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Pin1 and JNK1 cooperatively modulate TAp63γ

机译:PIN1和JNK1协同调制Tap63γ

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摘要

The p63 gene encodes at least 10 isoforms, which can be classified into TA and ∆N isotypes (TAp63 and ∆Np63 proteins) according to their differences at the N termini. TAp63γ is an important transcription factor. We previously reported that peptidyl‐prolyl isomerase (PPI) Pin1 directly binds to TAp63γ protein and identified that serine 12 (S12) in the transactivation domain (TAD) of TAp63γ is required for regulation of its transcriptional activity. In the present study, we report that Pin1 stimulates transcriptional and pro‐apoptotic activities of TAp63γ; this Pin1‐mediated stimulation may depend on phosphorylation of S12 mediated by JNK1 and results in striking activation of TAp63γ. JNK1 represses transactivity of TAp63γ in cells without abundant Pin1 proteins and enhances it in the presence of sufficient levels of Pin1. Collectively, our data suggest a novel mechanism for regulation of TAp63γ transactivity: TAp63γ with unphosphorylated S12 is moderately active, phosphorylation at this residue (pS12) makes it hypoactive, and Pin1 binds to the pS12‐P13 motif and makes TAp63γ hyperactive. Our findings will aid in the elucidation of the mechanism underlying modulation of TAp63γ.
机译:P63基因编码至少10种同种型,其可以根据它们在N Termini的差异分类为Ta和Δn同种型(Tap63和Δnp63蛋白)。 Tap63γ是一个重要的转录因子。我们之前报道的是,肽基 - 脯氨酰异构酶(PPI)PIN1直接与Tap63γ蛋白结合,并鉴定了Tap63γ的转移结构域(TAD)中的丝氨酸12(S12)来调节其转录活性。在本研究中,我们报告了P​​in1刺激了Tap63γ的转录和促凋亡活动;该PIN1介导的刺激可取决于由JNK1介导的S12的磷酸化,并导致TAP63γ的醒目激活。 JNK1在没有丰富的Pin1蛋白的细胞中抑制TIP63γ的交流,并在足够水平的PIN1的存在下增强它。统称,我们的数据表明了一种新的Tap63γ交流的调节机制:具有不磷酸化的S12的Tap63γ是适度的活性的,在该残基(PS12)处的磷酸化使得HIN1与PS12-P13基序结合并使TAP63γ过度结合。我们的研究结果将有助于阐明TAP63γ的潜在调节机制。

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