首页> 美国卫生研究院文献>International Journal of Molecular Sciences >Cloning and Expression of Ecdysone Receptor and Retinoid X Receptor from Procambarus clarkii: Induction by Eyestalk Ablation
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Cloning and Expression of Ecdysone Receptor and Retinoid X Receptor from Procambarus clarkii: Induction by Eyestalk Ablation

机译:克氏原螯虾蜕皮激素受体和类维生素A X受体的克隆与表达:眼柄消融诱导

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摘要

Ecdysone receptor and retinoid X receptor are key regulators in molting. Here, full length ecdysone receptor (PcEcR) and retinoid X receptor (PcRXR) cDNAs from Procambarus clarkii were cloned. Full length cDNA of PcEcR has 2500 bp, encoding 576 amino acid proteins, and full length cDNA of PcRXR has 2593 bp, in which a 15 bp and a 204 bp insert/deletion splice variant regions in DNA binding domain and hinge domain were identified. The two splice variant regions in PcRXR result four isoforms: PcRXR1-4, encoding 525, 520, 457 and 452 amino acids respectively. PcEcR was highly expressed in the hepatopancreas and eyestalk and PcRXR was highly expressed in the eyestalk among eight examined tissues. Both PcEcR and PcRXR had induced expression after eyestalk ablation (ESA) in the three examined tissues. In muscle, PcEcR and PcRXR were upregulated after ESA, PcEcR reached the highest level on day 3 after ESA and increased 33.5-fold relative to day 0, and PcRXR reached highest the level on day 1 after ESA and increased 2.7-fold relative to day 0. In the hepatopancreas, PcEcR and PcRXR dEcReased continuously after ESA, and the expression levels of PcEcR and PcRXR were only 0.7% and 1.7% on day 7 after ESA relative to day 0, respectively. In the ovaries, PcEcR was upregulated after ESA, reached the highest level on day 3 after ESA, increased 3.0-fold relative to day 0, and the expression level of PcRXR changed insignificantly after ESA (p > 0.05). The different responses of PcEcR and PcRXR after ESA indicates that different tissues play different roles (and coordinates their functions) in molting.
机译:蜕皮激素受体和类维生素A X受体是蜕皮中的关键调节剂。在这里,克隆了来自克氏原螯虾的全长蜕皮激素受体(PcEcR)和类维生素A X受体(PcRXR)cDNA。 PcEcR的全长cDNA为2500 bp,编码576种氨基酸蛋白,PcRXR的全长cDNA为2593 bp,其中在DNA结合域和铰链域中鉴定出15 bp和204 bp的插入/缺失剪接变体区。 PcRXR中的两个剪接变体区域产生四个同工型:PcRXR1-4,分别编码525、520、457和452个氨基酸。在八种检查的组织中,PcEcR在肝胰腺和眼球中高表达,PcRXR在眼睑中高表达。 PcEcR和PcRXR都在三个受检组织的眼球消融(ESA)后诱导了表达。在肌肉中,ESA后PcEcR和PcRXR上调,PcEcR在ESA后第3天达到最高水平,相对于第0天增加33.5倍,PcRXR在ESA后第1天达到最高水平,并且相对于第2天增加2.7倍0.在ESA后,肝胰腺中PcEcR和 PcRXR d EcR 不断升高,而 PcEcR PcRXR 的表达水平相对于第0天,ESA后第7天的em>分别仅为0.7%和1.7%。在卵巢中, PcEcR 在ESA后上调,在ESA后第3天达到最高水平,相对于第0天增加了3.0倍,并且 PcRXR 的表达水平发生了变化在ESA之后微不足道( p PcEcR PcRXR 的不同反应表明,不同的组织在蜕皮中发挥不同的作用(并协调其功能)。

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