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本文引用的文献

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Conversion of a putative Agrobacterium sugar-binding protein into a FRET sensor with high selectivity for sucrose.将一种假定的农杆菌糖结合蛋白转化为对蔗糖具有高选择性的荧光共振能量转移(FRET)传感器。
J Biol Chem. 2006 Oct 13;281(41):30875-83. doi: 10.1074/jbc.M605257200. Epub 2006 Aug 15.
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Sugar sensing and signaling in plants: conserved and novel mechanisms.植物中的糖感知与信号传导:保守机制与新机制
Annu Rev Plant Biol. 2006;57:675-709. doi: 10.1146/annurev.arplant.57.032905.105441.
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Direct evidence for a sugar transport mechanism in isolated vacuoles.分离液泡中糖转运机制的直接证据。
Plant Physiol. 1979 Jul;64(1):61-4. doi: 10.1104/pp.64.1.61.
4
CO(2) signaling in guard cells: calcium sensitivity response modulation, a Ca(2+)-independent phase, and CO(2) insensitivity of the gca2 mutant.保卫细胞中的二氧化碳信号传导:钙敏感性反应调节、一个不依赖钙离子的阶段以及gca2突变体的二氧化碳不敏感性
Proc Natl Acad Sci U S A. 2006 May 9;103(19):7506-11. doi: 10.1073/pnas.0602225103. Epub 2006 May 1.
5
Identification of a vacuolar sucrose transporter in barley and Arabidopsis mesophyll cells by a tonoplast proteomic approach.通过液泡膜蛋白质组学方法鉴定大麦和拟南芥叶肉细胞中的液泡蔗糖转运蛋白。
Plant Physiol. 2006 May;141(1):196-207. doi: 10.1104/pp.106.079533. Epub 2006 Mar 31.
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Glucose signaling in Saccharomyces cerevisiae.酿酒酵母中的葡萄糖信号传导
Microbiol Mol Biol Rev. 2006 Mar;70(1):253-82. doi: 10.1128/MMBR.70.1.253-282.2006.
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Using intrinsically fluorescent proteins for plant cell imaging.利用内在荧光蛋白进行植物细胞成像。
Plant J. 2006 Feb;45(4):599-615. doi: 10.1111/j.1365-313X.2006.02658.x.
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Evidence for high-capacity bidirectional glucose transport across the endoplasmic reticulum membrane by genetically encoded fluorescence resonance energy transfer nanosensors.通过基因编码的荧光共振能量转移纳米传感器证明内质网膜存在高容量双向葡萄糖转运。
Mol Cell Biol. 2005 Dec;25(24):11102-12. doi: 10.1128/MCB.25.24.11102-11112.2005.
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Changes in flux pattern of the central carbohydrate metabolism during kernel development in maize.玉米籽粒发育过程中中心碳水化合物代谢通量模式的变化
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Shining light on signaling and metabolic networks by genetically encoded biosensors.利用基因编码生物传感器揭示信号传导和代谢网络
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利用荧光共振能量转移(FRET)葡萄糖纳米传感器在拟南芥RNA沉默突变体的表皮细胞和完整根中检测到葡萄糖的快速代谢。

Rapid metabolism of glucose detected with FRET glucose nanosensors in epidermal cells and intact roots of Arabidopsis RNA-silencing mutants.

作者信息

Deuschle Karen, Chaudhuri Bhavna, Okumoto Sakiko, Lager Ida, Lalonde Sylvie, Frommer Wolf B

机构信息

Department of Plant Biology, Carnegie Institution, Stanford, California 94305, USA.

出版信息

Plant Cell. 2006 Sep;18(9):2314-25. doi: 10.1105/tpc.106.044073. Epub 2006 Aug 25.

DOI:10.1105/tpc.106.044073
PMID:16935985
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1560921/
Abstract

Genetically encoded glucose nanosensors have been used to measure steady state glucose levels in mammalian cytosol, nuclei, and endoplasmic reticulum. Unfortunately, the same nanosensors in Arabidopsis thaliana transformants manifested transgene silencing and undetectable fluorescence resonance energy transfer changes. Expressing nanosensors in sgs3 and rdr6 transgene silencing mutants eliminated silencing and resulted in high fluorescence levels. To measure glucose changes over a wide range (nanomolar to millimolar), nanosensors with higher signal-to-noise ratios were expressed in these mutants. Perfusion of leaf epidermis with glucose led to concentration-dependent ratio changes for nanosensors with in vitro K(d) values of 600 microM (FLIPglu-600 microDelta13) and 3.2 mM (FLIPglu-3.2 mDelta13), but one with 170 nM K(d) (FLIPglu-170 nDelta13) showed no response. In intact roots, FLIPglu-3.2 mDelta13 gave no response, whereas FLIPglu-600 microDelta13, FLIPglu-2 microDelta13, and FLIPglu-170 nDelta13 all responded to glucose. These results demonstrate that cytosolic steady state glucose levels depend on external supply in both leaves and roots, but under the conditions tested they are lower in root versus epidermal and guard cells. Without photosynthesis and external supply, cytosolic glucose can decrease to <90 nM in root cells. Thus, observed gradients are steeper than expected, and steady state levels do not appear subject to tight homeostatic control. Nanosensor-expressing plants can be used to assess glucose flux differences between cells, invertase-mediated sucrose hydrolysis in vivo, delivery of assimilates to roots, and glucose flux in mutants affected in sugar transport, metabolism, and signaling.

摘要

基因编码的葡萄糖纳米传感器已被用于测量哺乳动物细胞质、细胞核和内质网中的稳态葡萄糖水平。不幸的是,在拟南芥转化体中,相同的纳米传感器表现出转基因沉默和无法检测到的荧光共振能量转移变化。在sgs3和rdr6转基因沉默突变体中表达纳米传感器消除了沉默并导致高荧光水平。为了测量宽范围(纳摩尔到毫摩尔)的葡萄糖变化,在这些突变体中表达了具有更高信噪比的纳米传感器。用葡萄糖灌注叶表皮导致体外K(d)值为600 microM(FLIPglu-600 microDelta13)和3.2 mM(FLIPglu-3.2 mDelta13)的纳米传感器的浓度依赖性比率变化,但K(d)为170 nM(FLIPglu-170 nDelta13)的纳米传感器没有反应。在完整的根中,FLIPglu-3.2 mDelta13没有反应,而FLIPglu-600 microDelta13、FLIPglu-2 microDelta13和FLIPglu-170 nDelta13都对葡萄糖有反应。这些结果表明,细胞质稳态葡萄糖水平取决于叶片和根中的外部供应,但在测试条件下,根中的葡萄糖水平低于表皮细胞和保卫细胞。没有光合作用和外部供应,根细胞中的细胞质葡萄糖可降至<90 nM。因此,观察到的梯度比预期的更陡,并且稳态水平似乎不受严格的稳态控制。表达纳米传感器的植物可用于评估细胞间的葡萄糖通量差异、体内转化酶介导的蔗糖水解、同化物向根的输送以及糖运输、代谢和信号传导受影响的突变体中的葡萄糖通量。