Your search keyword '"Heike Brand"' showing total 3 results

1. A Novel Promoter Is Involved in the Expression of Estrogen Receptor α in Human Testis and Epididymis

Author

Martin Kos, Heike Brand, George Reid, Gilles Flouriot, Frank Gannon, Stefanie Denger, and Jörg Gromoll

Subjects

Male, medicine.medical_specialty, TATA box, Molecular Sequence Data, CAAT box, Gene Expression, Sequence Homology, Estrogen receptor, Biology, Transfection, Exon, Endocrinology, Internal medicine, Testis, medicine, Humans, RNA, Messenger, Promoter Regions, Genetic, Receptor, Cells, Cultured, Aged, Epididymis, Messenger RNA, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, Alternative splicing, Estrogen Receptor alpha, Chromosome Mapping, TATA Box, Molecular biology, Alternative Splicing, medicine.anatomical_structure, Receptors, Estrogen, RNA, Chromosomes, Human, Pair 6

Abstract

The role of estrogens in the development and physiology of the male reproductive tract remains provocative, with a growing body of evidence suggesting that estrogens are able to influence normal testis development and physiology, through their classical receptors, estrogen receptor (ER)-alpha and ER-beta. We describe the identification and characterization of a new promoter that is involved in the expression of ER-alpha in the epididymis and in testis. This promoter lies on chromosome 6q25.1, approximately 16 kb upstream of the first coding exon of ER-alpha. Sequence analysis indicates that this promoter has a conventional TATA box and GC box but no upstream CAAT sequence. Alternative splicing results in at least two species of mRNA encoding ER-alpha being synthesized from this promoter. Transcription profiling of human tissues shows that, among those tested, this promoter is predominantly active only in testis and epididymal tissues. Transient transfection assays using this new promoter in a number of cell lines indicate that the region we have identified functions as a promoter and that tissue-specific regulation is likely to be dependent on inhibitory sequences greater than 1 kb upstream of the transcription start site.

Published

2002

2. ERα Gene Expression in Human Primary Osteoblasts: Evidence for the Expression of Two Receptor Proteins

Author

Gilles Flouriot, Dominik Parsch, George Reid, Martin Kos, Vera Sonntag-Buck, Stefanie Denger, Kenneth S. Korach, Frank Gannon, and Heike Brand

Subjects

Gene isoform, Biology, Transfection, Gene product, Transactivation, Exon, Endocrinology, Gene expression, Tumor Cells, Cultured, Humans, Protein Isoforms, RNA, Messenger, Receptor, Molecular Biology, Osteoblasts, Reverse Transcriptase Polymerase Chain Reaction, Single-Strand Specific DNA and RNA Endonucleases, Alternative splicing, Estrogen Receptor alpha, Translation (biology), General Medicine, Precipitin Tests, Molecular biology, Alternative Splicing, Blotting, Southern, Gene Expression Regulation, Receptors, Estrogen, Electrophoresis, Polyacrylamide Gel

Abstract

The beneficial influence of E2 in the maintenance of healthy bone is well recognized. However, the way in which the actions of this hormone are mediated is less clearly understood. Western blot analysis of ERα in osteoblasts clearly demonstrated that the well characterized 66-kDa ERα was only one of the ERα isoforms present. Here we describe a 46-kDa isoform of ERα, expressed at a level similar to the 66-kDa isoform, that is also present in human primary osteoblasts. This shorter isoform is generated by alternative splicing of an ERα gene product, which results in exon 1 being skipped with a start codon in exon 2 used to initiate translation of the protein. Consequently, the transactivation domain AF-1 of this ERα isoform is absent. Functional analysis revealed that human (h)ERα46 is able to heterodimerize with the full-length ERα and also with ERβ. Further, a DNA-binding complex that corresponds to hERα46 is detectable in human osteoblasts. We have shown that hERα46 is a strong inhibitor of hERα66 when they are coexpressed in the human osteosarcoma cell line SaOs. As a functional consequence, proliferation of the transfected cells is inhibited when increasing amounts of hERα46 are cotransfected with hERα66. In addition to human bone, the expression of the alternatively spliced ERα mRNA variant is also detectable in bone of ERα knockout mice. These data suggest that, in osteoblasts, E2 can act in part through an ERα isoform that is markedly different from the 66-kDa receptor. The expression of two ERα protein isoforms may account, in part, for the differential action that estrogens and estrogen analogs have in different tissues. In particular, the current models of the action of estrogens should be reevaluated to take account of the presence of at least two ERα protein isoforms in bone and perhaps in other tissues.

Published

2001

3. The 3′-Untranslated Region of the Human Estrogen Receptor α Gene Mediates Rapid Messenger Ribonucleic Acid Turnover1

Author

Heike Brand, Mary-Rose Kenealy, Vera Sonntag-Buck, Thomas Dandekar, Gilles Flouriot, and Frank Gannon

Subjects

Chloramphenicol acetyltransferase, Untranslated region, Messenger RNA, Endocrinology, MRNA destabilization, Three prime untranslated region, RNA, Biology, Gene, Molecular biology, Estrogen receptor alpha

Abstract

Human estrogen receptor-alpha messenger RNA (hERalpha mRNA) has a relatively short half-life, which was determined to be approximately 5 h in MCF-7 cell line after actinomycin D treatment. The 3'-untranslated region (3'UTR) of hERalpha mRNA was previously shown to completely down-regulate chloramphenicol acetyltransferase activity when present at the 3'-end of chloramphenicol acetyltransferase transcripts, suggesting a destabilizing function of the hERalpha 3'UTR sequence. Chimeric genes composed of a serum-inducible Fos promoter, GH-coding sequences, and different segments of the hERalpha complementary DNA 3'UTR sequence were used to confirm this hypothesis and to localize the RNA region responsible for the destabilizing effect. The presence of the complete hERalpha 3'UTR reduced the half-life of the reporter mRNA from more than 24 to 3 h. When the hERalpha 3'UTR was subdivided into four fragments (UTR1-4), one fragment, UTR2, retained the most ability to down-regulate the reporter mRNA (t1/2 = 4 h). A stretch of four AUUUA motifs within UTR2 was shown not to mediate mRNA destabilization. In contrast, further subdivision of the UTR2 into three parts (UTR2a-c) resulted in the loss of the destabilizing activity. Finally, recombination of two UTR2 subfragments (UTR2a and -b) partially restored this function, indicating a cooperative role among the three UTR2a-c subfragments in the process that leads to destabilization of the hERalpha transcript.

Published

2000