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Characterization of glucocorticoid-induced changes in gene expression in the embryonic pituitary gland.

机译:糖皮质激素诱导的胚胎垂体基因表达变化的表征。

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We have previously shown that corticosterone (CORT) can induce premature differentiation of somatotrophs in the chicken embryo. CORT induction of GH mRNA is indirect, in that protein synthesis inhibition blocks its inducing effect. In this study, we used a custom chicken microarray to analyze global gene expression in the embryonic pituitary gland and to identify potential direct targets of CORT that may regulate its induction of somatotroph differentiation. Dispersed embryonic (e) day 11 pituitary cells were pretreated with cycloheximide then with CORT or treated with CORT alone for 24 hrs. Amplified RNA from these samples was then used on our microarray to analyze gene expression and in quantitative real-time PCR (qRT-PCR) analysis to determine relative gene expression levels. qRT-PCR from these samples showed that GH was induced within 1.5 hrs and continued to significantly increase until 3 hrs. Our microarray analysis revealed 25 direct early targets of CORT. From these 25 we chose 3 genes, Dexras1, Ras-dva, and Prostaglandin-D Synthase to transfect into e11 pituitary cells and measure their effect on GH mRNA. Neither of these genes had a direct effect on GH mRNA; however Dexras1 acted synergistically with CORT to induce GH mRNA. Dexras1 was discovered in murine AtT-20 corticotroph cells because its expression was rapidly induced in response to glucocorticoids. We report here a chicken Dexras1 cDNA that is 1631 by in length and encodes a protein of 278 amino acid residues. Comparison of the consensus chicken Dexras1 amino and nucleic acid sequence with those of human, mouse, and rat Dexras1 showed high homology among the species. Expression of Dexras1 mRNA was detected in various tissues by Northern analysis, but was highest in the pituitary. RT-PCR analysis showed expression of Dexras1 only in the pituitary. The precise role of DexRas1 is unidentified at the present time; however, its distribution in a range of tissues suggests a possible role in glucocorticoid action within a variety of systems.
机译:先前我们已经表明,皮质酮(CORT)可以诱导鸡胚中的营养体过早分化。 GH mRNA的CORT诱导是间接的,因为蛋白质合成抑制作用会阻断其诱导作用。在这项研究中,我们使用了定制的鸡微阵列来分析胚胎垂体中的整体基因表达,并确定可能调节CORT诱导体细胞营养分化的潜在直接靶标。将分散的胚胎(e)第11天垂体细胞先用环己酰亚胺预处理,然后再用CORT预处理,或者单独用CORT处理24小时。然后将这些样品中扩增出的RNA用于我们的微阵列上以分析基因表达,并用于定量实时PCR(qRT-PCR)分析以确定相对基因表达水平。这些样品的qRT-PCR显示GH在1.5小时内被诱导,并持续显着增加直至3小时。我们的微阵列分析揭示了CORT的25个直接早期靶标。从这25个基因中,我们选择3个基因Dexras1,Ras-dva和Prostaglandin-D合酶转染到e11垂体细胞中,并测量它们对GH mRNA的作用。这些基因均未直接影响GH mRNA。然而Dexras1与CORT协同作用诱导GH mRNA。 Dexras1是在鼠AtT-20皮质营养细胞中发现的,因为它的表达是响应糖皮质激素而迅速诱导的。我们在这里报告了鸡Dexras1 cDNA,长度为1631,编码278个氨基酸残基的蛋白质。共有鸡Dexras1的氨基酸和核酸序列与人,小鼠和大鼠Dexras1的氨基酸和核酸序列的比较显示出物种之间的高度同源性。通过Northern分析在各种组织中检测到Dexras1 mRNA的表达,但在垂体中最高。 RT-PCR分析显示Dexras1仅在垂体中表达。目前尚不清楚DexRas1的确切作用;然而,它在一系列组织中的分布表明在多种系统中糖皮质激素作用中可能发挥作用。

著录项

  • 作者

    Jenkins, Sultan Ali.;

  • 作者单位

    University of Maryland, College Park.;

  • 授予单位 University of Maryland, College Park.;
  • 学科 Biology Molecular.; Biology Animal Physiology.; Biology Zoology.; Agriculture Animal Culture and Nutrition.
  • 学位 Ph.D.
  • 年度 2006
  • 页码 137 p.
  • 总页数 137
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 分子遗传学;生理学;动物学;饲料;
  • 关键词

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