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拟南芥无细胞提取物,ACE,一种源自拟南芥愈伤组织培养的新型体外翻译系统。

Arabidopsis cell-free extract, ACE, a new in vitro translation system derived from Arabidopsis callus cultures.

机构信息

Division of Applied Bioscience, Graduate School of Agriculture, Hokkaido University, Sapporo, 060-8589 Japan.

出版信息

Plant Cell Physiol. 2011 Aug;52(8):1443-53. doi: 10.1093/pcp/pcr080. Epub 2011 Jun 15.

DOI:10.1093/pcp/pcr080
PMID:21677046
Abstract

The analysis of post-transcriptional regulatory mechanisms in plants has benefited greatly from the use of cell-free extract systems. Arabidopsis as a model system provides extensive genetic resources; however, to date a suitable cell-free translation system from Arabidopsis has not been available. In this study, we devised an Arabidopsis cell-free extract (ACE) to be used for in vitro translation studies. Protoplasts were prepared from callus cultures derived from Arabidopsis seedlings, and cell-free extracts were prepared after evacuolation of the protoplasts by Percoll gradient centrifugation. The new ACE system exhibits translation activity comparable with that of the wheat germ extract system. We demonstrated that ACE prepared from the 5'-3' exoribonuclease-deficient mutant of Arabidopsis, xrn4-5, exhibited increased stability of an uncapped mRNA as compared with that from wild-type Arabidopsis. We applied the ACE system to study post-transcriptional regulation of AtCGS1. AtCGS1 codes for cystathionine γ-synthase (CGS) that catalyzes the first committed step of methionine and S-adenosyl-l-methionine (AdoMet) biosynthesis in plants, and is feedback regulated by mRNA degradation coupled with translation elongation arrest. The ACE system was capable of reproducing translation elongation arrest and subsequent AtCGS1 mRNA degradation that are induced by AdoMet. The ACE system described here can be prepared in a month after seed sowing and will make it possible to study post-transcriptional regulation of plant genes while taking advantage of the genetics of Arabidopsis.

摘要

植物转录后调控机制的分析得益于无细胞提取系统的应用。拟南芥作为一种模式系统提供了广泛的遗传资源;然而,到目前为止,还没有适合的拟南芥无细胞翻译系统。在本研究中,我们设计了一种拟南芥无细胞提取物(ACE)用于体外翻译研究。从拟南芥幼苗的愈伤组织中制备原生质体,并用聚蔗糖梯度离心排空原生质体后制备无细胞提取物。新的 ACE 系统表现出与小麦胚乳提取物系统相当的翻译活性。我们证明,与来自野生型拟南芥的 ACE 相比,来自拟南芥 5'-3'外切核酸酶缺陷突变体 xrn4-5 的 ACE 显示出未加帽 mRNA 的稳定性增加。我们应用 ACE 系统研究 AtCGS1 的转录后调控。AtCGS1 编码半胱氨酸γ-合酶(CGS),它在植物中催化甲硫氨酸和 S-腺苷甲硫氨酸(AdoMet)生物合成的第一个关键步骤,并且通过与翻译延伸阻滞偶联的 mRNA 降解进行反馈调节。ACE 系统能够重现由 AdoMet 诱导的翻译延伸阻滞和随后的 AtCGS1 mRNA 降解。这里描述的 ACE 系统可以在播种后一个月内制备,这将使研究植物基因的转录后调控成为可能,同时利用拟南芥的遗传学。

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