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首页> 外文期刊>The New Phytologist >TIR-NB-LRR immune receptor SOC3 pairs with truncated TIR-NB protein CHS1 or TN2 to monitor the homeostasis of E3 ligase SAUL1
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TIR-NB-LRR immune receptor SOC3 pairs with truncated TIR-NB protein CHS1 or TN2 to monitor the homeostasis of E3 ligase SAUL1

机译:TiR-NB-LRR免疫受体SOC3对具有截短的TIR-NB蛋白CHS1或TN2,监测E3连接酶SAUL1的稳态

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摘要

Intracellular nucleotide binding (NB) and leucine-rich repeat (NLR) proteins function as immune receptors to recognize effectors from pathogens. They often guard host proteins that are the direct targets of those effectors. Recent findings have revealed that a typical NLR sometimes cooperates with another atypical NLR for effector recognition. Here, by using the CRISPR/Cas9 gene editing method, knockout analysis and biochemical assays, we uncovered differential pairings of typical Toll Interleukin1 receptor (TIR) type NLR (TNL) receptor SOC3 with atypical truncated TIR-NB (TN) proteins CHS1 or TN2 to guard the homeostasis of the E3 ligase SAUL1. Overaccumulation of SAUL1 is monitored by the SOC3-TN2 pair, while SAUL1's disappearance is guarded by the SOC3-CHS1 pair. SOC3 forms a head-to-head genomic arrangement with CHS1 and TN2, indicative of transcriptional co-regulation. Such intricate cooperative interactions can probably enlarge the recognition spectrum and increase the functional flexibility of NLRs, which can partly explain the overwhelming occurrence of NLR gene clustering in higher plants.
机译:细胞内核苷酸结合(Nb)和富含亮氨酸的重复(NLR)蛋白质作为免疫受体来识别来自病原体的效果。他们经常守护宿主蛋白,这些蛋白质是这些效果的直接目标。最近的发现表明,典型的NLR有时与另一个非典型NLR合作,用于效应识别。这里,通过使用CRISPR / CAS9基因编辑方法,敲除分析和生物化学测定,我们发现典型的Toll白细胞介素1受体(TIR)型NLR(TNL)受体SOC3的差异配对与非典型截短的TIR-NB(TN)蛋白CHS1或TN2保护E3 Ligase Saul1的稳态。 SOC3-TN2对监测SAUL1的过度累积,而SOUL1的消失由SOC3-CHS1对保护。 SOC3与CHS1和TN2形成头部到头基因组排列,指示转录共调序。这种复杂的协作相互作用可能会扩大识别谱并提高NLR的功能灵活性,其可以部分解释高等植物中NLR基因聚类的压倒性发生。

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