausing. A redistribution of polymerase on chromosome 4 genes, including depletion in the gene body, is observed on HP1a depletion. These findings demonstrate how gene regulation mechanisms can be modulated in specific domains of the genome and illustrate the necessity of examining regulatory pathways within chromatin sub-domains, rather than relying on genome-wide averages or on a limited set of reporter genes.

Published

2012