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GATA-3基因座中泌尿生殖系统、中枢神经系统和心内膜特异性转录调控元件的定位。

Localization of distant urogenital system-, central nervous system-, and endocardium-specific transcriptional regulatory elements in the GATA-3 locus.

作者信息

Lakshmanan G, Lieuw K H, Lim K C, Gu Y, Grosveld F, Engel J D, Karis A

机构信息

Department of Biochemistry, Molecular Biology and Cell Biology, Northwestern University, Evanston, Illinois 60208, USA.

出版信息

Mol Cell Biol. 1999 Feb;19(2):1558-68. doi: 10.1128/MCB.19.2.1558.

DOI:10.1128/MCB.19.2.1558
PMID:9891089
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC116084/
Abstract

We found previously that neither a 6-kbp promoter fragment nor even a 120-kbp yeast artificial chromosome (YAC) containing the whole GATA-3 gene was sufficient to recapitulate its full transcription pattern during embryonic development in transgenic mice. In an attempt to further identify tissue-specific regulatory elements modulating the dynamic embryonic pattern of the GATA-3 gene, we have examined the expression of two much larger (540- and 625-kbp) GATA-3 YACs in transgenic animals. A lacZ reporter gene was first inserted into both large GATA-3 YACs. The transgenic YAC patterns were then compared to those of embryos bearing the identical lacZ insertion in the chromosomal GATA-3 locus (creating GATA-3/lacZ "knock-ins"). We found that most of the YAC expression sites and tissues are directly reflective of the endogenous pattern, and detailed examination of the integrated YAC transgenes allowed the general localization of a number of very distant transcriptional regulatory elements (putative central nervous system-, endocardium-, and urogenital system-specific enhancers). Remarkably, even the 625-kbp GATA-3 YAC, containing approximately 450 kbp and 150 kbp of 5' and 3' flanking sequences, respectively, does not contain the full transcriptional regulatory potential of the endogenous locus and is clearly missing regulatory elements that confer tissue-specific expression to GATA-3 in a subset of neural crest-derived cell lineages.

摘要

我们先前发现,无论是一个6千碱基对的启动子片段,还是甚至一个包含整个GATA-3基因的120千碱基对的酵母人工染色体(YAC),都不足以在转基因小鼠的胚胎发育过程中重现其完整的转录模式。为了进一步鉴定调节GATA-3基因动态胚胎模式的组织特异性调控元件,我们检测了两个大得多(540千碱基对和625千碱基对)的GATA-3 YAC在转基因动物中的表达。首先将一个lacZ报告基因插入两个大的GATA-3 YAC中。然后将转基因YAC模式与在染色体GATA-3位点携带相同lacZ插入的胚胎(产生GATA-3/lacZ“敲入”)的模式进行比较。我们发现大多数YAC表达位点和组织直接反映了内源性模式,并且对整合的YAC转基因的详细检查使得能够大致定位许多非常遥远的转录调控元件(假定的中枢神经系统、心内膜和泌尿生殖系统特异性增强子)。值得注意的是,即使是包含分别约450千碱基对和150千碱基对的5'和3'侧翼序列的625千碱基对的GATA-3 YAC,也不包含内源性位点的全部转录调控潜力,并且明显缺少赋予GATA-3在一部分神经嵴衍生细胞谱系中组织特异性表达的调控元件。

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本文引用的文献

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Partial rescue of GATA-3 by yeast artificial chromosome transgenes.通过酵母人工染色体转基因对GATA-3进行部分挽救。
Dev Biol. 1998 Dec 15;204(2):451-63. doi: 10.1006/dbio.1998.8991.
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Alpha2p controls donor preference during mating type interconversion in yeast by inactivating a recombinational enhancer of chromosome III.α2p通过使III号染色体的重组增强子失活来控制酵母交配型相互转换过程中的供体偏好。
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Temporal and spatial control of murine GATA-3 transcription by promoter-proximal regulatory elements.启动子近端调控元件对小鼠GATA-3转录的时空控制
Dev Biol. 1997 Aug 1;188(1):1-16. doi: 10.1006/dbio.1997.8575.
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A "knockdown" mutation created by cis-element gene targeting reveals the dependence of erythroid cell maturation on the level of transcription factor GATA-1.通过顺式元件基因靶向产生的“敲低”突变揭示了红系细胞成熟对转录因子GATA-1水平的依赖性。
Proc Natl Acad Sci U S A. 1997 Jun 24;94(13):6781-5. doi: 10.1073/pnas.94.13.6781.
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The transcription factor GATA-3 is necessary and sufficient for Th2 cytokine gene expression in CD4 T cells.转录因子GATA-3对于CD4 T细胞中Th2细胞因子基因的表达是必需且充分的。
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Good genes in bad neighbourhoods.身处不良环境中的优良基因。
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