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首页> 美国卫生研究院文献>Philosophical Transactions of the Royal Society B: Biological Sciences >Control of NF-kappa B transcriptional activation by signal induced proteolysis of I kappa B alpha.
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Control of NF-kappa B transcriptional activation by signal induced proteolysis of I kappa B alpha.

机译:通过信号诱导的IκB alpha的蛋白水解来控制NF-κB转录激活。

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In unstimulated cells the transcription factor NF-kappa B is held in the cytoplasm in an inactive state by I kappa B inhibitor proteins. Ultimately activation of NF-kappa B is achieved by ubiquitination and proteasome-mediated degradation of I kappa B alpha and we have therefore investigated factors which control this proteolysis. Signal-induced degradation of I kappa B alpha exposes the nuclear localization signal of NF-kappa B, thus allowing it to translocate into the nucleus and activate transcription from responsive genes. An autoregulatory loop is established when NF-kappa B induces expression of the I kappa B alpha gene and newly synthesized I kappa B alpha accumulates in the nucleus where it negatively regulates NF-kappa B-dependent transcription. As part of this post-induction repression, the nuclear export signal on I kappa B alpha mediates transport of NF-kappa B-I kappa B alpha complexes from the nucleus to the cytoplasm. As nuclear export of I kappa B alpha is blocked by leptomycin B this drug was used to examine the effect of cellular location on susceptibility of I kappa B alpha to signal-induced degradation. In the presence of leptomycin B, I kappa B alpha is accumulated in the nucleus and in this compartment is resistant to signal-induced degradation. Thus signal-induced degradation of I kappa B alpha is mainly, if not exclusively a cytoplasmic process. An efficient nuclear export of I kappa B alpha is therefore essential for maintaining a low level of I kappa B alpha in the nucleus and allowing NF-kappa B to be transcriptionally active upon cell stimulation. We have detected a modified form of I kappa B alpha, conjugated to the small ubiquitin-like protein SUMO-1, which is resistant to signal-induced degradation. SUMO-1 modified I kappa B alpha remains associated with NF-kappa B and thus overexpression of SUMO-1 inhibits the signal-induced activation of NF-kappa B-dependent transcription. Reconstitution of the conjugation reaction with highly purified proteins demonstrated that in the presence of a novel E1 SUMO-1 activating enzyme, Ubch9 directly conjugated SUMO-1 to I kappa B alpha on residues K21 and K22, which are also used for ubiquitin modification. Thus, while ubiquitination targets proteins for rapid degradation, SUMO-1 modification acts antagonistically to generate proteins resistant to degradation.
机译:在未刺激的细胞中,转录因子NF-κB被IκB抑制剂蛋白以非活性状态保持在细胞质中。 NF-κB的最终活化是通过泛素化和蛋白酶体介导的IκBα降解而实现的,因此我们研究了控制该蛋白水解的因素。信号诱导的IκBα降解会暴露NFκB的核定位信号,从而使其易位进入细胞核并激活响应基因的转录。当NF-κB诱导I-κBalpha基因表达并且新合成的I-κBalpha积累在细胞核中时,它会负调节NF-κB依赖性转录,从而建立自动调节环。作为该诱导后抑制的一部分,IκBα上的核输出信号介导了NF-κB-1κBα复合物从细胞核到细胞质的转运。由于瘦素B阻断了IκBα的核输出,因此该药物用于检查细胞位置对IκBα对信号诱导的降解的敏感性的影响。在存在细霉素B的情况下,IκBα积累在细胞核中,并且在该区室中抵抗信号诱导的降解。因此,信号诱导的IκBα降解主要是,如果不是排他的话,则主要是细胞质过程。因此,IκB alpha的有效核输出对于在细胞核中维持低水平的IκB alpha以及使NF-κB在细胞刺激后具有转录活性至关重要。我们已经检测到与小泛素样蛋白SUMO-1偶联的IκB alpha的修饰形式,该蛋白可抵抗信号诱导的降解。 SUMO-1修饰的IκB alpha仍与NF-κB相关,因此SUMO-1的过表达抑制了信号诱导的NF-κB依赖性转录的激活。用高度纯化的蛋白质重建结合反应表明,在新型E1 SUMO-1活化酶的存在下,Ubch9将SUMO-1直接与残基K21和K22上的IκBα偶联,后者也用于泛素修饰。因此,尽管泛素化将蛋白质靶向快速降解,但SUMO-1修饰却起着拮抗作用,以产生抗降解蛋白质。

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