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首页> 外文期刊>Molecular and cellular neurosciences >Differential display of genes expressed at the midbrain - hindbrain junction identifies sprouty2: an FGF8-inducible member of a family of intracellular FGF antagonists.
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Differential display of genes expressed at the midbrain - hindbrain junction identifies sprouty2: an FGF8-inducible member of a family of intracellular FGF antagonists.

机译:在中脑-后脑连接处表达的基因的差异显示可识别budpy2:细胞内FGF拮抗剂家族的FGF8诱导成员。

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摘要

Specification and polarization of the midbrain and anterior hindbrain involve planar signals originating from the isthmus. Current evidence suggests that FGF8, expressed at the isthmus, provides this patterning influence. In this study, we have sought to identify novel genes which are involved in the process by which regional identity is imparted to midbrain and anterior hindbrain (rhombomere 1). An enhanced differential display reverse transcription method was used to clone cDNAs derived from transcripts expressed specifically in either rhombomere 1 or midbrain during the period of isthmic patterning activity. This gene expression screen identified 28 differentially expressed cDNAs. A clone upregulated in cDNA derived from rhombomere 1 tissue showed a 91% identity at the nucleotide level to the putative human receptor tyrosine kinase antagonist: sprouty2. In situ hybridization on whole chick embryos showed chick sprouty2 to be expressed initially within the isthmus and rhombomere 1, spatially and temporally coincident with Fgf8 expression. However, at later stages this domain was more extensive than that of Fgf8. Introduction of ligand-coated beads into either midbrain or hindbrain region revealed that sprouty2 could be rapidly induced by FGF8. These data suggest that sprouty2 participates in a negative feedback regulatory loop to modulate the patterning activity of FGF8 at the isthmus. Copyright 2000 Academic Press.
机译:中脑和后脑的规格和极化涉及源自峡部的平面信号。当前证据表明,在峡部表达的FGF8提供了这种模式影响。在这项研究中,我们试图确定涉及中脑和后脑区域识别(rhombomere 1)的过程中涉及的新基因。使用增强的差异显示逆转录方法克隆了在等轴模式活动期间,在rhombomere 1或中脑中特异性表达的转录本衍生的cDNA。该基因表达筛选鉴定了28个差异表达的cDNA。在来自rhombomere 1组织的cDNA中上调的克隆在核苷酸水平上与假定的人类受体酪氨酸激酶拮抗剂:budy2具有91%的同一性。在整个雏鸡胚胎上的原位杂交显示,雏鸡发芽2最初在地峡和菱形1中表达,在空间和时间上与Fgf8表达一致。但是,在后期,该域比Fgf8的域更广泛。将配体包被的珠引入中脑或后脑区域显示出FGF8可以快速诱导出buddy2。这些数据表明,budmy2参与负反馈调节回路,以调节峡部FGF8的模式活动。版权所有2000学术出版社。

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