Your search keyword '"Kumar, Swathi Ashok"' showing total 6 results

1. Genome-wide ChIP-Seq reveals a dramatic shift in the binding of the transcription factor erythroid Kruppel-like factor during erythrocyte differentiation

Author

Pilon, Andre M., Ajay, Subramanian S., Kumar, Swathi Ashok, Steiner, Laurie A., Cherukuri, Praveen F., Wincovitch, Stephen, Anderson, Stacie M., Mullikin, James C., Gallagher, Patrick G., Hardison, Ross C., Margulies, Elliott H., and Bodine, David M.

Published

2011

2. Erythroid GATA1 function revealed by genome-wide analysis of transcription factor occupancy, histone modifications, and mRNA expression

Author

Yong Cheng, Weisheng Wu, Kumar, Swathi Ashok, Duonan Yu, Deng, Wulan, Tripic, Tamara, King, David C., Kuan-Bei Chen, Ying Zhang, Drautz, Daniela, Giardine, Belinda, Schuster, Stephan C., Miller,Webb, Chiaromonte, Francesca, Yu Zhang, Blobel, Gerd A., Weiss, Mitchell J., and Hardison, Ross C.

Subjects

Histones -- Structure, Gene expression -- Analysis, Genetic transcription -- Research, Binding proteins -- Research, Health

Published

2009

3. Dynamics of the Epigenetic Landscape During Erythroid Differentiation after Gata1 Restoration

Author

Massachusetts Institute of Technology. Computer Science and Artificial Intelligence Laboratory, Kellis, Manolis, Ernst, Jason, Wu, Weisheng, Cheng, Yong, Keller, Cheryl A., Kumar, Swathi Ashok, Mishra, Tejaswini, Morrissey, Christapher, Dorman, Christine M., Chen, Kuan-Bei, Drautz, Daniela, Giardine, Belinda, Shibata, Yoichiro, Song, Lingyun, Pimkin, Max, Crawford, Gregory E., Furey, Terrence S., Miller, Webb, Taylor, James, Schuster, Stephan C., Zhang, Yu, Chiaromonte, Francesca, Blobel, Gerd A., Weiss, Mitchell J., Hardison, Ross C., Massachusetts Institute of Technology. Computer Science and Artificial Intelligence Laboratory, Kellis, Manolis, Ernst, Jason, Wu, Weisheng, Cheng, Yong, Keller, Cheryl A., Kumar, Swathi Ashok, Mishra, Tejaswini, Morrissey, Christapher, Dorman, Christine M., Chen, Kuan-Bei, Drautz, Daniela, Giardine, Belinda, Shibata, Yoichiro, Song, Lingyun, Pimkin, Max, Crawford, Gregory E., Furey, Terrence S., Miller, Webb, Taylor, James, Schuster, Stephan C., Zhang, Yu, Chiaromonte, Francesca, Blobel, Gerd A., Weiss, Mitchell J., and Hardison, Ross C.

Abstract

Interplays among lineage-specific nuclear proteins, chromatin modifying enzymes, and the basal transcription machinery govern cellular differentiation, but their dynamics of action and coordination with transcriptional control are not fully understood. Alterations in chromatin structure appear to establish a permissive state for gene activation at some loci, but they play an integral role in activation at other loci. To determine the predominant roles of chromatin states and factor occupancy in directing gene regulation during differentiation, we mapped chromatin accessibility, histone modifications, and nuclear factor occupancy genome-wide during mouse erythroid differentiation dependent on the master regulatory transcription factor GATA1. Notably, despite extensive changes in gene expression, the chromatin state profiles (proportions of a gene in a chromatin state dominated by activating or repressive histone modifications) and accessibility remain largely unchanged during GATA1-induced erythroid differentiation. In contrast, gene induction and repression are strongly associated with changes in patterns of transcription factor occupancy. Our results indicate that during erythroid differentiation, the broad features of chromatin states are established at the stage of lineage commitment, largely independently of GATA1. These determine permissiveness for expression, with subsequent induction or repression mediated by distinctive combinations of transcription factors, National Institutes of Health (U.S.) (Grant number RC1HG005334), National Science Foundation (U.S.). (Award 0905968)

Published

2012

4. Dynamics of the epigenetic landscape during erythroid differentiation after GATA1 restoration

Author

Wu, Weisheng, primary, Cheng, Yong, additional, Keller, Cheryl A., additional, Ernst, Jason, additional, Kumar, Swathi Ashok, additional, Mishra, Tejaswini, additional, Morrissey, Christapher, additional, Dorman, Christine M., additional, Chen, Kuan-Bei, additional, Drautz, Daniela, additional, Giardine, Belinda, additional, Shibata, Yoichiro, additional, Song, Lingyun, additional, Pimkin, Max, additional, Crawford, Gregory E., additional, Furey, Terrence S., additional, Kellis, Manolis, additional, Miller, Webb, additional, Taylor, James, additional, Schuster, Stephan C., additional, Zhang, Yu, additional, Chiaromonte, Francesca, additional, Blobel, Gerd A., additional, Weiss, Mitchell J., additional, and Hardison, Ross C., additional

Published

2011

5. Dynamics of the epigenetic landscape during erythroid differentiation after GATA1 restoration.

Author

Weisheng Wu, Yong Cheng, Keller, Cheryl A., Ernst, Jason, Kumar, Swathi Ashok, Mishra, Tejaswini, Morrissey, Christapher, Dorman, Christine M., Kuan-Bei Chen, Drautz, Daniela, Giardine, Belinda, Shibata, Yoichiro, Lingyun Song, Pimkin, Max, Crawford, Gregory E., Furey, Terrence S., Kellis, Manolis, Miller, Webb, Taylor, James, and Schuster, Stephan C.

Subjects

*CHROMATIN, *NUCLEAR proteins, *PROTEINS, *TRANSCRIPTION factors, *GENETIC regulation

Abstract

Interplays among lineage-specific nuclear proteins, chromatin modifying enzymes, and the basal transcription machinery govern cellular differentiation, but their dynamics of action and coordination with transcriptional control are not fully understood. Alterations in chromatin structure appear to establish a permissive state for gene activation at some loci, but they play an integral role in activation at other loci. To determine the predominant roles of chromatin states and factor occupancy in directing gene regulation during differentiation, we mapped chromatin accessibility, histone modifications, and nuclear factor occupancy genome-wide during mouse erythroid differentiation dependent on the master regulatory transcription factor GATA1. Notably, despite extensive changes in gene expression, the chromatin state profiles (proportions of a gene in a chromatin state dominated by activating or repressive histone modifications) and accessibility remain largely unchanged during GATA1-induced erythroid differentiation. In contrast, gene induction and repression are strongly associated with changes in patterns of transcription factor occupancy. Our results indicate that during erythroid differentiation, the broad features of chromatin states are established at the stage of lineage commitment, largely independently of GATA1. These determine permissiveness for expression, with subsequent induction or repression mediated by distinctive combinations of transcription factors. [ABSTRACT FROM AUTHOR]

Published

2011

6. Erythroid GATA1 function revealed by genome-wide analysis of transcription factor occupancy, histone modifications, and mRNA expression.

Author

Cheng Y, Wu W, Kumar SA, Yu D, Deng W, Tripic T, King DC, Chen KB, Zhang Y, Drautz D, Giardine B, Schuster SC, Miller W, Chiaromonte F, Zhang Y, Blobel GA, Weiss MJ, and Hardison RC

Subjects

Binding Sites, Cell Differentiation, Cell Line, Chromatin metabolism, Chromatin Immunoprecipitation, Erythroblasts cytology, Erythroid Cells cytology, GATA1 Transcription Factor pharmacology, Oligonucleotide Array Sequence Analysis, RNA, Messenger genetics, Erythropoiesis drug effects, GATA1 Transcription Factor metabolism, Gene Expression Regulation, Developmental, Genome, Histones metabolism, RNA, Messenger metabolism

Abstract

The transcription factor GATA1 regulates an extensive program of gene activation and repression during erythroid development. However, the associated mechanisms, including the contributions of distal versus proximal cis-regulatory modules, co-occupancy with other transcription factors, and the effects of histone modifications, are poorly understood. We studied these problems genome-wide in a Gata1 knockout erythroblast cell line that undergoes GATA1-dependent terminal maturation, identifying 2616 GATA1-responsive genes and 15,360 GATA1-occupied DNA segments after restoration of GATA1. Virtually all occupied DNA segments have high levels of H3K4 monomethylation and low levels of H3K27me3 around the canonical GATA binding motif, regardless of whether the nearby gene is induced or repressed. Induced genes tend to be bound by GATA1 close to the transcription start site (most frequently in the first intron), have multiple GATA1-occupied segments that are also bound by TAL1, and show evolutionary constraint on the GATA1-binding site motif. In contrast, repressed genes are further away from GATA1-occupied segments, and a subset shows reduced TAL1 occupancy and increased H3K27me3 at the transcription start site. Our data expand the repertoire of GATA1 action in erythropoiesis by defining a new cohort of target genes and determining the spatial distribution of cis-regulatory modules throughout the genome. In addition, we begin to establish functional criteria and mechanisms that distinguish GATA1 activation from repression at specific target genes. More broadly, these studies illustrate how a "master regulator" transcription factor coordinates tissue differentiation through a panoply of DNA and protein interactions.

Published

2009