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Literature DB >> 8336726

Transcription of the histone H5 gene is regulated by three differentiation-specific enhancers.

S Rousseau¹, M Asselin, J Renaud, A Ruiz-Carrillo.

Abstract

Histone H5, an early marker of the avian erythroid lineage, is expressed at low levels in early erythroid precursors and at higher levels in more mature cells. We show that the increase in H5 expression is due to transcriptional activation of the H5 gene following differentiation of precursor CFU(E). We have found and characterized two upstream enhancers, E1 (between -2233 and -1878 from the site of transcription initiation, +1) and E3 (between -1321 and -1163), and confirmed the presence of a downstream enhancer (C. D. Trainor, S. J. Stamler, and J. D. Engel, Nature [London] 328:827-830, 1987) E7 (between +846 and +1181) which are responsible for the increase in H5 gene transcription. The enhancers had a weak effect in nondifferentiated CFU(E) but a strong effect when the cells were induced to differentiate. Cooperation among the three enhancers, however, was not required for H5 gene activity in the differentiated cells. The enhancers contain binding sites for several ubiquitous and erythroid cell-specific nuclear proteins, including GATA-1, as demonstrated with GATA-1-specific antibodies. Although the GATA sites were required for enhancer function, the concentration of GATA-1, GATA-2, and GATA-3 decreased during cell differentiation, and overexpression of these factors had little effect on H5 transcription. Hence, the differentiation-specific effect of the enhancers is not mediated by changes in relative levels of the GATA factors. Functional analysis of the H5 promoter indicated that the requirement of several elements, including a GC box necessary for transcription enhancement, did not change during the early stages of CFU(E) differentiation. However, the UPE, a positive element in proliferating CFU(E) recognized by the transcription factor H4TF2, was dispensable in the differentiated cells. These results suggest that as the cells enter the final stages of differentiation, there is a reprogramming of the regulatory factors that control H5 transcription and that the enhancers rescue and increase the activity of the promoter.

Entities: Chemical Gene

Mesh：

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Year: 1993 PMID： 8336726 PMCID： PMC360129 DOI： 10.1128/mcb.13.8.4904-4917.1993

Source DB: PubMed Journal: Mol Cell Biol ISSN： 0270-7306 Impact factor: 4.272

58 in total

1. Role of an adenovirus E2 promoter binding factor in E1A-mediated coordinate gene control.

Authors: I Kovesdi; R Reichel; J R Nevins
Journal: Proc Natl Acad Sci U S A Date: 1987-04 Impact factor: 11.205

2. Erythroblast cell lines transformed by a temperature-sensitive mutant of avian erythroblastosis virus: a model system to study erythroid differentiation in vitro.

Authors: H Beug; G Doederlein; C Freudenstein; T Graf
Journal: J Cell Physiol Suppl Date: 1982

2. In situ footprinting of chicken histone H5 gene in mature and immature erythrocytes reveals common factor-binding sites.

Authors: J M Sun; R Ferraiuolo; J R Davie
Journal: Chromosoma Date: 1996-04 Impact factor: 4.316

3. Initiation binding repressor, a factor that binds to the transcription initiation site of the histone h5 gene, is a glycosylated member of a family of cell growth regulators [corrected].

Authors: A Gómez-Cuadrado; M Martín; M Noël; A Ruiz-Carrillo
Journal: Mol Cell Biol Date: 1995-12 Impact factor: 4.272

4. Selective synergy of immunoglobulin enhancer elements in B-cell development: a characteristic of kappa light chain enhancers, but not heavy chain enhancers.

Authors: R Fulton; B van Ness
Journal: Nucleic Acids Res Date: 1994-10-11 Impact factor: 16.971

4 in total

Transcription of the histone H5 gene is regulated by three differentiation-specific enhancers.

1. Role of an adenovirus E2 promoter binding factor in E1A-mediated coordinate gene control.

2. Erythroblast cell lines transformed by a temperature-sensitive mutant of avian erythroblastosis virus: a model system to study erythroid differentiation in vitro.

3. Genomic organization of the genes coding for the six main histones of the chicken: complete sequence of the H5 gene.

4. Inverted duplication of histone genes in chicken and disposition of regulatory sequences.

5. Fine analysis of the active H5 gene chromatin of chicken erythroid cells at different stages of differentiation.

6. Analysis of nuclear factor I binding to DNA using degenerate oligonucleotides.

7. Monoclonal antibodies against histone H5. Epitope mapping and binding to chromatin.

8. A simple, non-chromatographic procedure to purify immunoglobulins from serum and ascites fluid.

9. Repression of the H5 histone gene by a factor from erythrocytes that binds to the region of transcription initiation.

10. Endonuclease G: a (dG)n X (dC)n-specific DNase from higher eukaryotes.

1. Distribution of histone H3.3 in hematopoietic cell lineages.

2. In situ footprinting of chicken histone H5 gene in mature and immature erythrocytes reveals common factor-binding sites.

3. Initiation binding repressor, a factor that binds to the transcription initiation site of the histone h5 gene, is a glycosylated member of a family of cell growth regulators [corrected].

4. Selective synergy of immunoglobulin enhancer elements in B-cell development: a characteristic of kappa light chain enhancers, but not heavy chain enhancers.