Enhancement of secondary xylem cell proliferation by Arabidopsiscyclin D overexpression in tobacco plants

被引:0
|
作者
Takeo Fujii
Kanna Sato
Noriko Matsui
Takayuki Furuichi
Sachi Takenouchi
Nobuyuki Nishikubo
Yuzo Suzuki
Shinya Kawai
Taku Demura
Shinya Kajita
Yoshihiro Katayama
机构
[1] Graduate School of Bio-Applications and Systems Engineering,
[2] Tokyo University of Agriculture and Technology,undefined
[3] Graduate School of Agriculture,undefined
[4] Tokyo University of Agriculture and Technology,undefined
[5] Nara Institute of Science and Technology,undefined
[6] Plant Science Center,undefined
[7] RIKEN,undefined
[8] College of Bioresource Sciences,undefined
[9] Nihon University,undefined
[10] Forestry Research Institute,undefined
[11] Oji Paper Company Limited,undefined
来源
Plant Cell Reports | 2012年 / 31卷
关键词
Cell cycle; Cell division; Secondary xylem; Vascular cambium;
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暂无
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学科分类号
摘要
Secondary xylem is composed of daughter cells produced by the vascular cambium in the stem. Cell proliferation of the secondary xylem is the result of long-range cell division in the vascular cambium. Most xylem cells have a thickened secondary cell wall, representing a large amount of biomass storage. Therefore, regulation of cell division in the vascular cambium and differentiation into secondary xylem is important for biomass production. Cell division is regulated by cell cycle regulators. In this study, we confirm that cell cycle regulators influence cell division in the vascular cambium in tobacco. We produced transgenic tobacco that expresses Arabidopsis thaliana cyclin D2;1 (AtcycD2;1) and AtE2Fa–DPa under the control of the CaMV35S promoter. Each gene is a positive regulator of the cell cycle, and is known to influence the transition from G1 phase to S phase. AtcycD2;1-overexpressing tobacco had more secondary xylem cells when compared with control plants. In order to evaluate cell division activity in the vascular cambium, we prepared a Populus trichocarpacycB1;1 (PtcycB1;1) promoter containing a destruction box motif for ubiquitination and a β-glucuronidase-encoding gene (PtcycB1;1pro:GUS). In transgenic tobacco containing PtcycB1;1pro:GUS, GUS staining was specifically observed in meristem tissues, such as the root apical meristem and vascular cambium. In addition, mitosis-monitoring plants containing AtcycD2;1 had stronger GUS staining in the cambium when compared with control plants. Our results indicated that overexpression of AtcycD enhances cell division in the vascular cambium and increases secondary xylem differentiation in tobacco.
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页码:1573 / 1580
页数:7
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