Your search keyword '"Sung-Hae Lee"' showing total 7 results

1. Recruitment of transcription complexes to the beta-globin gene locus in vivo and in vitro.

Author

Vieira KF, Levings PP, Hill MA, Crusselle VJ, Kang SH, Engel JD, and Bungert J

Subjects

Animals, Humans, K562 Cells, Mice, RNA Polymerase II metabolism, Stem Cells, Transcription Factors metabolism, DNA metabolism, Globins genetics, Transcription, Genetic physiology

Abstract

Erythroid-specific, high level expression of the beta-globin genes is regulated by the locus control region (LCR), composed of multiple DNase I-hypersensitive sites and located far upstream of the genes. Recent studies have shown that LCR core elements recruit RNA polymerase II (pol II). In the present study we demonstrate the following: 1) pol II and other basal transcription factors are recruited to LCR core hypersensitive elements; 2) pol II dissociates from and re-associates with the globin gene locus during replication; 3) pol II interacts with the LCR but not with the beta-globin gene prior to erythroid differentiation in embryonic stem cells; and 4) the erythroid transcription factor NF-E2 facilitates the transfer of pol II from immobilized LCR constructs to a beta-globin gene in vitro. The data are consistent with the hypothesis that the LCR serves as the primary attachment site for the recruitment of macromolecular complexes involved in chromatin structure alterations and transcription of the globin genes.

Published

2004

2. Locus control region elements HS2 and HS3 in combination with chromatin boundaries confer high-level expression of a human beta-globin transgene in a centromeric region.

Author

Kang SH, Levings PP, Andersen F, Laipis PJ, Berns KI, Zori RT, and Bungert J

Subjects

Animals, Chickens, Humans, Mice, Mice, Transgenic, Centromere genetics, Chromatin physiology, Globins genetics, Locus Control Region, Transgenes

Abstract

Expression constructs are subject to position-effects in transgenic assays unless they harbour elements that protect them from negative or positive influences exerted by chromatin at the site of integration. Locus control regions (LCRs) and boundary elements are able to protect from position effects by preventing heterochromatization of linked genes. The LCR in the human beta-globin gene locus is located far upstream of the genes and composed of several erythroid specific DNase I hypersensitive (HS) sites. Previous studies demonstrated that the LCR HS sites act synergistically to confer position-independent and high-level globin gene expression at different integration sites in transgenic mice. Here we show that LCR HS sites 2 and 3, in combination with boundary elements derived from the chicken beta-globin gene locus, confer high-level human beta-globin gene expression in different chromosomal integration sites in transgenic mice. Moreover, we found that the construct is accessible to nucleases and highly expressed when integrated in a centromeric region. These results demonstrate that the combination of enhancer, chromatin opening and boundary activities can establish independent expression units when integrated into chromatin.

Published

2004

3. Characterization of the human beta-globin downstream promoter region.

Author

Leach KM, Vieira KF, Kang SH, Aslanian A, Teichmann M, Roeder RG, and Bungert J

Subjects

3T3 Cells, Animals, Base Sequence, Binding Sites genetics, DNA-Binding Proteins metabolism, Electrophoretic Mobility Shift Assay, Erythroid-Specific DNA-Binding Factors, Globins genetics, Humans, K562 Cells, Mice, Models, Biological, Molecular Sequence Data, Mutation, NF-E2 Transcription Factor, NF-E2 Transcription Factor, p45 Subunit, Protein Binding, Sequence Homology, Nucleic Acid, Transcription Factors metabolism, Transcription Factors, TFII metabolism, Tumor Cells, Cultured, Upstream Stimulatory Factors, Globins metabolism, Promoter Regions, Genetic genetics

Abstract

The human beta-globin gene is abundantly expressed specifically in adult erythroid cells. Stage-specific transcription is regulated principally by promoter proximal cis-regulatory elements. The basal promoter contains a non-canonical TATA-like motif as well as an initiator element. These two elements have been shown to interact with the TFII-D complex. Here we show that in addition to the TATA and initiator elements, conserved E-box motifs are located in the beta-globin downstream promoter. One of the E-box motifs overlaps the initiator and this composite element interacts with USF1 and TFII-I in vitro. Another E-box, located 60 bp 3' to the transcription initiation site, interacts with USF1 and USF2. Mutations of either the initiator or the downstream E-box impair transcription of the beta-globin gene in vitro. Mutations of a putative NF-E2-binding site in the downstream promoter region do not affect transcription in vitro. USF1, USF2, TFII-I and p45 can be crosslinked to a beta-globin promoter fragment in MEL cells in vivo, whereas only TFII-I and USF2 crosslink to the beta-globin gene in K562 cells. The summary data demonstrate that in addition to the well-characterized interactions of the TFII-D complex with the basal promoter, E-box motifs contribute to the efficient formation of transcription complexes on the adult beta-globin gene.

Published

2003

4. Locus control region elements HS2 and HS3 in combination with chromatin boundaries confer high-level expression of a human β-globin transgene in a centromeric region

Author

Robert T. Zori, Jörg Bungert, Philip J. Laipis, Kenneth I. Berns, Sung-Hae Lee Kang, Padraic P. Levings, and Felicie F. Andersen

Subjects

Genetics, Transgene, Centromere, Mice, Transgenic, Cell Biology, Biology, Locus Control Region, Chromatin, Globins, Mice, Genetic linkage, Gene expression, Animals, Humans, Transgenes, Globin, Enhancer, Chickens, Gene, Locus control region

Abstract

Expression constructs are subject to position-effects in transgenic assays unless they harbour elements that protect them from negative or positive influences exerted by chromatin at the site of integration. Locus control regions (LCRs) and boundary elements are able to protect from position effects by preventing heterochromatization of linked genes. The LCR in the human beta-globin gene locus is located far upstream of the genes and composed of several erythroid specific DNase I hypersensitive (HS) sites. Previous studies demonstrated that the LCR HS sites act synergistically to confer position-independent and high-level globin gene expression at different integration sites in transgenic mice. Here we show that LCR HS sites 2 and 3, in combination with boundary elements derived from the chicken beta-globin gene locus, confer high-level human beta-globin gene expression in different chromosomal integration sites in transgenic mice. Moreover, we found that the construct is accessible to nucleases and highly expressed when integrated in a centromeric region. These results demonstrate that the combination of enhancer, chromatin opening and boundary activities can establish independent expression units when integrated into chromatin.

Published

2004

5. Recruitment of Transcription Complexes to the β-Globin Gene Locus in Vivo and in Vitro

Author

Meredith A. Hill, Sung Hae Lee Kang, Jörg Bungert, James Douglas Engel, Padraic P. Levings, Valerie J. Crusselle, and Karen F. Vieira

Subjects

Transcription, Genetic, RNA polymerase II, urologic and male genital diseases, Biochemistry, Article, Mice, Transcription (biology), hemic and lymphatic diseases, Animals, Humans, Globin, Molecular Biology, Gene, Transcription factor, Locus control region, biology, General transcription factor, Stem Cells, DNA, Cell Biology, Molecular biology, Globins, Chromatin, biology.protein, RNA Polymerase II, K562 Cells, Transcription Factors

Abstract

Erythroid-specific, high level expression of the beta-globin genes is regulated by the locus control region (LCR), composed of multiple DNase I-hypersensitive sites and located far upstream of the genes. Recent studies have shown that LCR core elements recruit RNA polymerase II (pol II). In the present study we demonstrate the following: 1) pol II and other basal transcription factors are recruited to LCR core hypersensitive elements; 2) pol II dissociates from and re-associates with the globin gene locus during replication; 3) pol II interacts with the LCR but not with the beta-globin gene prior to erythroid differentiation in embryonic stem cells; and 4) the erythroid transcription factor NF-E2 facilitates the transfer of pol II from immobilized LCR constructs to a beta-globin gene in vitro. The data are consistent with the hypothesis that the LCR serves as the primary attachment site for the recruitment of macromolecular complexes involved in chromatin structure alterations and transcription of the globin genes.

Published

2004

6. Characterization of the human beta-globin downstream promoter region

Author

Karen F. Vieira, Robert G. Roeder, Ara Aslanian, Jörg Bungert, Sung-Hae Lee Kang, Martin Teichmann, and Kelly M. Leach

Subjects

NF-E2 Transcription Factor, Molecular Sequence Data, Response element, USF1, Electrophoretic Mobility Shift Assay, Biology, Models, Biological, Mice, Transcription Factors, TFII, Initiator element, Transcription (biology), Sequence Homology, Nucleic Acid, hemic and lymphatic diseases, Tumor Cells, Cultured, Genetics, Animals, Humans, Promoter Regions, Genetic, Enhancer, Transcription factor, Binding Sites, Base Sequence, Promoter, Articles, 3T3 Cells, Molecular biology, Globins, DNA-Binding Proteins, NF-E2 Transcription Factor, p45 Subunit, Mutation, biology.protein, Erythroid-Specific DNA-Binding Factors, Upstream Stimulatory Factors, K562 Cells, Protein Binding, Transcription Factors

Abstract

The human beta-globin gene is abundantly expressed specifically in adult erythroid cells. Stage-specific transcription is regulated principally by promoter proximal cis-regulatory elements. The basal promoter contains a non-canonical TATA-like motif as well as an initiator element. These two elements have been shown to interact with the TFII-D complex. Here we show that in addition to the TATA and initiator elements, conserved E-box motifs are located in the beta-globin downstream promoter. One of the E-box motifs overlaps the initiator and this composite element interacts with USF1 and TFII-I in vitro. Another E-box, located 60 bp 3' to the transcription initiation site, interacts with USF1 and USF2. Mutations of either the initiator or the downstream E-box impair transcription of the beta-globin gene in vitro. Mutations of a putative NF-E2-binding site in the downstream promoter region do not affect transcription in vitro. USF1, USF2, TFII-I and p45 can be crosslinked to a beta-globin promoter fragment in MEL cells in vivo, whereas only TFII-I and USF2 crosslink to the beta-globin gene in K562 cells. The summary data demonstrate that in addition to the well-characterized interactions of the TFII-D complex with the basal promoter, E-box motifs contribute to the efficient formation of transcription complexes on the adult beta-globin gene.

Published

2003

7. Combining chromatin immunoprecipitation and DNA footprinting: a novel method to analyze protein–DNA interactions in vivo

Author

Jörg Bungert, Sung-Hae Lee Kang, and Karen F. Vieira

Subjects

Immunoprecipitation, Molecular Sequence Data, DNA Footprinting, DNA footprinting, Biology, chemistry.chemical_compound, NF-E2 Transcription Factor, Genetics, Tumor Cells, Cultured, Animals, Humans, Promoter Regions, Genetic, NAR Methods Online, Base Sequence, Protein footprinting, DNA, Molecular biology, Precipitin Tests, Footprinting, Chromatin, Cell biology, Globins, DNA-Binding Proteins, chemistry, NF-E2 Transcription Factor, p45 Subunit, Erythroid-Specific DNA-Binding Factors, Upstream Stimulatory Factors, DNase footprinting assay, Chromatin immunoprecipitation, Protein Binding, Transcription Factors

Abstract

A variety of methods are available to analyze protein-DNA interactions in vivo. Two of the most prominent of these methods are chromatin immunoprecipitation (ChIP) and in vivo footprinting. Both of these procedures have specific limitations. For example, the ChIP assay fails to document where exactly a protein binds in vivo. The precipitation of a specific segment of DNA with antibodies directed against DNA-binding proteins does not necessarily indicate that the protein directly interacts with a sequence in the precipitate but could rather reflect protein-protein interactions. Furthermore, the results of in vivo footprinting studies are inconclusive if a DNA sequence is analyzed that is bound by a specific protein in only a certain fraction of cells. Finally, in vivo footprinting does not indicate which protein is bound at a specific site. We have developed a new procedure that combines the ChIP assay and DMS footprinting techniques. Using this method we show here that antibodies specific for USF1 and NF-E2 precipitate the murine beta-globin promoter in MEL cells. DMS footprinting analysis of the DNA precipitated with NF-E2 antibodies revealed a protection over a partial NF-E2-binding site in the beta-globin downstream promoter region. We believe that this novel method will generally benefit investigators interested in analyzing protein-DNA interactions in vivo.

Published

2002