Characterization of Peanut Germin-Like Proteins,AhGLPs in Plant Development and Defense

Background

Germin-like superfamily members are ubiquitously expressed in various plant species and play important roles in plant development and defense. Although several GLPs have been identified in peanut (Arachis hypogaea L.), their roles in development and defense remain unknown. In this research, we study the spatiotemporal expression of AhGLPs in peanut and their functions in plant defense.

Results

We have identified three new AhGLP members (AhGLP3b, AhGLP5b and AhGLP7b) that have distinct but very closely related DNA sequences. The spatial and temporal expression profiles revealed that each peanut GLP gene has its distinct expression pattern in various tissues and developmental stages. This suggests that these genes all have their distinct roles in peanut development. Subcellular location analysis demonstrated that AhGLP2 and 5 undergo a protein transport process after synthesis. The expression of all AhGLPs increased in responding to Aspergillus flavus infection, suggesting AhGLPs'' ubiquitous roles in defense to A. flavus. Each AhGLP gene had its unique response to various abiotic stresses (including salt, H₂O₂ stress and wound), biotic stresses (including leaf spot, mosaic and rust) and plant hormone stimulations (including SA and ABA treatments). These results indicate that AhGLPs have their distinct roles in plant defense. Moreover, in vivo study of AhGLP transgenic Arabidopsis showed that both AhGLP2 and 3 had salt tolerance, which made transgenic Arabidopsis grow well under 100 mM NaCl stress.

Conclusions

For the first time, our study analyzes the AhGLP gene expression profiles in peanut and reveals their roles under various stresses. These results provide an insight into the developmental and defensive roles of GLP gene family in peanut.     

超量表达细胞D型周期蛋白CYCD3;1影响拟南芥根的发育

用雌激素诱导表达的启动子（XVE启动子）超量表达CYCD3;1的结果表明CYCD3;1的超量表达不仅抑制拟南芥初生根的伸长,而且还抑制初生根对重力刺激的反应能力。     

Differential Auxin-Transporting Activities of PIN-FORMED Proteins in Arabidopsis Root Hair Cells

The Arabidopsis (Arabidopsis thaliana) genome includes eight PIN-FORMED (PIN) members that are molecularly diverged. To comparatively examine their differences in auxin-transporting activity and subcellular behaviors, we expressed seven PIN proteins specifically in Arabidopsis root hairs and analyzed their activities in terms of the degree of PIN-mediated root hair inhibition or enhancement and determined their subcellular localization. Expression of six PINs (PIN1–PIN4, PIN7, and PIN8) in root hair cells greatly inhibited root hair growth, most likely by lowering auxin levels in the root hair cell by their auxin efflux activities. The auxin efflux activity of PIN8, which had not been previously demonstrated, was further confirmed using a tobacco (Nicotiana tabacum) cell assay system. In accordance with these results, those PINs were localized in the plasma membrane, where they likely export auxin to the apoplast and formed internal compartments in response to brefeldin A. These six PINs conferred different degrees of root hair inhibition and sensitivities to auxin or auxin transport inhibitors. Conversely, PIN5 mostly localized to internal compartments, and its expression in root hair cells rather slightly stimulated hair growth, implying that PIN5 enhanced internal auxin availability. These results suggest that different PINs behave differentially in catalyzing auxin transport depending upon their molecular activity and subcellular localization in the root hair cell.Auxin plays a critical role in plant development and growth by forming local concentration gradients. Local auxin gradients, created by the polar cell-to-cell movement of auxin, are implicated in primary axis formation, root meristem patterning, lateral organ formation, and tropic movements of shoots and roots (for recent review, see Vanneste and Friml, 2009). The cell-to-cell movement of auxin is achieved by auxin influx and efflux transporters such as AUXIN-RESISTANT1 (AUX1)/LIKE-AUX1 for influx and PIN-FORMED (PIN) and the P-glycoprotein (PGP) of ABCB (ATP-binding cassette-type transporter subfamily B) for efflux. Since diffusive efflux of the natural auxin indole-3-acetic acid (IAA; pKa = 4.75) is not favorable and PINs are localized in the plasma membrane in a polar manner, PINs act as rate-limiting factors for cellular auxin efflux and polar auxin transport through the plant body. These PINs'' properties explain why representative physiological effects of auxin transport are associated with PINs.Auxin flows from young aerial parts all the way down to the root tip columella in which an auxin maximum is formed for root stem cell maintenance and moves up toward the root differentiation zone through root epidermal cells, where a part of it travels back to the root tip via cortical cells (Blilou et al., 2005). This directional auxin flow is supported by the polar localization of PINs: PIN1, PIN3, and PIN7 at the basal side of stele cells (Friml et al., 2002a, 2002b; Blilou et al., 2005), PIN4 at the basal side in root stem cells (Friml et al., 2002a), and PIN2 at the upper side of root epidermis and at the basal side of the root cortex (Luschnig et al., 1998; Müller et al., 1998). Another interesting aspect of PIN-mediated auxin transport is the dynamics in directionality of auxin flow due to environmental stimuli-directed changes of subcellular PIN polarity, as exemplified for PIN3, whose subcellular localization changes in response to the gravity vector (Friml et al., 2002b).An intriguing question is how different PIN proteins have different subcellular polarities, which might be attributable to PIN-specific molecular properties, cell-type-specific factors, or both. The different PIN subcellular polarities in different cell types seemingly indicate that cell-type-specific factors are involved in polarity. In the case of PIN1, however, both classes of factors appear to affect its subcellular localization because when expressed under the PIN2 promoter, PIN1 localizes to the upper or basal side of root epidermal cells, depending on the GFP insertion site of the protein (Wiśniewska et al., 2006). A recent study demonstrated that the polar targeting of PIN proteins is modulated by phosphorylation/dephosphorylation of the central hydrophilic loop of PINs, which is mediated by PINOID (PID; a Ser/Thr protein kinase)/PP2A phosphatase (Michniewicz et al., 2007). The central hydrophilic domain of PINs might provide the molecule-specific cue for PIN polarity, together with as yet unknown cell-specific factors. Different recycling behaviors of PINs, which show variable sensitivities to brefeldin A (BFA), also imply different molecular characters among PIN species. Most PIN1 proteins are internalized by BFA treatment, whereas considerable amounts of PIN2 remain in the plasma membrane in addition to internal accumulation after BFA treatment. Recycling and basal polar targeting of PIN1 is dependent on the BFA-sensitive guanine nucleotide exchange factor for adenosyl ribosylation factors (ARF GEFs), GNOM, which is the major target of BFA. In contrast, apical targeting and recycling of PIN2 is independent of GNOM and controlled by BFA-resistant ARF GEFs (Geldner et al., 2003; Kleine-Vehn and Friml, 2008).In contrast to their distinct subcellular localizations, the differential auxin-transporting activities of PINs remain to be studied. The divergent primary structures of PIN proteins are not only indicative of differential subcellular polarity, but also would represent their differential catalytic activities for auxin transport. The auxin efflux activities of Arabidopsis (Arabidopsis thaliana) PINs have been demonstrated using Arabidopsis and heterologous systems: PIN1 and PIN5 in Arabidopsis cells (Petrásek et al., 2006; Mravec et al., 2009); PIN2, PIN3, PIN4, PIN6, and PIN7 in tobacco (Nicotiana tabacum) Bright Yellow-2 (BY-2) cells (Lee and Cho, 2006; Petrásek et al., 2006; Mravec et al., 2008); PIN1, PIN2, PIN5, and PIN7 in yeast (Saccharomyces cerevisiae) cells (Petrásek et al., 2006; Blakeslee et al., 2007; Mravec et al., 2009; Yang and Murphy, 2009); and PIN1, PIN2, and PIN7 in HeLa cells (Petrásek et al., 2006; Blakeslee et al., 2007). Among the eight Arabidopsis PIN members, PIN1, PIN2, PIN3, PIN4, PIN6, and PIN7, which share a similar molecular structure in terms of the presence of a long central loop (hereafter called long-looped PINs; Fig. 1A; Supplemental Fig. S1), have been shown to catalyze auxin efflux at the cellular level. On the other hand, PIN5 and PIN8 possess a very short putative central loop (hereafter called short-looped PINs). Although PIN5 was recently shown to be localized in the endoplasmic reticulum (ER) and proposed to transport auxin metabolites into the ER lumen, its cellular function regarding its intracellular auxin-transporting activity has not been shown, and the auxin-transporting activity of PIN8 has yet to be demonstrated. In spite of the same transport directionality (auxin efflux) and similar molecular structures, the long-looped PINs exhibit sequence divergence not only in their central loop, but also in certain residues of the transmembrane domains. This structural divergence of long-looped PINs might be indicative of their differential auxin-transporting activities, which have not yet been quantitatively compared.Open in a separate windowFigure 1.Differential activities of PINs in the Arabidopsis root hair. A, Two distinctive PIN groups with different central hydrophilic loop sizes. Topology of PIN proteins was predicted by four different programs as described in Supplemental Figure S1. Numbers above indicate the number of transmembrane helices for each N- and C-terminal region, and numbers below indicate the number of amino acid residues of the central hydrophilic domain. B, Representative root images of control (Cont; Columbia-0) and root-hair-specific PIN-overexpressing (PINox; ProE7:PIN-GFP or ProE7:PIN [−]) plants. Bar = 100 μm for all. C, Root hair lengths of control and PINox plants. Six to 12 independent transgenic lines (average = 8.3), and 42 to 243 roots (average = 86.8) and 336 to 2,187 root hairs (average = 727.8) per construct, were observed for the estimation of root hair length. Data represent means ± se. The root hair lengths of PIN5ox lines were significantly longer than those of the control (P = 0.016 for PIN5ox; P < 0.0001 for PIN5-GFP1ox and PIN5-GFP2ox).To comparatively assess the cytological behaviors and molecular activities of different PIN members, it would be favorable to use a single assay system that provides a consistent cellular environment and enables quantitative estimation of PIN activity. In previous studies, we adopted the root hair single cell system to quantitatively assay auxin-transporting or regulatory activities of PINs, PGPs, AUX1, and PID (Lee and Cho, 2006; Cho et al., 2007a). Root hair growth is proportional to internal auxin levels in the root hair cell. Therefore, auxin efflux inhibits and auxin influx enhances root hair growth (Cho et al., 2007b; Lee and Cho, 2008). In addition, the use of a root-hair-specific promoter (Cho and Cosgrove, 2002; Kim et al., 2006) for expression of auxin transporters enables the transporters'' biological effect to be pinpointed to only the root hair cell, thus excluding probable non-cell-autonomous effects that could be caused by the general expression of auxin transporters.In this study, we expressed five long-looped PINs (PIN1, PIN2, PIN3, PIN4, and PIN7) and two short-looped PINs (PIN5 and PIN8) in root hair cells and compared their auxin-transporting activities and cytological dynamics. To directly measure the radiolabeled auxin-transporting activities of PIN5 and PIN8, we used an additional assay system, tobacco suspension cells. Our data revealed that PINs have differential molecular activities and pharmacological responses and that the short-looped and long-looped PINs have different subcellular localizations.     

Xyloglucan Deficiency Disrupts Microtubule Stability and Cellulose Biosynthesis in Arabidopsis,Altering Cell Growth and Morphogenesis

Xyloglucan constitutes most of the hemicellulose in eudicot primary cell walls and functions in cell wall structure and mechanics. Although Arabidopsis (Arabidopsis thaliana) xxt1 xxt2 mutants lacking detectable xyloglucan are viable, they display growth defects that are suggestive of alterations in wall integrity. To probe the mechanisms underlying these defects, we analyzed cellulose arrangement, microtubule patterning and dynamics, microtubule- and wall-integrity-related gene expression, and cellulose biosynthesis in xxt1 xxt2 plants. We found that cellulose is highly aligned in xxt1 xxt2 cell walls, that its three-dimensional distribution is altered, and that microtubule patterning and stability are aberrant in etiolated xxt1 xxt2 hypocotyls. We also found that the expression levels of microtubule-associated genes, such as MAP70-5 and CLASP, and receptor genes, such as HERK1 and WAK1, were changed in xxt1 xxt2 plants and that cellulose synthase motility is reduced in xxt1 xxt2 cells, corresponding with a reduction in cellulose content. Our results indicate that loss of xyloglucan affects both the stability of the microtubule cytoskeleton and the production and patterning of cellulose in primary cell walls. These findings establish, to our knowledge, new links between wall integrity, cytoskeletal dynamics, and wall synthesis in the regulation of plant morphogenesis.The primary walls of growing plant cells are largely constructed of cellulose and noncellulosic matrix polysaccharides that include hemicelluloses and pectins (Carpita and Gibeaut, 1993; Somerville et al., 2004; Cosgrove, 2005). Xyloglucan (XyG) is the most abundant hemicellulose in the primary walls of eudicots and is composed of a β-1,4-glucan backbone with side chains containing Xyl, Gal, and Fuc (Park and Cosgrove, 2015). XyG is synthesized in the Golgi apparatus before being secreted to the apoplast, and its biosynthesis requires several glycosyltransferases, including β-1,4-glucosyltransferase, α-1,6-xylosyltransferase, β-1,2-galactosyltransferase, and α-1,2-fucosyltransferase activities (Zabotina, 2012). Arabidopsis (Arabidopsis thaliana) XYLOGLUCAN XYLOSYLTRANSFERASE1 (XXT1) and XXT2 display xylosyltransferase activity in vitro (Faik et al., 2002; Cavalier and Keegstra, 2006), and strikingly, no XyG is detectable in the walls of xxt1 xxt2 double mutants (Cavalier et al., 2008; Park and Cosgrove, 2012a), suggesting that the activity of XXT1 and XXT2 are required for XyG synthesis, delivery, and/or stability.Much attention has been paid to the interactions between cellulose and XyG over the past 40 years. Currently, there are several hypotheses concerning the nature of these interactions (Park and Cosgrove, 2015). One possibility is that XyGs bind directly to cellulose microfibrils (CMFs). Recent data indicating that crystalline cellulose cores are surrounded with hemicelluloses support this hypothesis (Dick-Pérez et al., 2011). It is also possible that XyG acts as a spacer-molecule to prevent CMFs from aggregating in cell walls (Anderson et al., 2010) or as an adapter to link cellulose with other cell wall components, such as pectin (Cosgrove, 2005; Cavalier et al., 2008). XyG can be covalently linked to pectin (Thompson and Fry, 2000; Popper and Fry, 2005, 2008), and NMR data demonstrate that pectins and cellulose might interact to a greater extent than XyG and cellulose in native walls (Dick-Pérez et al., 2011). Alternative models exist for how XyG-cellulose interactions influence primary wall architecture and mechanics. One such model posits that XyG chains act as load-bearing tethers that bind to CMFs in primary cell walls to form a cellulose-XyG network (Carpita and Gibeaut, 1993; Pauly et al., 1999; Somerville et al., 2004; Cosgrove, 2005). However, results have been accumulating against this tethered network model, leading to an alternative model in which CMFs make direct contact, in some cases mediated by a monolayer of xyloglucan, at limited cell wall sites dubbed “biomechanical hotspots,” which are envisioned as the key sites of cell wall loosening during cell growth (Park and Cosgrove, 2012a; Wang et al., 2013; Park and Cosgrove, 2015). Further molecular, biochemical, and microscopy experiments are required to help distinguish which aspects of the load-bearing, spacer/plasticizer, and/or hotspot models most accurately describe the functions of XyG in primary walls.Cortical microtubules (MTs) direct CMF deposition by guiding cellulose synthase complexes in the plasma membrane (Baskin et al., 2004; Paredez et al., 2006; Emons et al., 2007; Sánchez-Rodriguez et al., 2012), and the patterned deposition of cellulose in the wall in turn can help determine plant cell anisotropic growth and morphogenesis (Baskin, 2005). Disruption of cortical MTs by oryzalin, a MT-depolymerizing drug, alters the alignment of CMFs, suggesting that MTs contribute to CMF organization (Baskin et al., 2004). CELLULOSE SYNTHASE (CESA) genes, including CESA1, CESA3, and CESA6, are required for normal CMF synthesis in primary cell walls (Kohorn et al., 2006; Desprez et al., 2007), and accessory proteins such as COBRA function in cellulose production (Lally et al., 2001). Live-cell imaging from double-labeled YFP-CESA6; CFP-ALPHA-1 TUBULIN (TUA1) Arabidopsis seedlings provides direct evidence that cortical MTs determine the trajectories of cellulose synthesis complexes (CSCs) and patterns of cellulose deposition (Paredez et al., 2006). Additionally, MT organization affects the rotation of cellulose synthase trajectories in the epidermal cells of Arabidopsis hypocotyls (Chan et al., 2010). Recently, additional evidence for direct guidance of CSCs by MTs has been provided by the identification of CSI1/POM2, which binds to both MTs and CESAs (Bringmann et al., 2012; Li et al., 2012). MICROTUBULE ORGANIZATION1 (MOR1) is essential for cortical MT organization (Whittington et al., 2001), but disruption of cortical MTs in the mor1 mutant does not greatly affect CMF organization (Sugimoto et al., 2003), and oryzalin treatment does not abolish CSC motility (Paredez et al., 2006).Conversely, the organization of cortical MTs can be affected by cellulose synthesis. Treatment with isoxaben, a cellulose synthesis inhibitor, results in disorganized cortical MTs in tobacco cells, suggesting that inhibition of cellulose synthesis affects MT organization (Fisher and Cyr, 1998), and treatment with 2,6-dichlorobenzonitrile, another cellulose synthesis inhibitor, alters MT organization in mor1 plants (Himmelspach et al., 2003). Cortical MT orientation in Arabidopsis roots is also altered in two cellulose synthesis-deficient mutants, CESA6^52-isx and kor1-3, suggesting that CSC activity can affect MT arrays (Paredez et al., 2008). Together, these results point to a bidirectional relationship between cellulose synthesis/patterning and MT organization.MTs influence plant organ morphology, but the detailed mechanisms by which they do so are incompletely understood. The dynamics and stability of cortical MTs are also affected by MT-associated proteins (MAPs). MAP18 is a MT destabilizing protein that depolymerizes MTs (Wang et al., 2007), MAP65-1 functions as a MT crosslinker, and MAP70-1 functions in MT assembly (Korolev et al., 2005; Lucas et al., 2011). MAP70-5 stabilizes existing MTs to maintain their length, and its overexpression induces right-handed helical growth (Korolev et al., 2007); likewise, MAP20 overexpression results in helical cell twisting (Rajangam et al., 2008). CLASP promotes microtubule stability, and its mutant is hypersensitive to microtubule-destabilizing drug oryzalin (Ambrose et al., 2007). KATANIN1 (KTN1) is a MT-severing protein that can sever MTs into short fragments and promote the formation of thick MT bundles that ultimately depolymerize (Stoppin-Mellet et al., 2006), and loss of KTN1 function results in reduced responses to mechanical stress (Uyttewaal et al., 2012). In general, cortical MT orientation responds to mechanical signals and can be altered by applying force directly to the shoot apical meristem (Hamant et al., 2008). The application of external mechanical pressure to Arabidopsis leaves also triggers MT bundling (Jacques et al., 2013). Kinesins, including KINESIN-13A (KIN-13A) and FRAGILE FIBER1 (FRA1), have been implicated in cell wall synthesis (Cheung and Wu, 2011; Fujikura et al., 2014). The identification of cell wall receptors and sensors is beginning to reveal how plant cell walls sense and respond to external signals (Humphrey et al., 2007; Ringli, 2010); some of them, such as FEI1, FEI2, THESEUS1 (THE1), FERONIA (FER), HERCULES RECEPTOR KINASE1 (HERK1), WALL ASSOCIATED KINASE1 (WAK1), WAK2, and WAK4, have been characterized (Lally et al., 2001; Decreux and Messiaen, 2005; Kohorn et al., 2006; Xu et al., 2008; Guo et al., 2009; Cheung and Wu, 2011). However, the relationships between wall integrity, cytoskeletal dynamics, and wall synthesis have not yet been fully elucidated.In this study, we analyzed CMF patterning, MT patterning and dynamics, and cellulose biosynthesis in the Arabidopsis xxt1 xxt2 double mutant that lacks detectable XyG and displays altered growth (Cavalier et al., 2008; Park and Cosgrove, 2012a). To investigate whether and how XyG deficiency affects the organization of CMFs and cortical MTs, we observed CMF patterning in xxt1 xxt2 mutants and Col (wild-type) controls using atomic force microscopy (AFM), field emission scanning electron microscopy (FESEM), transmission electron microscopy (TEM), and confocal microscopy (Hodick and Kutschera, 1992; Derbyshire et al., 2007; Anderson et al., 2010; Zhang et al., 2014). We also generated transgenic Col and xxt1 xxt2 lines expressing GFP-MAP4 (Marc et al., 1998) and GFP-CESA3 (Desprez et al., 2007), and analyzed MT arrays and cellulose synthesis using live-cell imaging. Our results show that the organization of CMFs is altered, that MTs in xxt1 xxt2 mutants are aberrantly organized and are more sensitive to external mechanical pressure and the MT-depolymerizing drug oryzalin, and that cellulose synthase motility and cellulose content are decreased in xxt1 xxt2 mutants. Furthermore, real-time quantitative RT-PCR measurements indicate that the enhanced sensitivity of cortical MTs to mechanical stress and oryzalin in xxt1 xxt2 plants might be due to altered expression of MT-stabilizing and wall receptor genes. Together, these data provide insights into the connections between the functions of XyG in wall assembly, the mechanical integrity of the cell wall, cytoskeleton-mediated cellular responses to deficiencies in wall biosynthesis, and cell and tissue morphogenesis.     

Proteins Induced by Physical Stimuli in Root Tips of Arabidopsis thaliana Seedling

Proteins newly synthesized in cells of root tips of Arabidopsisseedlings after gravistimulation and photo-induced tactile stimulationwere analyzed by two-dimensional gel electrophoresis. Intensitiesof two out of about 600 protein spots were observed to increasetransiently when culture flasks in which seedlings has beengrown were kept on their sides. When the flasks were kept verticalon a rocking table and rocked continuously for 24 hours, intensitiesof ten protein spots increased, and four spots appeared forthe first time. Analysis of [³²P]-labeled proteins revealedthat the continuous rocking treatment enhanced the phosphorylationof proteins in two spots. When the seedlings in flasks wereilluminated from the front, and the roots bent towards the backwall of the flasks, three spots appeared for the first timeand intensities of nine spots were enhanced. Three of the twelvespots whose intensities were enhanced by the photo-induced tactilestimulation were also affected by continuous rocking treatment.The roles of protein synthesis and phosphorylation in the pathwaysbetween the stimuli and the responses are discussed. (Received June 18, 1992; Accepted December 16, 1992)     

Differential Hypocotyl and Root Development of Arabidopsis Auxin-Insensitive Mutants

Arabidopsis , aux1-7, axr1-3 and axr2-1, grown in a natural sandy soil, without sucrose supplementation. The three mutants showed impaired epidermal cell elongation in the hypocotyls of 15-day-old seedlings, with axr2-1 showing the most marked effects. In addition, the roots of axr2-1 elongated faster and presented a more extended meristematic zone than the other genotypes. Unchanged epidermal cell length in the differentiation zone of axr2-1 relative to the wild-type suggested enhancement of cell proliferation. These alterations may have affected the timing and site of emergence of the root hairs, starting later and further from the root tip than in the other genotypes. Similarly to the wild-type, no root hair growth was initiated in axr2-1 drought-induced short roots, although the epidermis was differentiated into trichoblasts and atrichoblasts. On rehydration of the short roots, hair formation occurred from trichoblasts prior to epidermal cell elongation. Therefore, auxin-insensitivity in the axr2-1 mutant did not result in alterations of the hair-forming process itself. The differential development of axr2-1 seedlings, relative to the other auxin-insensitive mutants, suggested that the AXR2 gene has a complex, regulatory function in multiple hormone signaling. Received 26 July 2000/ Accepted in revised form 28 February 2001     

过表达VHA-c4和VHA-c5基因对拟南芥根长的影响

为研究液泡H+-ATPase c亚基VHA-c4和VHA-c5基因在植物生长发育过程中的作用,本研究构建了拟南芥VHA-c4和VHA-c5过表达载体并转化野生型拟南芥,分别获得9个和7个T2代转基因纯合体株系。采用半定量RT-PCR方法对过表达VHA-c4和VHA-c5的转基因纯合体进行阳性鉴定,发现其mRNA表达量均高于对照。对转基因纯合体进行暗培养和正常光照培养,结果显示,黑暗条件下,所有VHA-c4转基因株系的主根变短,而在正常光照下,所有VHA-c5转基因株系的主根变短,推测VHA-c4和VHA-c5分别在黑暗和光照条件下影响植物根的生长。用ABA和糖(葡萄糖和蔗糖)处理转基因纯合体,结果显示它们与野生型的表型无明显差异,表明VHA-c4和VHA-c5基因的过表达没有影响拟南芥对ABA和糖的响应。     

Al Inhibits Both Shoot Development and Root Growth in als3, an Al-Sensitive Arabidopsis Mutant

In als3, an Al-sensitive Arabidopsis mutant, shoot development and root growth are sensitive to Al. Mutant als3 seedlings grown in an Al-containing medium exhibit severely inhibited leaf expansion and root growth. In the presence of Al, unexpanded leaves accumulate callose, an indicator of Al damage in roots. The possibility that the inhibition of shoot development in als3 is due to the hyperaccumulation of Al in this tissue was examined. However, it was found that the levels of Al that accumulated in shoots of als3 are not different from the wild type. The inhibition of shoot development in als3 is not a consequence of nonspecific damage to roots, because other metals (e.g. LaCl3 or CuSO4) that strongly inhibit root growth did not block shoot development in als3 seedlings. Al did not block leaf development in excised als3 shoots grown in an Al-containing medium, demonstrating that the Al-induced damage in als3 shoots was dependent on the presence of roots. This suggests that Al inhibition of als3 shoot development may be a delocalized response to Al-induced stresses in roots following Al exposure.     

蛋白质N-糖基化在拟南芥生长周期中的变化规律及去糖基化对根发育的影响

蛋白质N-糖基化修饰在植物生长发育中发挥重要作用。为探究蛋白质N-糖基化在拟南芥(Arabidopsis thaliana)整个生长周期中的变化规律以及去N-糖基化对拟南芥生根发育的影响,通过N-糖链酶解和HPLC与MALDI-TOF-MS分析解析了不同生长时期的拟南芥Col-0植株的N-糖链组成(结构和含量)变化。以...     

Melatonin Antagonizes Cytokinin Responses to Stimulate Root Growth in Arabidopsis

Melatonin functions as the key growth regulator in various plant species. The mechanisms of the interactions between melatonin and cytokinins remain largely unknown. In this study, the kinetic effects of melatonin over a range of concentrations were investigated. The results showed that melatonin functioned as a positive regulator of root growth ranged from 0.1 to 100 nM. In contrast, exogenous cytokinin at 0.5–1 nM and overexpression of cytokinin biosynthesis gene ISOPENTENYLTRANSFERASE 8 (IPT8) inhibited primary root growth. Combined treatments with melatonin and cytokinin indicated that melatonin antagonized the inhibitory effect of cytokinin 6-benzylaminopurine (6-BA) on primary root elongation. Further analysis revealed that melatonin promotes primary root growth by modulating expression and distribution of auxin efflux transporters PIN2/3 and influx transporter AUX1. Moreover, the cytokinin signaling components AHK4, AHP2/3/5, and type-A ARR15 were down-regulated after melatonin treatment. The polar auxin transport inhibitor 2,3,5-triiodobenzoic acid (TIBA) impaired the promotive effect of melatonin on primary root growth, indicating that auxin transport is essential in melatonin-mediated root growth. Taken together, our data provided evidence to show that melatonin regulates primary root growth in coordination with cytokinin partially through auxin-dependent pathway.

     

Two Seven-Transmembrane Domain MILDEW RESISTANCE LOCUS O Proteins Cofunction in Arabidopsis Root Thigmomorphogenesis

Directional root expansion is governed by nutrient gradients, positive gravitropism and hydrotropism, negative phototropism and thigmotropism, as well as endogenous oscillations in the growth trajectory (circumnutation). Null mutations in phylogenetically related Arabidopsis thaliana genes MILDEW RESISTANCE LOCUS O 4 (MLO4) and MLO11, encoding heptahelical, plasma membrane–localized proteins predominantly expressed in the root tip, result in aberrant root thigmomorphogenesis. mlo4 and mlo11 mutant plants show anisotropic, chiral root expansion manifesting as tightly curled root patterns upon contact with solid surfaces. The defect in mlo4 and mlo11 mutants is nonadditive and dependent on light and nutrients. Genetic epistasis experiments demonstrate that the mutant phenotype is independently modulated by the Gβ subunit of the heterotrimeric G-protein complex. Analysis of expressed chimeric MLO4/MLO2 proteins revealed that the C-terminal domain of MLO4 is necessary but not sufficient for MLO4 action in root thigmomorphogenesis. The expression of the auxin efflux carrier fusion, PIN1-green fluorescent protein, the pattern of auxin-induced gene expression, and acropetal as well as basipetal auxin transport are altered at the root tip of mlo4 mutant seedlings. Moreover, addition of auxin transport inhibitors or the loss of EIR1/AGR1/PIN2 function abolishes root curling of mlo4, mlo11, and wild-type seedlings. These results demonstrate that the exaggerated root curling phenotypes of the mlo4 and mlo11 mutants depend on auxin gradients and suggest that MLO4 and MLO11 cofunction as modulators of touch-induced root tropism.     

IQM1基因过量表达对拟南芥气孔运动及根系生长的影响

拟南芥钙调素结合蛋白IQM家族共有6个成员,已证实IQM1是一个不依赖Ca2+的钙调素结合蛋白,其功能缺失突变体iqm1表现气孔开度小和根短的表型,而且突变体气孔开度并不因光、暗、脱落酸等诱导而变大或变小。该实验构建了IQM1基因双元表达载体并转化拟南芥,通过分子筛选及IQM1表达量分析,获得了IQM1基因过量表达植株。表型分析发现,IQM1过量表达植株在光诱导气孔开放处理后气孔开放度明显比野生型和iqm1-1增大,在暗诱导气孔关闭处理后气孔开度则显著变小;IQM1过量表达植株的主根比野生型和iqm1-1长,侧根数量比野生型和iqm1-1多,但IQM1过量表达对植株的生长形态、抽薹期、开花期及座果等方面却没有明显影响。研究表明,IQM1基因在植物气孔运动及根系生长中起着重要作用。     

Genetic Control of Root Hair Development in Arabidopsis thaliana

Visual examination of roots from 12,000 mutagenized Arabidopsis seedlings has led to the identification of more than 40 mutants impaired in root hair morphogenesis. Mutants from four phenotypic classes have been characterized in detail, and genetic tests show that these result from single nuclear recessive mutations in four different genes designated RHD1, RHD2, RHD3, and RHD4. The phenotypic analysis of the mutants and homozygous double mutants has led to a proposed model for root hair development and the stages at which the genes are normally required. The RHD1 gene product appears to be necessary for proper initiation of root hairs, whereas the RHD2, RHD3, and RHD4 gene products are required for normal hair elongation. These results demonstrate that root hair development in Arabidopsis is amenable to genetic dissection and should prove to be a useful model system to study the molecular mechanisms governing cell differentiation in plants.     

谷胱甘肽转移酶基因过量表达能加速盐胁迫下转基因拟南芥的生长

盐地碱蓬谷胱甘肽转移酶基因(glutathione s-transferase gene,GST)克隆到植物表达载体pROKⅡ35s启动子的下游,通过农杆菌介导,利用花絮浸泡法转化拟南芥.转化子在含有卡那霉素的培养基上经过筛选以后,将初步验证为阳性的转基因植株通过PCR-Southem进一步证实.经过选育,筛选并分离到卡那霉素的抗性并且遗传稳定的T3代纯合子转基因拟南芥品系.通过Northern杂交证实外源基因在转基因拟南芥中表达.在盐胁迫条件下,通过测量转基因植株(GT)和野生型植株(wY)的生物量和谷胱甘肽(氧化型:GSSG;还原型:GsH)发现:转基因植株的生物量较野生型有一定程度的提高;GssG含量在转基因品系中比野生型的含量明显高.因此,过量表达GsT能够提高转基因植株在盐胁迫条件下的生长,而且这很可能是由于还原型谷胱甘肽被氧化的结果.