植物体内蔗糖转运蛋白的功能和调控

蔗糖转运蛋白（sucrose transporter,SUT）负责蔗糖的跨膜运输,在韧皮部介导的源-库蔗糖运输和为库组织供应蔗糖的生理活动中起关键作用。本文介绍植物体内蔗糖转运蛋白基因家族、细胞定位与功能调节以及高等植物的蔗糖感受机制的研究进展。     

植物蔗糖转运蛋白表达的调控因素与分子机制

植物光合作用的产物主要以蔗糖的形式在植物体内进行从源到库的运输。蔗糖转运蛋白是此过程的重要参与者,其表达和调控与植物中光合作用产物的分配紧密关联,从而调控着植物的生长发育、结果结实、抗逆抗病等性状。蔗糖转运蛋白的表达受到植物发育时期、外界环境条件及激素的影响。蔗糖转运蛋白的调控机制有转录因子的调节、基因内部序列调控、蛋白质的磷酸化、蛋白之间的相互作用及质子转运体的活性调节等。综述了国内外对蔗糖转运蛋白表达与活性的调控因素及机制等最新的研究内容,以期为从多角度上探索植物蔗糖转运蛋白的功能和调控机制提供相关研究信息和思路。     

水稻蔗糖转运蛋白研究进展

蔗糖转运蛋白是光合产物运输与分配调控网络中的重要节点,主要参与蔗糖从"源"到"库"的质外体运输,在蔗糖的感应、"源"器官装载、韧皮部长距离运输和"库"器官卸载中起重要作用。总结和分析了水稻蔗糖转运蛋白基因家族的组成、蛋白结构特点、表达与调控特性、生物学功能等方面的研究进展,在此基础上,提出了蔗糖转运蛋白基础理论和应用研究方面存在的不足及应予重视和加强的主要方向。     

蔗糖膜运输系统与植物整体碳分配相关（综述）

蔗糖是光合作用的主要产物,作为碳同化的产物在植物体内进行分配。蔗糖的转运机制和效率通过减弱产物抑制来影响光合产率,通过控制源／库关系和生物量分配来调控植物活性。蔗糖在细胞质合成,或通过胞间连丝进行细胞问转运,或跨膜区域化,或外输入质外体被相邻细胞吸收。作为相对大极性的化合物,蔗糖的有效膜转运需要转运蛋白协助。跨液泡膜运输机制可能通过异化扩散、质子对向运输和同向运输;而跨质膜的运输则可能通过质子同向运输和异化扩散类似机制。近几十年仅在分子水平对质子同向运输进行了较为详尽的研究。这篇综述旨在综合介绍最近和过去关于蔗糖跨膜转运与植物整体碳分布机制。     

植物体内糖分子的长距离运输及其分子机制

植物器官(如叶、叶鞘、绿色的茎等)可以通过光合作用将CO₂合成为碳水化合物, 并经过长距离运输到达库组织(如新生组织、花粉、果实等)中进行贮存或利用。蔗糖是高等植物长距离运输碳水化合物的主要形式。蔗糖分子从源到库的运输包括源组织韧皮部的装载、维管束的运输和库组织韧皮部的卸载3个步骤。遗传学和分子生物学研究证明, 蔗糖转运蛋白、转化酶和单糖转运蛋白在糖分子的装载和卸载过程中发挥重要作用。该文综述了目前对光合产物运输过程及其调控分子机制的最新研究进展。     

植物蔗糖转运蛋白的基因与功能

蔗糖是植物体内碳水化合物长距离转运的主要( 甚至唯一) 形式, 为植物生长发育提供碳架与能量。蔗糖转运蛋白(sucrose transporter, SUT)负责蔗糖的跨膜运输, 在韧皮部介导的源-库蔗糖运输, 以及库组织的蔗糖供给中起关键作用。自从菠菜中克隆到第一个SUT基因以来, 已先后有多个SUT基因的cDNA得到克隆与功能分析, 涉及34种双子叶与单子叶植物。每种植物都有一个中等规模 的SUT基因家族, 其不同成员之间具有较高的氨基酸序列同源性, 但在蔗糖吸收的动力学特性、转运底物的特异性和表达谱等方面存在差异。本文系统介绍国内外(主要是国外)在植物SUT基因的克隆、分类与进化、细胞定位与功能, 以及研究方法等方面的研究进展, 并简要介绍我们在橡胶树SUT基因研究上的初步结果。     

植物蔗糖转运蛋白的基因与功能

蔗糖是植物体内碳水化合物长距离转运的主要（甚至唯一）形式，为植物生长发育提供碳架与能量。蔗糖转运蛋白（sucrose transporter，SUT）负责蔗糖的跨膜运输，在韧皮部介导的源-库蔗糖运输，以及库组织的蔗糖供给中起关键作用。自从菠菜中克隆到第一个SUT基因以来，已先后有多个SUT基因的cDNA得到克隆与功能分析，涉及34种双子叶与单子叶植物。每种植物都有一个中等规模的SUT基因家族，其不同成员之间具有较高的氨基酸序列同源性，但在蔗糖吸收的动力学特性、转运底物的特异性和表达谱等方面存在差异。本文系统介绍国内外（主要是国外）在植物SUT基因的克隆、分类与进化、细胞定位与功能，以及研究方法等方面的研究进展，并简要介绍我们在橡胶树SUT基因研究上的初步结果。     

甘薯蔗糖转运蛋白的功能分析

甘薯(Ipomoea batatas)是重要的粮食和工业加工原料作物。蔗糖是植物体内碳水化合物长距离转运的主要形式,蔗糖转运蛋白(sucrose transporter,SUT)在植物的生长代谢中调控蔗糖的跨膜运输和分配,在韧皮部介导的源-库蔗糖运输和为库组织供应蔗糖的生理活动中起关键作用。本研究根据不同淀粉性状甘薯块根中差异表达的2个SUT基因转录本,进行cDNA末端快速扩增(rapid amplification of cDNA ends,RACE)克隆,获得IbSUT62788和IbSUT81616的全长cDNA序列;通过系统发育分析明确其分类;通过在本氏烟草(Nicotiana benthamiana)中瞬时表达明确其亚细胞定位;通过酵母功能互补系统鉴定IbSUT62788和IbSUT81616是否具有吸收、转运蔗糖和己糖的能力。通过实时荧光定量PCR(real-time fluorescence quantitative polymerase chain reaction,RT-qPCR)分析IbSU62788和IbSUT81616在甘薯各器官中的表达特征;通过蘸花法得到外源表达IbSUT62788和IbSUT81616基因的拟南芥(Arabidopsis thaliana)植株,比较与野生型拟南芥的淀粉和糖含量的差异。结果表明,IbSUT62788和IbSUT81616分别编码505个和521个氨基酸的SUT蛋白,均属于SUT1亚家族。IbSUT62788和IbSUT81616均定位于细胞膜,在酵母系统中具有转运蔗糖、葡萄糖和果糖的能力。此外,IbSUT62788还具有转运甘露糖的能力。IbSUT62788在甘薯叶片、侧枝和茎中的表达量更高,IbSUT81616在侧枝、茎和块根中表达量更高。IbSUT62788和IbSUT81616在拟南芥中异源表达后,植株可以正常生长,但生物量增加。IbSUT62788的异源表达增加了拟南芥植株叶片可溶性糖含量、叶片大小和种子千粒重;IbSUT81616的异源表达增加了拟南芥植株叶片、根尖的淀粉积累量和种子千粒重,但减少了可溶性糖含量。本研究结果表明,IbSUT62788和IbSUT81616可能是调控甘薯蔗糖和糖含量性状的重要基因,在细胞膜上进行着蔗糖的跨膜运输、蔗糖进出库组织、韧皮部蔗糖的运输与卸载等生理功能,在拟南芥中异源表达造成的性状改变说明其在提高其他植物或作物产量中的应用潜力。本研究为揭示甘薯淀粉和糖代谢及重要品质性状形成机制提供了重要信息。     

水稻蔗糖转运及其与产量形成的关系

蔗糖是植物体内主要的光合产物和运输形式,在叶片中合成并经过维管组织向库器官转运,在库组织中水解并用于合成淀粉、蛋白质和纤维素等有机物。水稻蔗糖转运对调控作物生长发育和产量形成,特别是在逆境条件下的产量稳定,都具有十分重要的作用。本文重点综述了水稻蔗糖韧皮部装载、运输和卸载机制以及关键酶的活性和基因表达调控,并讨论了其与水稻产量形成的关系。     

《Molecular Plant》文章中文摘要

2011年第4卷第3期膜运输专刊(http://mplant.oxfordjournals.org/content/vol4/issue3/index.dtl)1Ayre BG(2011).Membrane-transport systems for sucrose in relation to whole-plant carbon partitioning.Mol Plant,4(3):377～394题目:蔗糖膜运输系统与植物整体碳分配相关(综述)摘要::蔗糖是光合作用的主要产物,作为碳同化的产物在植物体内进行分配。蔗糖的转运机制和效率通过减弱产物抑制来影响光合产率,通过控制源/库关系和生物量分配来调控植物活性。蔗糖在细胞质合     

Sucrose carrier RcSCR1 is involved in sucrose retrieval, but not in sucrose unloading in growing hypocotyls of Ricinus communis L

The transport of assimilates from source to sink tissues is mediated by the phloem. Along the vascular system the phloem changes its physiological function from loading phloem to transport and unloading phloem. Sucrose carrier proteins have been identified in the transport phloem, but it is unclear whether the physiological role of these transporters is phloem unloading of sucrose or retrieval of apoplasmic sucrose back into the sieve element/companion cell complex. Here, we describe the dynamic expression of the Ricinus communis sucrose carrier RcSCR1 in the hypocotyl at different sink strengths. Our results indicate that phloem unloading in castor bean is not catalysed by the phloem loader RcSCR1. However, this sucrose carrier represents the molecular basis of the sucrose retrieval mechanism along the transport phloem, which is dynamically adjusted to the sink strength. As a consequence, we assume that other release carrier(s) exist in sink tissues, such as the hypocotyl, in R. communis.     

Demonstration of an intramitochondrial invertase activity and the corresponding sugar transporters of the inner mitochondrial membrane in Jerusalem artichoke (<Emphasis Type="Italic">Helianthus tuberosus</Emphasis> L.) tubers

Genetic evidences indicate that alkaline/neutral invertases are present in plant cell organelles, and they might have a novel physiological function in mitochondria. The present study demonstrates an invertase activity in the mitochondrial matrix of Helianthus tuberosus tubers. The pH optimum, the kinetic parameters and the inhibitor profile of the invertase activity indicated that it belongs to the neutral invertases. In accordance with this topology, transport activities responsible for the mediation of influx/efflux of substrate/products were studied in the inner mitochondrial membrane. The transport of sucrose, glucose and fructose was shown to be bidirectional, saturable and independent of the mitochondrial respiration and membrane potential. Sucrose transport was insensitive to the inhibitors of the proton-sucrose symporters. The different kinetic parameters and inhibitors as well as the absence of cross-inhibition suggest that sucrose, glucose and fructose transport are mediated by separate transporters in the inner mitochondrial membrane. The mitochondrial invertase system composed by an enzyme activity in the matrix and the corresponding sugar transporters might have a role in both osmoregulation and intermediary metabolism.     

Evidence for the Transport of Maltose by the Sucrose Permease,CscB, of <Emphasis Type="Italic">Escherichia coli</Emphasis>

The purpose of this study was to examine the sugar recognition and transport properties of the sucrose permease (CscB), a secondary active transporter from Escherichia coli. We tested the hypothesis that maltose transport is conferred by the wild-type CscB transporter. Cells of E. coli HS4006 harboring pSP72/cscB were red on maltose MacConkey agar indicator plates. We were able to measure “downhill” maltose transport and establish definitive kinetic behavior for maltose entry in such cells. Maltose was an effective competitor of sucrose transport in cells with CscB, suggesting that the respective maltose and sucrose binding sites and translocation pathways through the CscB channel overlap. Accumulation (“uphill” transport) of maltose by cells with CscB was profound, demonstrating active transport of maltose by CscB. Sequencing of cscB encoded on plasmid pSP72/cscB used in cells for transport studies indicate an unaltered primary CscB structure, ruling out the possibility that mutation conferred maltose transport by CscB. We conclude that maltose is a bona fide substrate for the sucrose permease of E. coli. Thus, future studies of sugar binding, transport, and permease structure should consider maltose, as well as sucrose. Yang Peng and Sanath Kumar contributed equally to this paper.     

Energy coupling of membrane transport and efficiency of sucrose dissimilation in yeast

Proton coupled transport of α-glucosides via Mal11 into Saccharomyces cerevisiae costs one ATP per imported molecule. Targeted mutation of all three acidic residues in the active site resulted in sugar uniport, but expression of these mutant transporters in yeast did not enable growth on sucrose. We then isolated six unique transporter variants of these mutants by directed evolution of yeast for growth on sucrose. In three variants, new acidic residues emerged near the active site that restored proton-coupled sucrose transport, whereas the other evolved transporters still catalysed sucrose uniport. The localization of mutations and transport properties of the mutants enabled us to propose a mechanistic model of proton-coupled sugar transport by Mal11. Cultivation of yeast strains expressing one of the sucrose uniporters in anaerobic, sucrose-limited chemostat cultures indicated an increase in the efficiency of sucrose dissimilation by 21% when additional changes in strain physiology were taken into account. We thus show that a combination of directed and evolutionary engineering results in more energy efficient sucrose transport, as a starting point to engineer yeast strains with increased yields for industrially relevant products.     

Exploring the photosynthetic production capacity of sucrose by cyanobacteria

Because cyanobacteria are photosynthetic, fast-growing microorganisms that can accumulate sucrose under salt stress, they have a potential application as a sugar source for the biomass-derived production of renewable fuels and chemicals. In the present study, the production of sucrose by the cyanobacteria Synechocystis sp. PCC6803, Synechococcus elongatus PCC7942, and Anabaena sp. PCC7120 was examined. The three species displayed different growth curves and intracellular sucrose accumulation rates in response to NaCl. Synechocystis sp. PCC6803 was used to examine the impact of modifying the metabolic pathway on the levels of sucrose production. The co-overexpression of sps (slr0045), spp (slr0953), and ugp (slr0207) lead to a 2-fold increase in intracellular sucrose accumulation, whereas knockout of ggpS (sll1566) resulted in a 1.5-fold increase in the production of this sugar. When combined, these genetic modifications resulted in a fourfold increase in intracellular sucrose accumulation. To explore methods for optimizing the transport of the intracellular sucrose to the growth medium, the acid-wash technique and the CscB (sucrose permease)-dependent export method were evaluated using Synechocystis sp. PCC6803. Whereas the acid-wash technique proved to be effective, the CscB-dependent export method was not effective. Taken together, these results suggest that using genetic engineering, photosynthetic cyanobacteria can be optimized for efficient sucrose production.     

Sucrose transport by Streptococcus mutans. Evidence for multiple transport systems

The transport of sucrose by selected mutant and wild-type cells of Streptococcus mutans was studied using washed cocci harvested at appropriate phases of growth, incubated in the presence of fluoride and appropriately labelled substrates. The rapid sucrose uptake observed cannot be ascribed to possible extracellular formation of hexoses from sucrose and their subsequent transport, formation of intracellular glycogen-like polysaccharide, or binding of sucrose or extracellular glucans to the cocci. Rather, there are at least three discrete transport systems for sucrose, two of which are $\text{phospho}\text{enol}\text{pyruvate-dependent}$ phosphotransferases with relatively low apparent $\text{K}{}_{\mathrm{<mtext>m</mtext>}}$ values and the other a non-phosphotransferase (non-PTS) third transport system (termed TTS) with a relatively high apparent $\text{K}{}_{\mathrm{<mtext>m</mtext>}}$. For strain 6715-13 mutant 33, the $\text{K}{}_{\mathrm{<mtext>m</mtext>}}$ values are 6.25·10^?5 M, 2.4·10^?4 M, and 3.0·10^?3 M, respectively; for strain NCTC-10449, the $\text{K}{}_{\mathrm{<mtext>m</mtext>}}$ values are 7.1·10^?5 M, 2.5·10^?4 M and 3.3·10^?3 M, respectively. The two lower $\text{K}{}_{\mathrm{<mtext>m</mtext>}}$ systems could not be demonstrated in mid-log phase glucose-adapted cocci, a condition known to repress sucrose-specific phosphotransferase activity, but under these conditions the highest $\text{K}{}_{\mathrm{<mtext>m</mtext>}}$ system persists. Also, a mutant devoid of sucrose-specific phosphotransferase activity fails to evidence the two high affinity (low apparent $\text{K}{}_{\mathrm{<mtext>m</mtext>}}$) systems, but still has the lowest affinity (highest $\text{K}{}_{\mathrm{<mtext>m</mtext>}}$) system. There was essentially no uptake at 4°C indicating these processes are energy dependent. The third transport system, whose nature is unknown, appears to function under conditions of sucrose abundance and rapid growth which are known to repress $\text{phospho}\text{enol}\text{pyruvate-dependent}$ sucrose-specific phosphotransferase activity in S. mutans. These multiple transport systems seem well-adapted to S. mutans which is faced with fluctuating supplies of sucrose in its natural habitat on the surfaces of teeth.     

Characteristics of the sucrose uptake system of vacuoles isolated from red beet tissue. Kinetics and specifity of the sucrose uptake system

The uptake of sucrose against a concentration gradient into the dextran-impermeable [³H]H₂O space of red beet (Beta vulgaris L.) vacuoles has been studied using silicone-layer-filtering centrifugation on both fluorometric and ¹⁴C-measurement of sucrose. Sucrose transport into vacuoles proceeds partly by an active transport system and partly by passive permeation. The K _M(20°C) for active sucrose uptake was found to be about 22 mM and the V _Max(20°C) was about 174 nmol sucrose x (unit betacyanin)^-1 x h^-1. The temperature dependency of sucrose transport appears to have an activation energy of 35,0 KJ×mol^-1. Among various mono-, di-, and trisaccharides tested, raffinose acts as a competitive inhibitor of sucrose uptake.Abbreviations EDTA ethylenediamine tetraacetic acid - fr. wt. fresh weight - Tris tris-(hydroxymethyl)-aminomethan     

Valine uptake in the tap root of sugar beet: a comparative analysis with sucrose uptake

Given the lack of data on the absorption of amino acids in the tap root of Beta vulgaris, we studied the uptake of valine and compared it with that of sucrose at the same concentration (1 mM). The uptake of both substrates shared some similar characteristics. In particular, the absorption in both cases was controlled by an active process as evidenced by the inhibitory effect of CCCP and inhibitors of ATPases (DES, DCCD, orthovanadate). Both absorptions also involved the thiol and histidyl groups of protein carriers included in the plasmalemma as shown by treatment with specific compounds (PCMBS, mersalyl, NEM) inhibiting the transport of the nutrients in tissues and in purified PMV. However, it was shown that these uptakes present major differences. Firstly, unlike sucrose uptake, valine uptake was very sensitive to transmembrane electrical potential. Indeed, hyperpolarizing treatment with FC increased valine uptake but did not modify sucrose uptake. By contrast, treatment with high concentrations of KCl, which should result in depolarization of the cells, considerably decreased valine uptake and activated sucrose uptake. Secondly, ion mobilizations were different in the two types of transport. Unlike sucrose, application of valine to tissues strongly modified the time course of H⁺ influx. By contrast, sucrose uptake was controlled by K⁺ involvement as shown by effects either of modulators of K⁺ mobilization (LiCl, TEA) or of treatments inducing K⁺ starvation from the external medium.     

<Emphasis Type="Italic">LeFRK2</Emphasis> is required for phloem and xylem differentiation and the transport of both sugar and water

It has been suggested that LeFRK2, the major fructose-phosphorylating enzyme in tomato plants, may be required for stem xylem development. Yet, we do not know if this enzyme affects the development of individual vessels, whether it affects water conductance, or whether it affects phloem development and sugar transport. Here, we show that suppression of LeFRK2 results in a significant reduction in the size of vascular cells and slows fiber maturation. The vessels in stems of LeFRK2-antisense plants are narrower than in WT plants and have thinner secondary cell walls. Although the cambium produces rounded secondary vessels, these vessels become deformed during the early stages of xylem maturation. Water conductance is then reduced in stems, roots, and leaves, suggesting that LeFRK2 influences xylem development throughout the entire vascular system. Interestingly, the build-up of positive xylem pressure under static (no-flow) conditions was also decreased. Suppression of LeFRK2 reduced the length and width of the sieve elements, as well as callose deposition. To examine the effect of LeFRK2 suppression on phloem transport, we created triple-grafted plants in which a portion of the wild-type stem was replaced with an antisense interstcok, and compared the contents of the transported sugar, sucrose, in the different portions of these stems. Sucrose contents above and within the LeFRK2-antisense interstock were significantly higher than those below the graft. These results show that the antisense interstock restricted the downward movement of sucrose, suggesting that LeFRK2 is required for both phloem and xylem development. Contribution No. 114/2009 from the Volcani Center ARO.     

Evidence for solution flow in the phloem of willow

Sucrose specific mass transfer measurements were made in a translocating willow shoot (Salix viminalis L.) by a steady state labelling technique and the translocate sucrose specific activity, concentration and velocity monitored by analysis of the honeydew from two colonies of the willow aphid Tuberolachnus salignus Gmelin. The values of sucrose SMT obtained were related to the simultaneous measurements of translocate concentration and velocity and to the gradients of sucrose concentration within the stem transport path to determine if transport was a bulk flow or a diffusional analogue. Estimates of potassium ion concentration in the sieve tubes were made, using aphid honeydew, and related to the sucrose SMT measured simultaneously. Correlations were found between translocate concentration, velocity and SMT which suggested that solution flow was occurring rather than a process analogous to diffusion. Evidence was obtained that velocity of flow was a valid concept and that the measured velocity was being lowered by leakage of tracer from the sieve tubes. The analysis of potassium concentration suggested that if solution flow was occurring then potassium must be very exchangeable down the transport path. A good correlation was observed between the SMT of sucrose and the combined gradient of sucrose and potassium concentration, though this gradient was in the opposite direction to transport in some cases.Abbreviations SMT Sucrose specific mass transfer rate - SAR Specific activity ratio - OP Osmotic pressure