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DST序列在植物SAUR基因中高度保守,可靶向烟草中用于快速降解的报告转录本。

DST sequences, highly conserved among plant SAUR genes, target reporter transcripts for rapid decay in tobacco.

作者信息

Newman T C, Ohme-Takagi M, Taylor C B, Green P J

机构信息

Department of Energy Plant Research Laboratory, Michigan State University, East Lansing 48824-1312.

出版信息

Plant Cell. 1993 Jun;5(6):701-14. doi: 10.1105/tpc.5.6.701.

Abstract

DST elements are highly conserved sequences located in the 3' untranslated regions (UTRs) of a set of unstable soybean transcripts known as the small auxin-up RNAs (SAURs). To test whether DST sequences could function as mRNA instability determinants in plants, a model system was developed to facilitate the direct measurement of mRNA decay rates in stably transformed cells of tobacco. Initial experiments established that the chloramphenicol acetyltransferase (CAT) and beta-glucuronidase (GUS) transcripts degraded with similar half-lives in this system. In addition, their decay kinetics mirrored the apparent decay kinetics of the corresponding transcripts produced in transgenic plants under the control of a regulated promoter (Cab-1). The model system was then used to measure the decay rates of GUS reporter transcripts containing copies of the DST sequence inserted into the 3'UTR. An unmodified CAT gene introduced on the same vector served as the internal reference. These experiments and a parallel set utilizing a beta-globin reporter gene demonstrated that a synthetic dimer of the DST sequence was sufficient to destabilize both reporter transcripts in stably transformed tobacco cells. The decrease in transcript stability caused by the DST sequences in cultured cells was paralleled by a coordinate decrease in transcript abundance in transgenic tobacco plants. The implications of these results for the potential function of DST sequences within the SAUR transcripts are discussed.

摘要

DST元件是高度保守的序列,位于一组不稳定的大豆转录本的3'非翻译区(UTR),这些转录本被称为小生长素上调RNA(SAURs)。为了测试DST序列是否能作为植物中mRNA不稳定的决定因素,开发了一个模型系统,以方便直接测量烟草稳定转化细胞中mRNA的降解速率。初步实验表明,氯霉素乙酰转移酶(CAT)和β-葡萄糖醛酸酶(GUS)转录本在该系统中以相似的半衰期降解。此外,它们的降解动力学反映了在调控启动子(Cab-1)控制下转基因植物中产生的相应转录本的表观降解动力学。然后,该模型系统用于测量含有插入到3'UTR中的DST序列拷贝的GUS报告基因转录本的降解速率。同一载体上引入的未修饰的CAT基因用作内部对照。这些实验以及利用β-珠蛋白报告基因的平行实验表明,DST序列的合成二聚体足以使稳定转化的烟草细胞中的两种报告基因转录本不稳定。培养细胞中DST序列引起的转录本稳定性降低与转基因烟草植物中转录本丰度的相应降低平行。讨论了这些结果对SAUR转录本中DST序列潜在功能的影响。

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