Functional characterization of a human histone gene cluster duplication

Corey D. Braastad; Hayk Hovhannisyan; Andre J. Van Wijnen; Janet L. Stein; Gary S. Stein

doi:10.1016/j.gene.2004.07.036

Functional characterization of a human histone gene cluster duplication

Corey D. Braastad, Hayk Hovhannisyan, Andre J. Van Wijnen, Janet L. Stein, Gary S. Stein

Orthopedic Surgery

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Abstract

Histones are the major protein component of nucleosomes, and de novo histone synthesis is essential for packaging newly replicated DNA into chromatin. As a result, histone gene expression is exquisitely and functionally coupled with DNA replication. Vastly divergent organisms such as yeast, fly and human all demonstrate the phylogenetically conserved propensity to maintain clustering of histone genes at one or more genomic loci. Although specific mechanisms are unclear, clustering is presumed to be important for common stringent transcriptional control of these genes at the G1/S phase transition. In this study, we describe a genomic duplication of the human histone gene cluster located at chromosome 1q21, which effectively doubles the previously known size and gene number of that cluster. The duplication persists in all examined tissues and cell lines, and the duplicated genes are transcriptionally active. Levels of messenger RNAs for duplicated histone H4 genes are high relative to those for non-duplicated H4 genes. Our data suggest that transcriptionally robust histone H4 genes may have been preferentially duplicated during evolution.

Original language	English (US)
Pages (from-to)	35-40
Number of pages	6
Journal	Gene
Volume	342
Issue number	1
DOIs	https://doi.org/10.1016/j.gene.2004.07.036
State	Published - Nov 1 2004

Keywords

1q21
Cell cycle
Gene amplification
Histone
Histone mRNA
Human genome

ASJC Scopus subject areas

Genetics

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10.1016/j.gene.2004.07.036

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title = "Functional characterization of a human histone gene cluster duplication",

abstract = "Histones are the major protein component of nucleosomes, and de novo histone synthesis is essential for packaging newly replicated DNA into chromatin. As a result, histone gene expression is exquisitely and functionally coupled with DNA replication. Vastly divergent organisms such as yeast, fly and human all demonstrate the phylogenetically conserved propensity to maintain clustering of histone genes at one or more genomic loci. Although specific mechanisms are unclear, clustering is presumed to be important for common stringent transcriptional control of these genes at the G1/S phase transition. In this study, we describe a genomic duplication of the human histone gene cluster located at chromosome 1q21, which effectively doubles the previously known size and gene number of that cluster. The duplication persists in all examined tissues and cell lines, and the duplicated genes are transcriptionally active. Levels of messenger RNAs for duplicated histone H4 genes are high relative to those for non-duplicated H4 genes. Our data suggest that transcriptionally robust histone H4 genes may have been preferentially duplicated during evolution.",

keywords = "1q21, Cell cycle, Gene amplification, Histone, Histone mRNA, Human genome",

author = "Braastad, {Corey D.} and Hayk Hovhannisyan and {Van Wijnen}, {Andre J.} and Stein, {Janet L.} and Stein, {Gary S.}",

note = "Funding Information: This publication was made possible by grants from the National Institutes of Health (GM32010 and 5P30 DK32520). Its contents are solely the responsibility of the authors and do not necessarily represent the official view of the National Institutes of Health. We thank all members of our laboratory, and in particular Drs. William Holmes, Shirwin Pockwinse and Humberto Rossi, for the thoughtful discussions and assistance with reagents. We also thank Rosa Mastrotataro for technical assistance. Copyright: Copyright 2012 Elsevier B.V., All rights reserved.",

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AU - Stein, Gary S.

N1 - Funding Information: This publication was made possible by grants from the National Institutes of Health (GM32010 and 5P30 DK32520). Its contents are solely the responsibility of the authors and do not necessarily represent the official view of the National Institutes of Health. We thank all members of our laboratory, and in particular Drs. William Holmes, Shirwin Pockwinse and Humberto Rossi, for the thoughtful discussions and assistance with reagents. We also thank Rosa Mastrotataro for technical assistance. Copyright: Copyright 2012 Elsevier B.V., All rights reserved.

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Y1 - 2004/11/1

N2 - Histones are the major protein component of nucleosomes, and de novo histone synthesis is essential for packaging newly replicated DNA into chromatin. As a result, histone gene expression is exquisitely and functionally coupled with DNA replication. Vastly divergent organisms such as yeast, fly and human all demonstrate the phylogenetically conserved propensity to maintain clustering of histone genes at one or more genomic loci. Although specific mechanisms are unclear, clustering is presumed to be important for common stringent transcriptional control of these genes at the G1/S phase transition. In this study, we describe a genomic duplication of the human histone gene cluster located at chromosome 1q21, which effectively doubles the previously known size and gene number of that cluster. The duplication persists in all examined tissues and cell lines, and the duplicated genes are transcriptionally active. Levels of messenger RNAs for duplicated histone H4 genes are high relative to those for non-duplicated H4 genes. Our data suggest that transcriptionally robust histone H4 genes may have been preferentially duplicated during evolution.

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Functional characterization of a human histone gene cluster duplication

Abstract

Keywords

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