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本文引用的文献

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Establishment of an Experimental System for the Study of Tracheary Element Differentiation from Single Cells Isolated from the Mesophyll of Zinnia elegans.用于研究从百日草叶肉中分离的单个细胞的管状分子分化的实验系统的建立。
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Multiple gene detection by in situ RT-PCR in isolated plant cells and tissues.通过原位逆转录聚合酶链反应在分离的植物细胞和组织中进行多基因检测。
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Expansins abundant in secondary xylem belong to subgroup A of the alpha-expansin gene family.在次生木质部中大量存在的扩张蛋白属于α-扩张蛋白基因家族的A亚组。
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Signals that control plant vascular cell differentiation.控制植物维管细胞分化的信号。
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Impact of altered gibberellin metabolism on biomass accumulation, lignin biosynthesis, and photosynthesis in transgenic tobacco plants.赤霉素代谢改变对转基因烟草植株生物量积累、木质素生物合成及光合作用的影响
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XYLOGENESIS: INITIATION, PROGRESSION, AND CELL DEATH.木质部发生:起始、进程及细胞死亡
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Immunocytochemical localization of polygalacturonase during tracheary element differentiation in Zinnia elegans.百日草气管元件分化过程中多聚半乳糖醛酸酶的免疫细胞化学定位
Planta. 2004 Mar;218(5):729-39. doi: 10.1007/s00425-003-1167-4. Epub 2004 Jan 31.
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APL regulates vascular tissue identity in Arabidopsis.APL调控拟南芥中的维管组织特性。
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Transcriptional regulation of secondary growth in Arabidopsis thaliana.拟南芥次生生长的转录调控
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Cell differentiation, secondary cell-wall formation and transformation of callus tissue of Pinus radiata D. Don.辐射松愈伤组织的细胞分化、次生细胞壁形成及转化
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百日草中木质部发生的新型标志物受生长素和细胞分裂素的差异调节。

Novel markers of xylogenesis in zinnia are differentially regulated by auxin and cytokinin.

作者信息

Pesquet Edouard, Ranocha Philippe, Legay Sylvain, Digonnet Catherine, Barbier Odile, Pichon Magalie, Goffner Deborah

机构信息

Unité Mixte de Recherche, Centre National de la Recherche Scientifique/Université Paul Sabatier 5546, Surfaces Cellulaires et Signalisation chez les Végétaux, Pôle de Biotechnologie Végétale, 31326 Castanet, Tolosan, France.

出版信息

Plant Physiol. 2005 Dec;139(4):1821-39. doi: 10.1104/pp.105.064337. Epub 2005 Nov 23.

DOI:10.1104/pp.105.064337
PMID:16306148
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1310562/
Abstract

The characterization of in vitro xylogenic cultures of zinnia (Zinnia elegans) has led to major discoveries in the understanding of xylem formation in plants. We have constructed and characterized a subtractive library from zinnia cultures enriched in genes that are specifically expressed at the onset of secondary wall deposition and tracheary element (TE) programmed cell death. This Late Xylogenesis Library (LXL) consisted of 236 nonredundant cDNAs, 77% of which encoded novel sequences in comparison with the 17,622 expressed sequence tag sequences publicly available. cDNA arrays were constructed to examine dynamic global gene expression during the course of TE formation. As a first step in dissecting auxin and cytokinin signaling during TE differentiation, macroarrays were probed with cDNAs from cells cultured in different hormonal conditions. Fifty-one percent of the LXL genes were induced by either auxin or cytokinin individually, the large majority by auxin. To determine the potential involvement of these categories of genes in TE differentiation, multiplex in situ-reverse transcription-PCR was performed on cells for two genes encoding putative cell wall proteins: Gibberellin stimulated transcript-1, induced by auxin alone, and expansin 5, induced by cytokinin alone. All transcriptionally active TEs expressed both genes, indicating that, although these genes may not be considered as specific markers for TE differentiation per se, they are nevertheless an integral part of TE differentiation program. Among the non-TE population, four different gene expression-based cell types could be distinguished. Together, these results demonstrate the underlying complexity of hormonal perception and the existence of several different cell types in in vitro TE cell cultures.

摘要

百日草(Zinnia elegans)体外木质化培养的特性研究,在理解植物木质部形成方面取得了重大发现。我们构建并鉴定了一个来自百日草培养物的消减文库,该文库富含在次生壁沉积起始阶段和管状分子(TE)程序性细胞死亡时特异性表达的基因。这个晚期木质化文库(LXL)由236个非冗余cDNA组成,与公开可用的17,622个表达序列标签序列相比,其中77%编码新序列。构建cDNA阵列以检测TE形成过程中的动态全局基因表达。作为剖析TE分化过程中生长素和细胞分裂素信号传导的第一步,用来自不同激素条件下培养细胞的cDNA探测宏阵列。LXL基因中有51%分别由生长素或细胞分裂素单独诱导,其中绝大多数由生长素诱导。为了确定这些基因类别在TE分化中的潜在作用,对编码假定细胞壁蛋白的两个基因的细胞进行了多重原位逆转录PCR:仅由生长素诱导的赤霉素刺激转录本-1和仅由细胞分裂素诱导的扩张蛋白5。所有转录活性的TE都表达这两个基因,这表明,尽管这些基因本身可能不被视为TE分化的特异性标记,但它们仍然是TE分化程序的一个组成部分。在非TE群体中,可以区分出四种基于基因表达的不同细胞类型。总之,这些结果证明了激素感知的潜在复杂性以及体外TE细胞培养中存在几种不同的细胞类型。