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表达针对L-半乳糖酸-1,4-内酯脱氢酶的反义RNA的抗坏血酸缺陷型转基因烟草细胞的生成及特性

Generation and properties of ascorbic acid-deficient transgenic tobacco cells expressing antisense RNA for L-galactono-1,4-lactone dehydrogenase.

作者信息

Tabata K, Oba K, Suzuki K, Esaka M

机构信息

Faculty of Applied Biological Science, Hiroshima University, Kagamiyama, Higashi-Hiroshima, 739-8528 Japan.

出版信息

Plant J. 2001 Jul;27(2):139-48. doi: 10.1046/j.1365-313x.2001.01074.x.

Abstract

In higher plants, the terminal step of L-ascorbic acid (AsA) biosynthesis is catalyzed by the enzyme L-galactono-1,4-lactone dehydrogenase (EC 1.3.2.3, GalLDH). We generated AsA-deficient transgenic tobacco BY-2 cell lines by antisense expression of the GalLDH cDNA that was amplified from BY-2 cells using PCR. Two transgenic cell-lines, AS1-1 and AS2-2, having a marked expression of antisense RNA were analyzed. Antisense suppression of GalLDH mRNA led to a significant decline in the GalLDH activity. The AsA levels in the transgenic cell lines were found to be 30% lower than the wild-type BY-2 cells. In synchronous cultures, division of AS1-1 and AS2-2 cells was restrained with a concomitant decrease in mitotic index that was probably due to a decline in AsA levels. The rate of cell growth was also found to be less than that of the wild-type cells. Interestingly, there was a significant phenotypic difference between the transgenic and wild-type cells. The calli of AS1-1 and AS2-2 appeared to be sticky and soft. Back extrusion method also showed that AsA-deficient BY-2 callus was rheologically soft. Furthermore, microscopic analysis revealed that AS1-1 and AS2-2 cells were abnormally slender, suggesting a potential for a significant and a uni-axial elongation. Thus, we observed that decline in the AsA levels has an adverse effect on the division, growth and structure of a plant cell.

摘要

在高等植物中,L-抗坏血酸(AsA)生物合成的最后一步由L-半乳糖-1,4-内酯脱氢酶(EC 1.3.2.3,GalLDH)催化。我们通过使用PCR从BY-2细胞中扩增出的GalLDH cDNA的反义表达,生成了AsA缺陷型转基因烟草BY-2细胞系。分析了两个反义RNA有明显表达的转基因细胞系AS1-1和AS2-2。GalLDH mRNA的反义抑制导致GalLDH活性显著下降。发现转基因细胞系中的AsA水平比野生型BY-2细胞低30%。在同步培养中,AS1-1和AS2-2细胞的分裂受到抑制,同时有丝分裂指数下降,这可能是由于AsA水平下降所致。细胞生长速率也低于野生型细胞。有趣的是,转基因细胞和野生型细胞之间存在显著的表型差异。AS1-1和AS2-2的愈伤组织显得黏软。回挤法也表明AsA缺陷的BY-2愈伤组织在流变学上较软。此外,显微镜分析显示AS1-1和AS2-2细胞异常细长,表示有显著的单轴伸长潜力。因此,我们观察到AsA水平下降对植物细胞的分裂、生长和结构有不利影响。

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