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通过反义RNA技术下调苜蓿谷氨酰胺合成酶基因家族特定成员的表达

Down-regulation of specific members of the glutamine synthetase gene family in alfalfa by antisense RNA technology.

作者信息

Temple S J, Bagga S, Sengupta-Gopalan C

机构信息

Department of Agronomy and Horticulture, New Mexico State University, Las Cruces 88003, USA.

出版信息

Plant Mol Biol. 1998 Jun;37(3):535-47. doi: 10.1023/a:1006099512706.

DOI:10.1023/a:1006099512706
PMID:9617820
Abstract

Glutamine synthetase (GS) catalyzes the ATP-dependent condensation of NH3 with glutamate to produce glutamine. In plants GS is an octameric enzyme and is located either in the cytoplasm (GS1) or in the chloroplast (GS2). Two distinct classes of GS1 genes with unique 3'-untranslated region (3'UTR) have been identified in alfalfa. We have demonstrated that the two classes exhibit differential expression pattern in the different plant organs suggesting different functional roles for the different isozymes. To determine the functional significance of the two classes of GS1 genes in alfalfa, we have utilized antisense gene constructs aimed specifically at the 3'UTR of the two GS1 genes and introduced them individually into alfalfa. Our data show that the gene constructs are effective in lowering the corresponding transcript level very effectively though there were organ-specific differences in the level of reduction. No transcript corresponding to the antisense gene construct was detected in any of the alfalfa transformants though they accumulated to significant levels in transgenic tobacco containing the same construct. This suggests that the antisense transcript was not stable in the presence of the homologous target sequence. Transgenic alfalfa with up to 80% reduction in the transcript level corresponding to each gene class, however, showed no reduction in GS activity or GS1 polypeptide level. The results suggest that GS1 mRNA levels are not rate-limiting for GS1 polypeptide synthesis and that GS levels are controlled both at the transcriptional and translational/post-translational level.

摘要

谷氨酰胺合成酶(GS)催化氨与谷氨酸在ATP依赖下缩合生成谷氨酰胺。在植物中,GS是一种八聚体酶,位于细胞质(GS1)或叶绿体(GS2)中。在苜蓿中已鉴定出两类具有独特3'非翻译区(3'UTR)的GS1基因。我们已经证明,这两类基因在不同植物器官中表现出不同的表达模式,表明不同的同工酶具有不同的功能作用。为了确定苜蓿中两类GS1基因的功能意义,我们利用了专门针对这两个GS1基因3'UTR的反义基因构建体,并将它们分别导入苜蓿。我们的数据表明,尽管在降低水平上存在器官特异性差异,但基因构建体能够非常有效地降低相应的转录水平。在任何苜蓿转化体中均未检测到与反义基因构建体对应的转录本,尽管它们在含有相同构建体的转基因烟草中积累到显著水平。这表明在同源靶序列存在的情况下,反义转录本不稳定。然而,对应于每个基因类别的转录水平降低高达80%的转基因苜蓿,其GS活性或GS1多肽水平并未降低。结果表明,GS1 mRNA水平不是GS1多肽合成的限速因素,并且GS水平在转录和翻译/翻译后水平均受到控制。

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