Your search keyword '"Clare SE"' showing total 2 results

1. Characterization of the H1t promoter: role of conserved histone 1 AC and TG elements and dominance of the cap-proximal silencer.

Author

Horvath GC, Clare SE, Kistler MK, and Kistler WS

Subjects

3T3 Cells, Animals, Blotting, Western, Electrophoretic Mobility Shift Assay, Gene Expression Regulation, Genes, Reporter, Mice, Mutagenesis, RNA, Messenger analysis, Regulatory Sequences, Nucleic Acid, Ribonucleases metabolism, Transfection, Histones genetics, Promoter Regions, Genetic

Abstract

H1t is a testis-specific variant histone 1 gene transcribed in pachytene spermatocytes. As part of a program to understand its transcriptional control, we have investigated the effect of the cap-proximal, GC-rich silencer element in the context of various lengths of upstream sequence. By transient transfection of NIH 3T3 cells, we showed that a targeted mutation in the silencer has a large (>10-fold) effect on reporter gene expression, regardless of the length of upstream sequence present. No other discrete silencing activity was observed in the upstream region extending to nucleotide -1842. Similarly, when the silencer mutation was introduced into the natural gene, H1t expression was readily detected in permanently transfected cells by both RNase protection and Western blot analysis, regardless of the extent of 5' or 3' flanking genomic DNA. In constructs with the mutated silencer, we showed interdependence of the characteristic H1 AC and TG box regulatory elements. Promoter up-regulation occurred only when both were intact, and possibly identical binding factors were demonstrated for each by electrophoretic mobility shift assays. In view of its precisely regulated but limited expression, it is interesting that H1t retains all the promoter elements known to activate standard H1 genes, including the TG/AC unit, SP1 site, and CCAAT element. Their presence emphasizes the apparent dominance of the silencer element in most cells.

Published

2001

2. Characterization of the promoter region of the rat testis-specific histone H1t gene.

Author

Clare SE, Hatfield WR, Fantz DA, Kistler WS, and Kistler MK

Subjects

Animals, Base Sequence, Consensus Sequence, Cross-Linking Reagents, DNA chemistry, DNA Footprinting, Deoxyribonuclease I, Electrophoresis, Liver metabolism, Male, Molecular Sequence Data, Rats, Rats, Sprague-Dawley, Repetitive Sequences, Nucleic Acid, Transcription, Genetic, Ultraviolet Rays, Histones genetics, Promoter Regions, Genetic, Testis metabolism

Abstract

Histone H1t is synthesized only in male germ cells during the late pachytene stage of meiosis and is retained in spermatids until the nucleus elongates. Transgenic experiments suggest that spermatocyte-directing sequences lie within 140 base pairs of the cap site. To study the mechanism of this specificity we compared the DNase I footprints made on the immediate promoter regions of H1t and H1d (a typical somatic H1) by testis and liver extracts and observed both common and differentially protected regions. The common footprints of H1t included an Sp1 consensus (GC box 1) and a CCAAT motif. Electrophoretic mobility shift assays (EMSA) identified ubiquitous binding factors for GC box 1 and a binding factor for the CCAAT element that we identified immunologically as H1TF2. H1t-specific footprints occurred over the palindrome CCTAGG and a GC-rich sequence downstream of the TATA box (GC box 2). EMSA analysis of the palindrome identified testis-specific as well as ubiquitous binding factors. UV irradiation of a palindrome-binding reaction generated a cross-linked doublet of about 50 kDa from both testis and liver. Protein factors that bound to the GC box 2 sequence were similar from testis and liver, and GC box 1 and an Sp1 consensus competed for them. In vitro transcription directed by H1t occurred at comparable levels in testis and liver extracts. The importance of both GC box 1 and CCAAT elements was demonstrated by deletion analysis and by oligonucleotide competition. No dependence on the H1t palindrome was observed for in vitro transcription.

Published

1997