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Brn3a和Nurr1介导缰核发育的基因调控途径。

Brn3a and Nurr1 mediate a gene regulatory pathway for habenula development.

作者信息

Quina Lely A, Wang Shirong, Ng Lydia, Turner Eric E

机构信息

Department of Psychiatry, University of California, San Diego, La Jolla, California 92093-0603, USA.

出版信息

J Neurosci. 2009 Nov 11;29(45):14309-22. doi: 10.1523/JNEUROSCI.2430-09.2009.

Abstract

The habenula is a dorsal diencephalic structure consisting of medial and lateral subnuclei and a principal output tract, the fasciculus retroflexus, which together form a link between the limbic forebrain and ventral midbrain. Here, we have used microarray and bioinformatic approaches in the mouse to show that the habenula is a distinctive molecular territory of the CNS, with a unique profile of neurotransmitter, ion channel, and regulatory factor expression. Neurons of the medial habenula and part of the lateral habenula express the transcription factor Brn3a/Pou4f1, and Brn3a-expressing habenular neurons project exclusively to the interpeduncular nucleus in the ventral midbrain. In Brn3a mutant embryos, the fasciculus retroflexus is directed appropriately, but habenular neurons fail to innervate their targets. Microarray analysis of Brn3a null embryos shows that this factor regulates an extensive program of habenula-enriched genes, but not generic neural properties. The orphan nuclear receptor Nurr1/Nr4a2 is coexpressed with Brn3a in the developing habenula, is downstream of Brn3a, and mediates expression of a subset of Brn3a-regulated transcripts. Together, these findings begin to define a gene regulatory pathway for habenula development in mammals.

摘要

缰核是间脑背侧的一个结构,由内侧和外侧亚核以及一条主要输出通路——后屈束组成,它们共同构成了边缘前脑和腹侧中脑之间的一个连接。在此,我们利用小鼠的微阵列和生物信息学方法表明,缰核是中枢神经系统中一个独特的分子区域,具有独特的神经递质、离子通道和调节因子表达谱。内侧缰核和部分外侧缰核的神经元表达转录因子Brn3a/Pou4f1,且表达Brn3a的缰核神经元仅投射至腹侧中脑的脚间核。在Brn3a突变胚胎中,后屈束的走向正常,但缰核神经元无法支配其靶标。对Brn3a基因敲除胚胎的微阵列分析表明,该因子调控着大量缰核富集基因的表达程序,但不调控一般的神经特性。孤儿核受体Nurr1/Nr4a2在发育中的缰核中与Brn3a共表达,位于Brn3a下游,并介导Brn3a调控转录本的一个子集的表达。总之,这些发现开始确定哺乳动物缰核发育的基因调控途径。

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