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利用合成生物学方法在细菌中重建植物泛素化级联反应。

Reconstitution of the plant ubiquitination cascade in bacteria using a synthetic biology approach.

机构信息

State Key Laboratory of Plant Genomics, Center for Agricultural Research Resources, Institute of Genetics and Developmental Biology, Chinese Academy of Sciences, Shijiazhuang, Hebei, 050021, China.

University of Chinese Academy of Sciences, Beijing, 100049, China.

出版信息

Plant J. 2017 Aug;91(4):766-776. doi: 10.1111/tpj.13603. Epub 2017 Jun 25.

DOI:10.1111/tpj.13603
PMID:28509348
Abstract

Ubiquitination modulates nearly all aspects of plant life. Here, we reconstituted the Arabidopsis thaliana ubiquitination cascade in Escherichia coli using a synthetic biology approach. In this system, plant proteins are expressed and then immediately participate in ubiquitination reactions within E. coli cells. Additionally, the purification of individual ubiquitination components prior to setting up the ubiquitination reactions is omitted. To establish the reconstituted system, we co-expressed Arabidopsis ubiquitin (Ub) and ubiquitination substrates with E1, E2 and E3 enzymes in E. coli using the Duet expression vectors. The functionality of the system was evaluated by examining the auto-ubiquitination of a RING (really interesting new gene)-type E3 ligase AIP2 and the ubiquitination of its substrate ABI3. Our results demonstrated the fidelity and specificity of this system. In addition, we applied this system to assess a subset of Arabidopsis E2s in Ub chain formation using E2 conjugation assays. Affinity-tagged Ub allowed efficient purification of Ub conjugates in milligram quantities. Consistent with previous reports, distinct roles of various E2s in Ub chain assembly were also observed in this bacterial system. Therefore, this reconstituted system has multiple advantages, and it can be used to screen for targets of E3 ligases or to study plant ubiquitination in detail.

摘要

泛素化调节植物生命的几乎所有方面。在这里,我们使用合成生物学方法在大肠杆菌中重新构建了拟南芥泛素化级联。在这个系统中,植物蛋白在大肠杆菌细胞内表达后立即参与泛素化反应。此外,在建立泛素化反应之前,省略了对单个泛素化成分的纯化。为了建立重组系统,我们使用 Duet 表达载体在大肠杆菌中共同表达拟南芥泛素 (Ub) 和泛素化底物与 E1、E2 和 E3 酶。通过检查 RING(真正有趣的新基因)型 E3 连接酶 AIP2 的自动泛素化及其底物 ABI3 的泛素化来评估该系统的功能。我们的结果证明了该系统的保真度和特异性。此外,我们还应用该系统通过 E2 缀合测定来评估拟南芥 E2 亚基在 Ub 链形成中的作用。亲和标签化的 Ub 允许以毫克级的量有效纯化 Ub 缀合物。与先前的报道一致,在这个细菌系统中也观察到各种 E2 在 Ub 链组装中的不同作用。因此,这个重组系统具有多种优势,可用于筛选 E3 连接酶的靶标或详细研究植物泛素化。

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