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首页> 外文期刊>BMC Developmental Biology >Analysis of the Rana catesbeiana tadpole tail fin proteome and phosphoproteome during T3-induced apoptosis: identification of a novel type I keratin
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Analysis of the Rana catesbeiana tadpole tail fin proteome and phosphoproteome during T3-induced apoptosis: identification of a novel type I keratin

机译:T3诱导细胞凋亡过程中的牛蛙ana尾鳍蛋白质组和磷酸化蛋白质组的分析:新型I型角蛋白的鉴定。

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Background Thyroid hormones (THs) are vital in the maintenance of homeostasis and in the control of development. One postembryonic developmental process that is principally regulated by THs is amphibian metamorphosis. This process has been intensively studied at the genomic level yet very little information at the proteomic level exists. In addition, there is increasing evidence that changes in the phosphoproteome influence TH action. Results Here we identify components of the proteome and phosphoproteome in the tail fin that changed within 48 h of exposure of premetamorphic Rana catesbeiana tadpoles to 10 nM 3,5,3'-triiodothyronine (T3). To this end, we developed a cell and protein fractionation method combined with two-dimensional gel electrophoresis and phosphoprotein-specific staining. Altered proteins were identified using mass spectrometry (MS). We identified and cloned a novel Rana larval type I keratin, RLK I, which may be a target for caspase-mediated proteolysis upon exposure to T3. In addition, the RLK I transcript is reduced during T3-induced and natural metamorphosis which is consistent with a larval keratin. Furthermore, GILT, a protein involved in the immune system, is changed in phosphorylation state which is linked to its activation. Using a complementary MS technique for the analysis of differentially-expressed proteins, isobaric tags for relative and absolute quantitation (iTRAQ) revealed 15 additional proteins whose levels were altered upon T3 treatment. The success of identifying proteins whose levels changed upon T3 treatment with iTRAQ was enhanced through de novo sequencing of MS data and homology database searching. These proteins are involved in apoptosis, extracellular matrix structure, immune system, metabolism, mechanical function, and oxygen transport. Conclusion We have demonstrated the ability to derive proteomics-based information from a model species for postembryonic development for which no genome information is currently available. The present study identifies proteins whose levels and/or phosphorylation states are altered within 48 h of the induction of tadpole tail regression prior to overt remodeling of the tail. In particular, we have identified a novel keratin that is a target for T3-mediated changes in the tail that can serve as an indicator of early response to this hormone.
机译:背景甲状腺激素(THs)在维持体内平衡和控制发育中至关重要。一种主要受THs调控的胚后发育过程是两栖动物变态。这个过程已经在基因组水平上进行了深入研究,但在蛋白质组学水平上却很少有信息。此外,越来越多的证据表明磷酸化蛋白质组的变化会影响TH的作用。结果在这里,我们确定了在变态的蛙蛙(Rana catesbeiana)48暴露于10 nM 3,5,3'-triiodothyronine(T 3 )48小时内,尾鳍中的蛋白质组和磷酸化蛋白质组的成分发生了变化。为此,我们开发了一种结合二维凝胶电泳和磷蛋白特异性染色的细胞和蛋白质分级分离方法。使用质谱(MS)鉴定出改变的蛋白质。我们鉴定并克隆了一种新型的Rana幼虫I型角蛋白RLK I,它可能是半胱天冬酶介导的T 3 介导蛋白水解的靶标。此外,在T 3 诱导的自然变态过程中,RLK I转录物减少,这与幼虫角蛋白一致。此外,GILT(一种参与免疫系统的蛋白质)的磷酸化状态发生了变化,这与其激活有关。使用互补质谱技术分析差异表达的蛋白质时,同量异位标记用于相对定量和绝对定量(iTRAQ)发现了另外15种蛋白质,其水平在T 3 处理后发生了变化。通过对MS数据进行从头测序和同源数据库搜索,提高了鉴定用iTRAQ进行T 3 处理后水平发生变化的蛋白质的成功。这些蛋白质参与细胞凋亡,细胞外基质结构,免疫系统,新陈代谢,机械功能和氧气转运。结论我们已经证明了从模型种中获得基于蛋白质组学信息的能力,用于胚胎后发育,目前尚无基因组信息。本研究鉴定了在over的明显重塑之前the诱导的48h内其水平和/或磷酸化状态发生改变的蛋白质。特别是,我们确定了一种新型角蛋白,它是T 3 介导的尾巴变化的靶标,可作为对此激素早期反应的指标。

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