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鸡δ1-和δ2-晶状体蛋白增强子在转基因小鼠中的晶状体优先活性以及视黄酸对δ1-晶状体蛋白基因响应性调控的证据。

Lens-preferred activity of chicken delta 1- and delta 2-crystallin enhancers in transgenic mice and evidence for retinoic acid-responsive regulation of the delta 1-crystallin gene.

作者信息

Li X, Cvekl A, Bassnett S, Piatigorsky J

机构信息

Laboratory of Molecular and Developmental Biology, National Eye Institute, National Institutes of Health, Bethesda, Maryland 20892-2730, USA.

出版信息

Dev Genet. 1997;20(3):258-66. doi: 10.1002/(SICI)1520-6408(1997)20:3<258::AID-DVG8>3.0.CO;2-6.

DOI:10.1002/(SICI)1520-6408(1997)20:3<258::AID-DVG8>3.0.CO;2-6
PMID:9216065
Abstract

There are two tandemly linked delta-crystallin genes [5' delta 1 -delta 2 3'] in the chicken, with the delta 1-crystallin gene being expressed much more highly (50-100-fold) in the embryonic lens than the delta 2-crystallin gene. Previous transfection experiments have shown that a lens-preferred enhancer exists in the third intron of each chicken delta-crystallin gene. In the present investigation we have used transgenic mice to establish that both the chicken delta 1- and delta 2-crystallin enhancers are preferentially active in the mouse lens in combination with their homologous promoter and the chloramphenicol acetyltransferase (CAT) reporter gene. The promoter/ CAT constructs lacking the enhancers were inactive in the transgenic mice. In one case, a truncated delta 2-crystallin promoter (-308/+24) in combination with the enhancer was also active in the Purkinje cells of the cerebellum of the transgenic mice, which could prove useful in future experiments. Finally, retinoic acid receptors (RAR beta) activated the delta 1-crystallin, but not the delta 2-crystallin enhancer in teh recombinant plasmids in cotransfected embryonic chicken lens epithelial cells treated with retinoic acid. This activation did not occur when using the care enhancer (fragment B4) lacking surrounding flanking sequences (fragment B3 and B5) of the enhancer. Together these experiments show that the chicken delta-crystallin enhancers show lens-preference in transgenic mice despite the absence of delta-crystallin in this species and add retinoic acid nuclear receptors to the growing list of transcription factors (including Pax-6, Sox-2, and delta EF3) that directly or indirectly contribute to the high expression of the delta 1-crystallin gene in the lens.

摘要

鸡体内有两个串联连接的δ-晶体蛋白基因[5'δ1-δ2 3'],其中δ1-晶体蛋白基因在胚胎晶状体中的表达水平比δ2-晶体蛋白基因高得多(50-100倍)。先前的转染实验表明,每个鸡δ-晶体蛋白基因的第三个内含子中存在一个晶状体偏好性增强子。在本研究中,我们利用转基因小鼠证实,鸡δ1-和δ2-晶体蛋白增强子与它们的同源启动子和氯霉素乙酰转移酶(CAT)报告基因结合时,在小鼠晶状体中具有优先活性。缺乏增强子的启动子/CAT构建体在转基因小鼠中无活性。在一个案例中,一个截短的δ2-晶体蛋白启动子(-308/+24)与增强子结合时,在转基因小鼠小脑的浦肯野细胞中也具有活性,这在未来的实验中可能会有用。最后,在用视黄酸处理的共转染胚胎鸡晶状体上皮细胞中,视黄酸受体(RARβ)激活了重组质粒中的δ1-晶体蛋白增强子,但未激活δ2-晶体蛋白增强子。当使用缺乏增强子周围侧翼序列(片段B3和B5)的对照增强子(片段B4)时,这种激活并未发生。这些实验共同表明,尽管该物种中不存在δ-晶体蛋白,但鸡δ-晶体蛋白增强子在转基因小鼠中表现出晶状体偏好性,并将视黄酸核受体添加到越来越多的直接或间接导致δ1-晶体蛋白基因在晶状体中高表达的转录因子(包括Pax-6、Sox-2和δEF3)列表中。

相似文献

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Lens-preferred activity of chicken delta 1- and delta 2-crystallin enhancers in transgenic mice and evidence for retinoic acid-responsive regulation of the delta 1-crystallin gene.鸡δ1-和δ2-晶状体蛋白增强子在转基因小鼠中的晶状体优先活性以及视黄酸对δ1-晶状体蛋白基因响应性调控的证据。
Dev Genet. 1997;20(3):258-66. doi: 10.1002/(SICI)1520-6408(1997)20:3<258::AID-DVG8>3.0.CO;2-6.
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Lens-specific activity of the chicken delta 1-crystallin enhancer in the mouse.鸡δ1-晶体蛋白增强子在小鼠中的晶状体特异性活性。
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Chick delta1-crystallin enhancer influences mouse alphaA-crystallin promoter activity in transgenic mice.鸡δ1-晶体蛋白增强子影响转基因小鼠中鼠αA-晶体蛋白启动子的活性。
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Lens protein gene expression: alpha-crystallins and MIP.晶状体蛋白基因表达:α-晶体蛋白和MIP
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Differential expression of the two delta-crystallin/argininosuccinate lyase genes in lens, heart, and brain of chicken embryos.鸡胚晶状体、心脏和大脑中两种δ-晶体蛋白/精氨琥珀酸裂解酶基因的差异表达。
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A complex enhancer of the chicken beta A3/A1-crystallin gene depends on an AP-1-CRE element for activity.鸡βA3/A1-晶体蛋白基因的一个复杂增强子的活性依赖于一个AP-1-CRE元件。
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