Your search keyword '"Joseph S Bowness"' showing total 12 results

1. Xist-mediated silencing requires additive functions of SPEN and Polycomb together with differentiation-dependent recruitment of SmcHD1

Author

Joseph S. Bowness, Tatyana B. Nesterova, Guifeng Wei, Lisa Rodermund, Mafalda Almeida, Heather Coker, Emma J. Carter, Artun Kadaster, and Neil Brockdorff

Subjects

CP: Microbiology, Biology (General), QH301-705.5

Abstract

Summary: X chromosome inactivation (XCI) is mediated by the non-coding RNA Xist, which directs chromatin modification and gene silencing in cis. The RNA binding protein SPEN and associated corepressors have a central role in Xist-mediated gene silencing. Other silencing factors, notably the Polycomb system, have been reported to function downstream of SPEN. In recent work, we found that SPEN has an additional role in correct localization of Xist RNA in cis, indicating that its contribution to chromatin-mediated gene silencing needs to be reappraised. Making use of a SPEN separation-of-function mutation, we show that SPEN and Polycomb pathways, in fact, function in parallel to establish gene silencing. We also find that differentiation-dependent recruitment of the chromosomal protein SmcHD1 is required for silencing many X-linked genes. Our results provide important insights into the mechanism of X inactivation and the coordination of chromatin-based gene regulation with cellular differentiation and development.

Published

2022

2. Systematic allelic analysis defines the interplay of key pathways in X chromosome inactivation

Author

Tatyana B. Nesterova, Guifeng Wei, Heather Coker, Greta Pintacuda, Joseph S. Bowness, Tianyi Zhang, Mafalda Almeida, Bianca Bloechl, Benoit Moindrot, Emma J. Carter, Ines Alvarez Rodrigo, Qi Pan, Ying Bi, Chun-Xiao Song, and Neil Brockdorff

Subjects

Science

Abstract

Xist RNA is the master regulator of X chromosome inactivation. Here the authors describe a systematic analysis of Xist-mediated allelic silencing in mouse ESC models and define the contribution of different pathways that regulate gene silencing.

Published

2019

3. Locus-specific expression of transposable elements in single cells with CELLO-seq

Author

Neil Brockdorff, Aaron T. L. Lun, Joseph S Bowness, John C. Marioni, Daniel J. Gaffney, Rebecca V Berrens, Guocheng Lan, Florian Bieberich, Andrian Yang, Maria Imaz, Cheuk-Ting Law, and Christopher E. Laumer

Subjects

Transposable element, 0303 health sciences, Cell, Biomedical Engineering, food and beverages, Bioengineering, Locus (genetics), Computational biology, Biology, Applied Microbiology and Biotechnology, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, Expression (architecture), Complementary DNA, medicine, Molecular Medicine, Human Induced Pluripotent Stem Cells, 030217 neurology & neurosurgery, 030304 developmental biology, Biotechnology

Abstract

Transposable elements (TEs) regulate diverse biological processes, from early development to cancer. Expression of young TEs is difficult to measure with next-generation, single-cell sequencing technologies because their highly repetitive nature means that short complementary DNA reads cannot be unambiguously mapped to a specific locus. Single CELl LOng-read RNA-sequencing (CELLO-seq) combines long-read single cell RNA-sequencing with computational analyses to measure TE expression at unique loci. We used CELLO-seq to assess the widespread expression of TEs in two-cell mouse blastomeres as well as in human induced pluripotent stem cells. Across both species, old and young TEs showed evidence of locus-specific expression with simulations demonstrating that only a small number of very young elements in the mouse could not be mapped back to the reference with high confidence. Exploring the relationship between the expression of individual elements and putative regulators revealed large heterogeneity, with TEs within a class showing different patterns of correlation and suggesting distinct regulatory mechanisms.

Published

2021

4. Progress toward understanding chromosome silencing by Xist RNA

Author

Neil Brockdorff, Joseph S Bowness, and Guifeng Wei

Subjects

Receptors, Cytoplasmic and Nuclear, Review, Biology, X-inactivation, 03 medical and health sciences, 0302 clinical medicine, X Chromosome Inactivation, Genetics, Gene silencing, Gene Silencing, Gene, 030304 developmental biology, 0303 health sciences, Proteins, RNA-Binding Proteins, Chromosome, RNA, Methyltransferases, Chromatin, Cell biology, DNA-Binding Proteins, 030220 oncology & carcinogenesis, RNA, Long Noncoding, XIST, Function (biology), Developmental Biology

Abstract

The X inactive-specific transcript (Xist) gene is the master regulator of X chromosome inactivation in mammals. Xist produces a long noncoding (lnc)RNA that accumulates over the entire length of the chromosome from which it is transcribed, recruiting factors to modify underlying chromatin and silence X-linked genes in cis. Recent years have seen significant progress in identifying important functional elements in Xist RNA, their associated RNA-binding proteins (RBPs), and the downstream pathways for chromatin modification and gene silencing. In this review, we summarize progress in understanding both how these pathways function in Xist-mediated silencing and the complex interplay between them.

Published

2020

5. Acute depletion of METTL3 implicates N6-methyladenosine in alternative intron/exon inclusion in the nascent transcriptome

Author

Mafalda Almeida, Joseph S Bowness, Jernej Ule, Greta Pintacuda, Heather Coker, Neil Brockdorff, and Guifeng Wei

Subjects

Intron, RNA, Biology, Cell biology, Transcriptome, chemistry.chemical_compound, Exon, chemistry, RNA splicing, Genetics, splice, N6-Methyladenosine, Gene, Genetics (clinical)

Abstract

RNA N6-methyladenosine (m6A) modification plays important roles in multiple aspects of RNA regulation. m6A is installed cotranscriptionally by the METTL3/14 complex, but its direct roles in RNA processing remain unclear. Here, we investigate the presence of m6A in nascent RNA of mouse embryonic stem cells. We find that around 10% of m6A peaks are located in alternative introns/exons, often close to 5′ splice sites. m6A peaks significantly overlap with RBM15 RNA binding sites and the histone modification H3K36me3. Acute depletion of METTL3 disrupts inclusion of alternative introns/exons in the nascent transcriptome, particularly at 5′ splice sites that are proximal to m6A peaks. For terminal or variable-length exons, m6A peaks are generally located on or immediately downstream from a 5′ splice site that is suppressed in the presence of m6A and upstream of a 5′ splice site that is promoted in the presence of m6A. Genes with the most immediate effects on splicing include several components of the m6A pathway, suggesting an autoregulatory function. Collectively, our findings demonstrate crosstalk between the m6A machinery and the regulation of RNA splicing.

Published

2021

6. Time-resolved structured illumination microscopy reveals key principles of Xist RNA spreading

Author

Neil Brockdorff, Lothar Schermelleh, Bramman Rajkumar, Tatyana B. Nesterova, David Miguel Susano Pinto, Joseph S Bowness, Heather Coker, Lisa Rodermund, Roel Oldenkamp, and Guifeng Wei

Subjects

RNA localization, Chemistry, Structured illumination microscopy, RNA, XIST, Dual color, Function (biology), Cell biology, Chromatin

Abstract

Xist RNA directs the process of X-chromosome inactivation in mammals by spreading in cis along the chromosome from which it is transcribed and recruiting chromatin modifiers to silence gene transcription. To elucidate mechanisms of Xist RNA cis-confinement, we established a sequential dual color labeling, super-resolution imaging approach to trace individual Xist RNA molecules over time, enabling us to define fundamental parameters of spreading. We demonstrate a feedback mechanism linking Xist RNA synthesis and degradation, and an unexpected physical coupling between preceding and newly synthesized Xist RNA molecules. Additionally, we show that the protein SPEN, a key factor for Xist-mediated gene-silencing, has a distinct function in Xist RNA localization, stability and in coupling behavior. Our results provide important insights towards understanding the unique dynamic properties of Xist RNA.One Sentence SummaryVisualizing Xist RNA dynamics in single cells during X chromosome inactivation

Published

2020

7. Locus-specific expression of transposable elements in single cells with CELLO-seq

Author

Rebecca V, Berrens, Andrian, Yang, Christopher E, Laumer, Aaron T L, Lun, Florian, Bieberich, Cheuk-Ting, Law, Guocheng, Lan, Maria, Imaz, Joseph S, Bowness, Neil, Brockdorff, Daniel J, Gaffney, and John C, Marioni

Subjects

Mice, Induced Pluripotent Stem Cells, DNA Transposable Elements, Animals, Humans, RNA

Abstract

Transposable elements (TEs) regulate diverse biological processes, from early development to cancer. Expression of young TEs is difficult to measure with next-generation, single-cell sequencing technologies because their highly repetitive nature means that short complementary DNA reads cannot be unambiguously mapped to a specific locus. Single CELl LOng-read RNA-sequencing (CELLO-seq) combines long-read single cell RNA-sequencing with computational analyses to measure TE expression at unique loci. We used CELLO-seq to assess the widespread expression of TEs in two-cell mouse blastomeres as well as in human induced pluripotent stem cells. Across both species, old and young TEs showed evidence of locus-specific expression with simulations demonstrating that only a small number of very young elements in the mouse could not be mapped back to the reference with high confidence. Exploring the relationship between the expression of individual elements and putative regulators revealed large heterogeneity, with TEs within a class showing different patterns of correlation and suggesting distinct regulatory mechanisms.

Published

2020

8. Acute depletion of METTL3 identifies a role forN6-methyladenosine in alternative intron/exon inclusion in the nascent transcriptome

Author

Neil Brockdorff, Jernej Ule, Guifeng Wei, Mafalda Almeida, Joseph S Bowness, Greta Pintacuda, and Heather Coker

Subjects

Transcriptome, chemistry.chemical_compound, Exon, chemistry, RNA splicing, Intron, RNA, Binding site, N6-Methyladenosine, Biology, Gene, Cell biology

Abstract

RNAN6-methyladenosine (m6A) modification plays important roles in multiple aspects of RNA regulation. m6A is installed co-transcriptionally by the METTL3/14 complex, but its direct roles in RNA processing remain unclear. Here we investigate the presence of m6A in nascent RNA of mouse embryonic stem cells (mESCs). We find that around 10% m6A peaks are in introns, often close to 5’-splice sites. RNA m6A peaks significantly overlap with RBM15 RNA binding sites and the histone modification H3K36me3. Interestingly, acute dTAG depletion of METTL3 reveals that inclusion of m6A-bearing alternative introns/exons in the nascent transcriptome is disrupted. For terminal or variable-length exons, m6A peaks are generally located upstream of a repressed 5’-splice site, and downstream of an enhanced 5’-splice site. Intriguingly, genes with the most immediate effects on splicing include several components of the m6A pathway, suggesting an autoregulatory function. Our findings demonstrate a direct crosstalk between m6A machinery and the regulation of RNA processing.

Published

2020

9. Acute depletion of METTL3 implicates

Author

Guifeng, Wei, Mafalda, Almeida, Greta, Pintacuda, Heather, Coker, Joseph S, Bowness, Jernej, Ule, and Neil, Brockdorff

Subjects

Alternative Splicing, Mice, RNA Splicing, Research, Animals, Exons, Methyltransferases, RNA Splice Sites, Transcriptome, Introns

Abstract

RNA N(6)-methyladenosine (m(6)A) modification plays important roles in multiple aspects of RNA regulation. m(6)A is installed cotranscriptionally by the METTL3/14 complex, but its direct roles in RNA processing remain unclear. Here, we investigate the presence of m(6)A in nascent RNA of mouse embryonic stem cells. We find that around 10% of m(6)A peaks are located in alternative introns/exons, often close to 5′ splice sites. m(6)A peaks significantly overlap with RBM15 RNA binding sites and the histone modification H3K36me3. Acute depletion of METTL3 disrupts inclusion of alternative introns/exons in the nascent transcriptome, particularly at 5′ splice sites that are proximal to m(6)A peaks. For terminal or variable-length exons, m(6)A peaks are generally located on or immediately downstream from a 5′ splice site that is suppressed in the presence of m(6)A and upstream of a 5′ splice site that is promoted in the presence of m(6)A. Genes with the most immediate effects on splicing include several components of the m(6)A pathway, suggesting an autoregulatory function. Collectively, our findings demonstrate crosstalk between the m(6)A machinery and the regulation of RNA splicing.

Published

2020

10. The many faces of Polycomb regulation by RNA

Author

Neil Brockdorff, Mafalda Almeida, and Joseph S Bowness

Subjects

X Chromosome, Polycomb-Group Proteins, Computational biology, macromolecular substances, X-inactivation, Article, 03 medical and health sciences, Genomic Imprinting, 0302 clinical medicine, X Chromosome Inactivation, Gene expression, Genetics, Animals, Humans, 030304 developmental biology, Polycomb Repressive Complex 1, 0303 health sciences, biology, Mechanism (biology), Polycomb Repressive Complex 2, RNA, Gene Expression Regulation, biology.protein, XIST, RNA, Long Noncoding, PRC1, PRC2, Genomic imprinting, 030217 neurology & neurosurgery, Developmental Biology

Abstract

Many intricate pathways contribute to the timely control of gene expression during development. Polycomb repressive complexes (PRC1 and PRC2) and long non-coding RNAs (lncRNAs) are players associated with gene repression in various developmental processes such as X chromosome inactivation (XCI) and genomic imprinting. Historically, lncRNAs were proposed to directly recruit PRC2. However, recent evidence suggests that promiscuous interactions between PRC2 and RNA fine-tune the function of the complex through a multiplicity of mechanisms. A PRC2-recruitment model was definitively overturned in the paradigm of XCI by Xist RNA, being replaced by a novel mechanism which puts PRC1 in the spotlight. This review focuses on these recent advances in understanding the interplay between RNA and Polycomb complexes for gene expression control.

Published

2020

11. Xist Repeats B and C, but not Repeat A, mediate de novo recruitment of the Polycomb system in X chromosome inactivation

Author

Joseph S Bowness, Tatyana B. Nesterova, Guifeng Wei, Mafalda Almeida, and Neil Brockdorff

Subjects

Genetics, XIST, Cell Biology, Biology, Molecular Biology, General Biochemistry, Genetics and Molecular Biology, X-inactivation, Developmental Biology

Published

2021

12. Systematic allelic analysis defines the interplay of key pathways in X chromosome inactivation

Author

Chun-Xiao Song, Neil Brockdorff, Bianca Bloechl, Benoit Moindrot, Qi Pan, Guifeng Wei, Greta Pintacuda, Ying Bi, Heather Coker, Ines Alvarez Rodrigo, Joseph S Bowness, Emma J. Carter, Tatyana B. Nesterova, Tianyi Zhang, and Mafalda Almeida

Subjects

X Chromosome, Science, Polycomb-Group Proteins, Biology, X-inactivation, Article, Cell Line, Histones, 03 medical and health sciences, Gene Knockout Techniques, Mice, 0302 clinical medicine, X Chromosome Inactivation, Gene silencing, Animals, Gene Silencing, Dosage compensation, Allele, lcsh:Science, Gene, 030304 developmental biology, Genetics, 0303 health sciences, RNA, Chromosome, RNA-Binding Proteins, Mouse Embryonic Stem Cells, Chromatin, DNA-Binding Proteins, Long non-coding RNAs, lcsh:Q, XIST, RNA, Long Noncoding, Epigenetics, 030217 neurology & neurosurgery

Abstract

Xist RNA, the master regulator of X chromosome inactivation, acts in cis to induce chromosome-wide silencing. Whilst recent studies have defined candidate silencing factors, their relative contribution to repressing different genes, and their relationship with one another is poorly understood. Here we describe a systematic analysis of Xist-mediated allelic silencing in mouse embryonic stem cell-based models. Using a machine learning approach we identify distance to the Xist locus and prior gene expression levels as key determinants of silencing efficiency. We go on to show that Spen, recruited through the Xist A-repeat, plays a central role, being critical for silencing of all except a subset of weakly expressed genes. Polycomb, recruited through the Xist B/C-repeat, also plays a key role, favouring silencing of genes with pre-existing H3K27me3 chromatin. LBR and the Rbm15/m6A-methyltransferase complex make only minor contributions to gene silencing. Together our results provide a comprehensive model for Xist-mediated chromosome silencing., Xist RNA is the master regulator of X chromosome inactivation. Here the authors describe a systematic analysis of Xist-mediated allelic silencing in mouse ESC models and define the contribution of different pathways that regulate gene silencing.

Published

2018