Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes

Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes

<p>Abstract</p> <p>Background</p> <p>Mammalian hepatic lipase (HL) genes are transcribed almost exclusively in hepatocytes. The basis for this liver-restricted expression is not completely understood. We hypothesized that the responsible cis-acting elements are conserve...

Full description

Bibliographic Details
Main Authors: Jansen Hans, Botma Gert-Jan, van Deursen Diederik, Verhoeven Adrie JM
Format: Article
Language:English
Published: BMC 2007-04-01
Series:BMC Genomics
Online Access:http://www.biomedcentral.com/1471-2164/8/99
id doaj-e086b6cb2fe34b089b8661325664a86c
record_format Article
spelling doaj-e086b6cb2fe34b089b8661325664a86c2020-11-25T02:19:31ZengBMCBMC Genomics1471-21642007-04-01819910.1186/1471-2164-8-99Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genesJansen HansBotma Gert-Janvan Deursen DiederikVerhoeven Adrie JM<p>Abstract</p> <p>Background</p> <p>Mammalian hepatic lipase (HL) genes are transcribed almost exclusively in hepatocytes. The basis for this liver-restricted expression is not completely understood. We hypothesized that the responsible cis-acting elements are conserved among mammalian HL genes. To identify these elements, we made a genomic comparison of 30 kb of 5'-flanking region of the rat, mouse, rhesus monkey, and human HL genes. The in silico data were verified by promoter-reporter assays in transfected hepatoma HepG2 and non-hepatoma HeLa cells using serial 5'-deletions of the rat HL (-2287/+9) and human HL (-685/+13) promoter region.</p> <p>Results</p> <p>Highly conserved elements were present at the proximal promoter region, and at 14 and 22 kb upstream of the transcriptional start site. Both of these upstream elements increased transcriptional activity of the human HL (-685/+13) promoter region 2–3 fold. Within the proximal HL promoter region, conserved clusters of transcription factor binding sites (TFBS) were identified at -240/-200 (module A), -80/-40 (module B), and -25/+5 (module C) by the rVista software. In HepG2 cells, modules B and C, but not module A, were important for basal transcription. Module B contains putative binding sites for hepatocyte nuclear factors HNF1α. In the presence of module B, transcription from the minimal HL promoter was increased 1.5–2 fold in HepG2 cells, but inhibited 2–4 fold in HeLa cells.</p> <p>Conclusion</p> <p>Our data demonstrate that searching for conserved non-coding sequences by comparative genomics is a valuable tool in identifying candidate enhancer elements. With this approach, we found two putative enhancer elements in the far upstream region of the HL gene. In addition, we obtained evidence that the -80/-40 region of the HL gene is responsible for enhanced HL promoter activity in hepatoma cells, and for silencing HL promoter activity in non-liver cells.</p> http://www.biomedcentral.com/1471-2164/8/99
collection DOAJ
language English
format Article
sources DOAJ
author Jansen Hans
Botma Gert-Jan
van Deursen Diederik
Verhoeven Adrie JM
spellingShingle Jansen Hans
Botma Gert-Jan
van Deursen Diederik
Verhoeven Adrie JM
Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes
BMC Genomics
author_facet Jansen Hans
Botma Gert-Jan
van Deursen Diederik
Verhoeven Adrie JM
author_sort Jansen Hans
title Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes
title_short Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes
title_full Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes
title_fullStr Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes
title_full_unstemmed Comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes
title_sort comparative genomics and experimental promoter analysis reveal functional liver-specific elements in mammalian hepatic lipase genes
publisher BMC
series BMC Genomics
issn 1471-2164
publishDate 2007-04-01
description <p>Abstract</p> <p>Background</p> <p>Mammalian hepatic lipase (HL) genes are transcribed almost exclusively in hepatocytes. The basis for this liver-restricted expression is not completely understood. We hypothesized that the responsible cis-acting elements are conserved among mammalian HL genes. To identify these elements, we made a genomic comparison of 30 kb of 5'-flanking region of the rat, mouse, rhesus monkey, and human HL genes. The in silico data were verified by promoter-reporter assays in transfected hepatoma HepG2 and non-hepatoma HeLa cells using serial 5'-deletions of the rat HL (-2287/+9) and human HL (-685/+13) promoter region.</p> <p>Results</p> <p>Highly conserved elements were present at the proximal promoter region, and at 14 and 22 kb upstream of the transcriptional start site. Both of these upstream elements increased transcriptional activity of the human HL (-685/+13) promoter region 2–3 fold. Within the proximal HL promoter region, conserved clusters of transcription factor binding sites (TFBS) were identified at -240/-200 (module A), -80/-40 (module B), and -25/+5 (module C) by the rVista software. In HepG2 cells, modules B and C, but not module A, were important for basal transcription. Module B contains putative binding sites for hepatocyte nuclear factors HNF1α. In the presence of module B, transcription from the minimal HL promoter was increased 1.5–2 fold in HepG2 cells, but inhibited 2–4 fold in HeLa cells.</p> <p>Conclusion</p> <p>Our data demonstrate that searching for conserved non-coding sequences by comparative genomics is a valuable tool in identifying candidate enhancer elements. With this approach, we found two putative enhancer elements in the far upstream region of the HL gene. In addition, we obtained evidence that the -80/-40 region of the HL gene is responsible for enhanced HL promoter activity in hepatoma cells, and for silencing HL promoter activity in non-liver cells.</p>
url http://www.biomedcentral.com/1471-2164/8/99
work_keys_str_mv AT jansenhans comparativegenomicsandexperimentalpromoteranalysisrevealfunctionalliverspecificelementsinmammalianhepaticlipasegenes
AT botmagertjan comparativegenomicsandexperimentalpromoteranalysisrevealfunctionalliverspecificelementsinmammalianhepaticlipasegenes
AT vandeursendiederik comparativegenomicsandexperimentalpromoteranalysisrevealfunctionalliverspecificelementsinmammalianhepaticlipasegenes
AT verhoevenadriejm comparativegenomicsandexperimentalpromoteranalysisrevealfunctionalliverspecificelementsinmammalianhepaticlipasegenes
_version_ 1724876290796814336

Similar Items