Regulation of sulfate uptake and expression of sulfate transporter genes in Brassica oleracea as affected by atmospheric H(2)S and pedospheric sulfate nutrition

Demand-driven signaling will contribute to regulation of sulfur acquisition and distribution within the plant. To investigate the regulatory mechanisms pedospheric sulfate and atmospheric H(2)S supply were manipulated in Brassica oleracea. Sulfate deprivation of B. oleracea seedlings induced a rapid increase of the sulfate uptake capacity by the roots, accompanied by an increased expression of genes encoding specific sulfate transporters in roots and other plant parts. More prolonged sulfate deprivation resulted in an altered shoot-root partitioning of biomass in favor of the root. B. oleracea was able to utilize atmospheric H(2)S as S-source; however, root proliferation and increased sulfate transporter expression occurred as in S-deficient plants. It was evident that in B. oleracea there was a poor shoot to root signaling for the regulation of sulfate uptake and expression of the sulfate transporters. cDNAs corresponding to 12 different sulfate transporter genes representing the complete gene family were isolated from Brassica napus and B. oleracea species. The sequence analysis classified the Brassica sulfate transporter genes into four different groups. The expression of the different sulfate transporters showed a complex pattern of tissue specificity and regulation by sulfur nutritional status. The sulfate transporter genes of Groups 1, 2, and 4 were induced or up-regulated under sulfate deprivation, although the expression of Group 3 sulfate transporters was not affected by the sulfate status. The significance of sulfate, thiols, and O-acetylserine as possible signal compounds in the regulation of the sulfate uptake and expression of the transporter genes is evaluated.     

Nitrogen Use Efficiency of Crop Plants: Physiological Constraints upon Nitrogen Absorption

Current global nitrogen fertilizer use has reached approximately one hundred billion kg per annum. In many agricultural systems, a very substantial portion of this applied nitrogen fertilizer is lost from soil to groundwaters, rivers and oceans. While soil physicochemical properties play a significant part in these losses, there are several characteristic features of plant nitrogen transporter function that facilitate N losses. Nitrate and ammonium efflux from roots result in a reduction of net nitrogen uptake. As external nitrate and ammonium concentrations, respectively, are increased, particularly into the range of concentrations that are typical of agricultural soils, elevated rates of nitrate and ammonium efflux result. The rapid down-regulation of high-affinity influx as plants become nitrogen replete further reduces the root's capacity to acquire external nitrogen; only nitrogen-starved roots absorb with both high capacity and high affinity. The results of studies using molecular biology methods demonstrate that genes encoding nitrate and ammonium transporters are rapidly down-regulated when nitrogen is resupplied to nitrogen-starved plants. Provision of ammonium to roots of plants actively absorbing nitrate imposes a block on nitrate uptake, the extent of which depends on the ammonium concentration, thus further reducing the efficient utilization of soil nitrate. During the daily variation of incoming light and during periods of low incident irradiation (i.e. heavy cloud cover) the expression levels of genes encoding nitrate and ammonium transporters, and rates of nitrate and ammonium uptake, are substantially reduced. Low temperatures reduce growth and nitrogen demand, and appear to discriminate against high-affinity nitrogen influx. In sum, these several factors conspire to limit rates of plant nitrogen uptake to values that are well below capacity. These characteristics of the plant's nitrogen uptake systems facilitate nitrogen losses from soils.     

Regulation of high-affinity sulphate transporters in plants: towards systematic analysis of sulphur signalling and regulation

Plants require the function of plasma membrane-bound sulphate transporters for the initial uptake of inorganic sulphate. Part of this fundamental process is the energy-dependent proton/sulphate co-transport systems that are located in the surface cell layers of roots. During sulphur limitation, plants are able to activate the expression of sulphate transporters that facilitate the uptake of sulphate in roots. SULTR1;1 and SULTR1;2 are suggested to be the essential components of the sulphate uptake system in Arabidopsis roots. The physiological importance of SULTR1;1 and SULTR1;2 is supported by characteristics that can cope with sulphur deficiency: they were (i) functional high-affinity sulphate transporters; (ii) induced by sulphur limitation at the mRNA levels; and (iii) predominantly localized in the root hairs, epidermis, and cortex. The expression of high-affinity sulphate transporters was primarily regulated by sulphur in a promoter-dependent manner. Aside from the sulphur-specific regulation, the induction of SULTR1;1 and SULTR1;2 high-affinity sulphate transporters by sulphur limitation was dependent on the supply of carbon and nitrogen. In this review, the application of SULTR promoter-GFP systems for the analysis of regulatory pathways of sulphate acquisition in plants is described.     

AtCHX13 is a plasma membrane K+ transporter

Potassium (K+) homeostasis is essential for diverse cellular processes, although how various cation transporters collaborate to maintain a suitable K+ required for growth and development is poorly understood. The Arabidopsis (Arabidopsis thaliana) genome contains numerous cation:proton antiporters (CHX), which may mediate K+ transport; however, the vast majority of these transporters remain uncharacterized. Here, we show that AtCHX13 (At2g30240) has a role in K+ acquisition. AtCHX13 suppressed the sensitivity of yeast (Saccharomyces cerevisiae) mutant cells defective in K+ uptake. Uptake experiments using (86)Rb+ as a tracer for K+ demonstrated that AtCHX13 mediated high-affinity K+ uptake in yeast and in plant cells with a K(m) of 136 and 196 microm, respectively. Functional green fluorescent protein-tagged versions localized to the plasma membrane of both yeast and plant. Seedlings of null chx13 mutants were sensitive to K+ deficiency conditions, whereas overexpression of AtCHX13 reduced the sensitivity to K+ deficiency. Collectively, these results suggest that AtCHX13 mediates relatively high-affinity K+ uptake, although the mode of transport is unclear at present. AtCHX13 expression is induced in roots during K+-deficient conditions. These results indicate that one role of AtCHX13 is to promote K+ uptake into plants when K+ is limiting in the environment.     

The phosphate uptake mechanism

The slow rate of diffusion of phosphate in soil results in a zone of depletion of phosphate ions in solution around the roots of plants in low phosphate soils. Transfer of phosphate to the site of uptake into the root symplasm limits phosphate uptake in such soils. This transfer involves movement across the depletion zone and through the root apoplasm. The apoplasm is made up of the cell walls of epidermal and cortical cells, together with the associated intercellular spaces. Although the pores in the open latticework of these cell walls permit movement of nutrients around cells, they increase the path length across which phosphate ions have to diffuse. The structural components and net negative charges of the cell walls also influence the effective concentrations of phosphate in the apoplasm. This concentration may be further modified by excreted organic compounds around cell walls and the presence of micro-organisms that use such compounds as carbon sources. A membrane on the inner surface of the cell wall, the plasmalemma, separates the apoplasm from the symplasm. Uptake of nutrients into the root symplasm occurs through transporter proteins embedded in this membrane. Understanding of the mechanisms by which phosphate is transported across the plasmalemma into the plant symplasm has advanced considerably over the past 4 years due to the application of molecular techniques. Genes encoding the transporters involved in this process have been isolated from a number of plant species. These transporters belong to a family of membrane proteins characterized by having 12 membrane-spanning domains arranged in a '6+6' configuration. H₂PO₄ ^– ions, together with protons, are transported through this protein. This transport process is driven by the potential across the membrane maintained by the action of a H⁺-ATPase, the `proton pump', that extrudes protons to the outer surface of the membrane. The expression of genes encoding high-affinity root phosphate transporters is regulated by the phosphorus (P) status of the plant. The transduction pathway involved in this regulation is not known at present. It is a systemic response rather than a localized response, however, the overall phosphate status of the plant being the controlling factor. Under phosphate stress, the expression of genes encoding these phosphate transporters is up-regulated. This results in a greater number of transporter proteins in the plasmalemma and enhanced phosphate uptake rates, if phosphate is available at the membrane surface. Uptake occurs around the root tip, into epidermal cells with their associated root hairs and into cells in the outer layers of the root cortex. Further back along the root axis, phosphate can also be taken up by transfer from mycorrhizal fungi to root cortical cells.Strategies for increasing nutrient uptake by overexpressing genes encoding high-affinity phosphate transporters are likely to be mainly applicable to situations where a reasonable phosphate concentration can be maintained at the outer surface of the plasmalemma. Maintaining such a concentration is a major problem in the phosphate deficient soils of the semi-arid tropics (SAT), so emphasis in these soils is on strategies to improve the movement of phosphate to the surface of the plasmalemma. There may be scope, however, for manipulating the expression of genes involved in the internal mobilisation of phosphate within the plant, thereby improving phosphate utilisation.     

Differential regulation of nramp and irt metal transporter genes in wild type and iron uptake mutants of tomato

Metal transporters regulated by iron can transport a variety of divalent metals, suggesting that iron regulation is important for specificity of iron transport. In plants, the iron-regulated broad-range metal transporter IRT1 is required for uptake of iron into the root epidermis. Functions of other iron-regulated plant metal transporters are not yet established. To deduce novel plant iron transport functions we studied the regulation of four tomato metal transporter genes belonging to the nramp and irt families with respect to environmental and genetic factors influencing iron uptake. We isolated Lenramp1 and Lenramp3 from tomato and demonstrate that these genes encode functional NRAMP metal transporters in yeast, where they were iron-regulated and localized mainly to intracellular vesicles. Lenramp1 and Leirt1 revealed both root-specific expression and up-regulation by iron deficiency, respectively, in contrast to Leirt2 and Lenramp3. Lenramp1 and Leirt1, but not Lenramp3 and Leirt2, were down-regulated in the roots of fer mutant plants deficient in a bHLH gene regulating iron uptake. In chloronerva mutant plants lacking the functional enzyme for synthesis of the plant-specific metal chelator nicotianamine Leirt1 and Lenramp1 were up-regulated despite sufficient iron supply independent of a functional fer gene. Lenramp1 was expressed in the vascular root parenchyma in a similar cellular pattern as the fer gene. However, the fer gene was not sufficient for inducing Lenramp1 and Leirt1 when ectopically expressed. Based on our results, we suggest a novel function for NRAMP1 in mobilizing iron in the vascular parenchyma upon iron deficiency in plants. We discuss fer/nicotianamine synthase-dependent and -independent regulatory pathways for metal transporter gene regulation.     

植物磷营养高效的分子生物学研究进展

挖掘利用植物自身的磷高效营养遗传资源是农业可持续发展的关键。磷高效营养性状涉及根形态、根分泌物、膜与体内磷转运以及菌根等许多方面,表现为数量遗传性状及受多基因控制。近年来,许多高亲和磷转运子基因已被克隆, 磷向地上部转运和磷吸收负反馈调节的控制基因也被发现, 对于根系分泌有机酸和酸性磷酸酶的基因的控制也有了一定的了解, 但目前对于根毛、排根、根构型以及菌根的营养学意义性状的分子生物学研究进展缓慢。     

与高等植物吸收(NO_3)~-/(NH_4)~+、(PO_4)~(3-)和K~+有关的膜转运蛋白编码基因的分子生物学研究现状

高等植物对土壤中营养元素的吸收是其一切生命活动过程的基础,尤其在营养元素缺乏的状态下,更与其抗营养饥饿等特性息息相关。兼于土壤中Ｎ、Ｐ、Ｋ元素缺乏的严重性与普遍性,以及Ｎ、Ｐ、Ｋ对高等植物生长和发育的重要性,有关高等植物吸收营养元素的膜转运蛋白编码基因的分子生物学研究已引起有关学者的高度重视。ＮＯ－３／ＮＨ＋４、ＰＯ３－４与Ｋ＋膜转运蛋白均有低亲和力和高亲和力系统（ＬｏｗＡｆｉｎｉｔｙＴｒａｎｓｐｏｒｔｅｒ＆ＨｉｇｈＡｆｉｎｉｔｙＴｒａｎｓｐｏｒｔｅｒ）。对ＰＯ４３－和Ｋ＋而言,低亲和力系统是组成性表达的系统,在正常营养状态下对根系吸收营养起重要作用。而高亲和力系统是受营养缺乏而诱导表达的系统,对于植物的抗逆性、耐营养饥饿至关重要。迄今为止,与之有关的基因的全长ｃＤＮＡ或全基因已在几种植物中被克隆。此外,对基因的表达特性亦有广泛研究。本文简要概述这三大营养元素的膜转运蛋白编码基因的分子生物学研究现状。     

The HAK1 gene of barley is a member of a large gene family and encodes a high-affinity potassium transporter.

The high-affinity K+ uptake system of plants plays a crucial role in nutrition and has been the subject of extensive kinetic studies. However, major components of this system remain to be identified. We isolated a cDNA from barley roots, HvHAK1, whose translated sequence shows homology to the Escherichia coli Kup and Schwanniomyces occidentalis HAK1 K+ transporters. HvHAK1 conferred high-affinity K+ uptake to a K(+)-uptake-deficient yeast mutant exhibiting the hallmark characteristics of the high-affinity K+ uptake described for barley roots. HvHAK1 also mediated low-affinity Na+ uptake. Another cDNA (HvHAK2) encoding a polypeptide 42% identical to HvHAK1 was also isolated. Analysis of several genomes of Triticeae indicates that HvHAK1 belongs to a multigene family. Translated sequences from bacterial DNAs and Arabidopsis, rice, and possibly human cDNAs show homology to the Kup-HAK1-HvHAK1 family of K+ transporters.     

高等植物K+吸收转运蛋白及其分子调节

K 在植物的生命活动中发挥着十分重要的作用。植物对K 的吸收,可分为高亲和吸收与低亲和吸收。在分子水平上,高亲和吸收主要由KUP/HAK/KT及HKT家族的K 转运蛋白来承担;而Shaker、KCO等家族的K 通道蛋白,则主要在植物的低亲和吸收中发挥重要作用。AKT1、HAK5及其在植物中的同源基因在高等植物K 吸收转运中占有举足轻重的地位。KUP/HAK/KT家族基因的调节,主要是转录水平的调节,而K 通道蛋白的调节则可能主要是一种翻译后调节。植物的蛋白激酶通过磷酸化K 通道蛋白来调节通道的活性,从而改变K 的吸收特性。本文综述了高等植物K 吸收运转及调节的分子机制研究方面的最新进展,并对研究的前景进行了展望。