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成对样同源结构域蛋白Phox2a和Phox2b负责多巴胺β-羟化酶基因的去甲肾上腺素能细胞特异性转录。

Paired-like homeodomain proteins, Phox2a and Phox2b, are responsible for noradrenergic cell-specific transcription of the dopamine beta-hydroxylase gene.

作者信息

Yang C, Kim H S, Seo H, Kim C H, Brunet J F, Kim K S

机构信息

Department of Neurology, University of Tennessee, College of Medicine, Memphis 38163, USA.

出版信息

J Neurochem. 1998 Nov;71(5):1813-26. doi: 10.1046/j.1471-4159.1998.71051813.x.

DOI:10.1046/j.1471-4159.1998.71051813.x
PMID:9798905
Abstract

Recently, a murine paired-like homeobox gene, Phox2a, has been identified whose product is critical for the development of several major noradrenergic neuron populations, including the locus coeruleus. In noradrenergic neurons, dopamine beta-hydroxylase (DBH) is a hallmark protein and catalyzes the conversion of dopamine to noradrenaline. Our previous studies have shown that a composite promoter (domain IV), residing at -185 to -150 bp upstream of the transcription start site, is critical for DBH transcription and is comprised of multiple cis-acting elements, including a cyclic AMP response element, a YY1 binding site, and two core motifs of the homeodomain (HD)-binding site. Here, we show that the HD-binding site residing within domain IV is a noradrenergic-specific cis-acting element. In contrast, the cyclic AMP response element is active in all cell lines tested. We provide evidence that Phox2a is expressed only in DBH-positive cell lines and interacts with the HD-binding site. Forced expression of Phox2a robustly activates DBH promoter activity in DBH-negative cell lines (>10-fold), but increased it only marginally (<50%) in DBH-positive cell lines. Furthermore, another protein factor with an identical HD, Phox2b, also activates DBH transcription with an efficiency comparable to that of Phox2a. In contrast, neither Phox2a nor Phox2b was able to transactivate tyrosine hydroxylase transcription, indicating that these transcription factors differentially activate catecholamine-synthesizing gene transcription. Together with the Phox2a knockout experiment, the studies described here make Phox2a and Phox2b the first strong candidate transcription factors for determining a neurotransmitter phenotype in vertebrates.

摘要

最近,一种小鼠配对样同源盒基因Phox2a被鉴定出来,其产物对于包括蓝斑核在内的几个主要去甲肾上腺素能神经元群体的发育至关重要。在去甲肾上腺素能神经元中,多巴胺β-羟化酶(DBH)是一种标志性蛋白,催化多巴胺转化为去甲肾上腺素。我们之前的研究表明,位于转录起始位点上游-185至-150 bp处的一个复合启动子(结构域IV)对于DBH转录至关重要,它由多个顺式作用元件组成,包括一个环磷酸腺苷反应元件、一个YY1结合位点以及同源结构域(HD)结合位点的两个核心基序。在此,我们表明位于结构域IV内的HD结合位点是一个去甲肾上腺素能特异性顺式作用元件。相比之下,环磷酸腺苷反应元件在所有测试的细胞系中都有活性。我们提供的证据表明,Phox2a仅在DBH阳性细胞系中表达,并与HD结合位点相互作用。在DBH阴性细胞系中,Phox2a的强制表达能强力激活DBH启动子活性(>10倍),但在DBH阳性细胞系中仅使其略有增加(<50%)。此外,另一种具有相同HD的蛋白因子Phox2b也能以与Phox2a相当的效率激活DBH转录。相比之下,Phox2a和Phox2b都不能反式激活酪氨酸羟化酶转录,这表明这些转录因子对儿茶酚胺合成基因转录的激活具有差异性。结合Phox2a基因敲除实验,本文所述研究使Phox2a和Phox2b成为确定脊椎动物神经递质表型的首批强有力的候选转录因子。

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