A Golgi-localized Hexose Transporter Is Involved in Heterotrimeric G Protein-mediated Early Development in Arabidopsis

Helen X. Wang^*, Ravisha R. Weerasinghe^*, Tony D. Perdue^*, Nihal G. Cakmakci^*, J. Philip Taylor^*, William F. Marzluff^*^,, and Alan M. Jones^*^,

Departments of *Biology, Pharmacology, and Biochemistry and Biophysics, The University of North Carolina at Chapel Hill, Chapel Hill, NC 27599-3280

Submitted January 23, 2006; Revised July 3, 2006; Accepted July 12, 2006
Monitoring Editor: J. Silvio Gutkind

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Signal transduction involving heterotrimeric G proteins is universalamong fungi, animals, and plants. In plants and fungi, the bestunderstood function for the G protein complex is its modulationof cell proliferation and one of several important signals thatare known to modulate the rate at which these cells proliferateis D-glucose. Arabidopsis thaliana seedlings lacking the $beta$ subunit(AGB1) of the G protein complex have altered cell division inthe hypocotyl and are D-glucose hypersensitive. With the aimto discover new elements in G protein signaling, we screenedfor gain-of-function suppressors of altered cell proliferationduring early development in the agb1-2 mutant background. Oneagb1-2-dependent suppressor, designated sgb1-1^D for suppressorof G protein beta1 (agb1-2), restored to wild type the alteredcell division in the hypocotyl and sugar hypersensitivity ofthe agb1-2 mutant. Consistent with AGB1 localization, SGB1 isfound at the highest steady-state level in tissues with activecell division, and this level increases in hypocotyls when grownon D-glucose and sucrose. SGB1 is shown here to be a Golgi-localizedhexose transporter and acts genetically with AGB1 in early seedlingdevelopment.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

An evolutionarily ancient mechanism for sensing extracellularsignals involves the heterotrimeric G proteins, composed of ${alpha}$ , $beta$ , and ${gamma}$ subunits. Heterotrimeric G protein complexes link ligandperception via seven-transmembrane (7TM), G protein-coupledreceptors (GPCRs) to downstream effectors. Genes that encodeG protein signaling elements have been identified in amoebae,fungi, plants, and animals, but among all multicellular eukaryotes,plants have the simplest repertoire of G protein elements todate. Specifically, the Arabidopsis genome encodes a singlecanonical G ${alpha}$ and G $beta$ (AGB1) subunit and two G ${gamma}$ subunits and a singleregulator of G signaling (RGS1) protein (Jones and Assmann,2004). There are as yet no plant GPCRs having confirmed ligands,although plants do have a limited set of predicted 7TM proteins(Moriyama and Jones, unpublished data). Similarly, there arefew known downstream effectors that physically interact witheither the plant G ${alpha}$ subunit or the G $beta$ ${gamma}$ dimer. One example is apirin protein (Lapik and Kaufman, 2003), known to serve as atranscriptional cofactor in humans, but with unknown functionin Arabidopsis. Based on either genetic or biochemical tests,G ${alpha}$ effectors in plants also include phospholipase D (Mishra etal., 2006) and ion channels (Aharon et al., 1998; Wang et al.,2001). Recently, we reported that a plant interactor and putativeeffector to G ${alpha}$ is an outer membrane plastid protein designatedTHF1, and this protein together with G ${alpha}$ comprises part of a D-glucosesignaling network (Huang et al., 2006).

In animals and yeast, heterotrimeric G proteins couple a diverseset of signals such as photons, ions, small molecules, sugars,peptides, and protein ligands (Jones and Assmann, 2004) to controla broad range of physiology (Csaszar and Abel, 2001; Rosenkildeet al., 2001; Rockman et al., 2002). Many GPCR ligands stimulatecell proliferation, and these pathways are co-opted in disease(Dhanasekaran et al., 1995; Radhika and Dhanasekaran, 2001).Twelve carcinomas have been linked to mutations in GPCRs, andtwo carcinomas have been associated with activating mutationsin G ${alpha}$ subunits, suggesting a connection between G protein-coupledpathways and cancer and/or cell proliferation. Other mutationsof G ${alpha}$ subunits also have transforming potential when tested incultured cell lines. Virally encoded GPCRs can be essentialfor infectivity or neoplastic potential of the virus, as isthe case for cytomegalovirus infection or Kaposi's sarcoma,respectively (Sadee et al., 2001).

In yeast, the role of the G $beta$ ${gamma}$ (Ste4/Ste18) dimer in regulatingcell proliferation is the best understood. The protein–proteininterface between the three sets of effectors and Ste4 subunitbecomes available after the yeast G ${alpha}$ subunit (GPA1) becomes activated.Ste4 binds three effectors that ultimately regulate gene transcriptionthrough a mitogen-activated protein kinase cascade leading togrowth arrest (Dohlman, 2002). Sugar is an important signalthat controls yeast cell proliferation and size (Vanoni et al.,2005), and the G $beta$ ${gamma}$ dimer is required in most, but not all fungi.

In Arabidopsis, altered cell proliferation either from defectivecell division and/or expansion control is the underlying causefor many of the phenotypes of tissues and organs lacking the $beta$ subunit of the heterotrimeric G protein complex (agb1-2) (Leaseet al., 2001; Ullah et al., 2001, 2003; Chen et al., 2006a).For example, 2-d-old agb1-2 etiolated hypocotyls have one-halfthe number of epidermal cells as wild-type hypocotyls (Ullahet al., 2003). Adult plants have altered morphology, conspicuouslyrounder leaves, larger rosettes, and short siliques, but theyalso have several other quantitative changes as well (see Figure 4of Ullah et al., 2003). Auxin-induced lateral root initiationand high-sugar sensing are also aberrant in the agb1-2 seedlings(Ullah et al., 2001, 2002, 2003; Chen et al., 2003; Chen andJones, 2004). agb1-2 single and agb1-2 gpa1-4 double mutantseedlings grown on 6% D-glucose have a complex response. Seedlingslacking AGB1 are severely hypersensitive to D-glucose. Seedlingsthat are able to germinate on high glucose have greatly expandedepinastic leaves and increased anthocyanin content (SupplementalFigure S1, B and C).

Using a genetic approach, we sought components downstream ofthe G protein complex regulation of cell proliferation and possiblysugar signaling. We found a novel Golgi hexose transporter thatsuppresses some of the loss-of-function G $beta$ phenotypes, includingthe deficiency in hypocotyl development and the altered sugarsensitivity of young seedlings. The biological function of thistransporter was previously unknown and its genetic interactionwith G $beta$ represents the first involvement of the G protein pathwayin sugar transport and the first signal transduction pathwaybetween the Golgi and G $beta$ ${gamma}$ dimer of G proteins in a plant cell.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Screen for Dominant Extragenic Mutations That Suppress the agb1-2 Hypocotyl and Hook Phenotypes and Plasmid Rescue
agb1-2 was transformed with the activation tagging vector, pSK1015,by Agrobacterium-mediated transformation (Bechtold et al., 1993).The activation-tagging vector consisted of four CaMV 35S enhancersand bar gene as a selection maker as described by Weigel etal. (2000). T1 seeds were sterilized (2.5% NaOCl), stratifiedin H₂O for at least 2 d, and then sown on medium at a densityof $~$ 2000 seeds per Petri dish (100 x 15 mm) containing 1/2 Murashigeand Skoog salts (MS), 1% sucrose, 0.5% phyto agar (ResearchProducts International, St. Prospect, IL), pH 5.7, 200 mg/lTimentin. After a 2- to 4-h light pretreatment, seeds were incubatedin the dark at 23°C for 60 h. Control plant seeds were placedon the same plates in a marked area for reference. In total,2,000,000 seedlings were screen without selection for transformation.Because the transformation efficiency was ${approx}$ 1%, we estimate that20,000 seedlings contained the activation tag. Seedlings lookingsimilar to Col-0 were selected as suppressor candidates. Theseplants were transferred into soil and grown at 23°C in long-dayconditions (16 h of light and 8 h of dark). Plasmid rescue usingHindIII-digested SGB1-1^D genomic DNA was carried out as describedby Weigel et al. (2000).

Cloning, Reverse Transcription-Polymerase Chain Reaction (RT-PCR), and Sequencing
SGB1 mRNA (1488 base pairs) was predicted based on the TAIRdatabase information for locus At1g79820 (http://www.arabidopsis.org/abrc).The promoter sequence was defined here as the upstream sequenceof SGB1 between the stop codon of the upstream locus, At1g79830,and start codon of At1g79820. All PCR reactions for cloningwere conducted using high-fidelity Phusion DNA polymerase (Phusion,Espoo, Finland). The PCR products were verified by sequencing.The 14 plasmids generated for this study are listed in SupplementalTable S1 followed by a description of their construction. Theprimers used for cloning, genotyping, and sequencing are listedin Supplemental Table S1. The SGB1 cDNA was PCR amplified usingthe first-strand cDNA and ligated into pENTR D-TOPO (Invitrogen,Carlsbad, CA). For fusion proteins, the SGB1 promoter flankedby NotI in pHW106 was cut and inserted into pHW123 in the NotIsite. The resulting plasmid was recombined with proper destinationvectors to make pHW128, 129 and 130, as listed in SupplementalTable S3. The binary vectors were transformed into Agrobacteriumstrain GV3101 by electroporation. Arabidopsis plants were transformedusing floral infiltration (Bechtold et al., 1993).

The cDNA sequence of Arabidopsis SGB1 was optimized for yeastpreferred codon for the first eight amino acids at the N terminusand the stop codon at C terminus (Supplemental Table S1). Yeastexpression plasmids used in this study contained the ADH promoterfor high-level constitutive expression. The 1.5-kilobase (kb)SGB1 fragment from pHW116, digested with XmaI, was insertedinto the yeast/Escherichia coli shuttle vector p416 ADH in theXmaI site (CEN6 ARSH4 URA3) (Mumberg et al., 1995). The vectorswere either antisense (pHW117) or sense (pHW118). The vectorswere transformed into yeast strains using TE/LiAc/PEG protocol(Clontech, Mountain View, CA). The transformed yeast were grownon synthetic medium (SD) with uracil dropout as the selectionmarker. The medium was supplemented with 2% glucose for allstrains except 2% maltose for the mutant strain EBY.VW4000.

The oocyte expression vector pXFRM contains Sp6 promoter, 5'-and 3'- $beta$ -globin untranslated region regions for efficient translationin oocyte systems (Wang et al., 1999; Sànchez and Marzluff,2002). The SGB1 cDNA with restriction sites NcoI at 5' and XmaIat 3' end was PCR amplified. The PCR product was digested withNcoI and XmaI and inserted into the digested pXFRM vector; thisgenerated pHW136 (SGB1 sense in frame) and pHW139 (with a spontaneousmutation). To make pHW137 with SGB1 antisense, SGB1 fragmentwas cut with XmaI from pHW117 and inserted into XmaI-digestedpXFRM vector.

mRNA levels were determined using a total of RNA isolated fromvarious tissues plants by using RNAeasy plant mini kit (QIAGEN,Valencia, CA). RT PCR was performed using ThermoScrpt RT-PCRsystem (Invitrogen). First-strand cDNA synthesis was performedusing a poly(dT) primer.

Bioinformatics and Cladistics
Unrooted phylogenetic trees (unrooted) were constructed usingthe GeneBee algorithm accessed at http://www.genebee.msu.su/services/hlp/phtree-hlp.html(Brodsky et al., 1992, 1995). Homologues used for constructionsof the phylogenetic trees were chosen from BLAST results byusing the full-length Arabidopsis SGB1 protein sequence againstthe Arabidopsis (cut-off at 4 x 10^–16), yeast (cut-offat 4.8 x 10^–11), and human genomes (cut-off at 8 x 10^–11).Topological models were generated using a topological algorithmto generate unrooted phylogenetic trees for Arabidopsis andyeast comparisons. A cluster model was used in the comparisonto human glucose transporters. Organelle targeting probabilitieswere calculated using TargetP version 1.01 Server from http://www.cbs.dtu.dk/services/TargetP/(Nielsenet al., 1997; Olof et al., 2000), which generated the same dataas in TAIR for At1g79820 (http://www.mitoz.bcs.uwa.edu.au/apmdb/Flatfile-Script.php?chrlocus=AT1G79820.1).

Microscopies
Confocal laser-scanning microscopy was performed on roots, leaves,and seedlings by using a Zeiss LSM510 confocal laser scanningmicroscope (Carl Zeiss, Thornwood, NY). Freshly prepared plantparts were placed on a glass slide in a drop of water and coveredwith a glass coverslip. All images were collected using a ZeissPlanNeofluar 40x numerical aperture 1.3 oil immersion objective.Yellow fluorescent protein (YFP) was visualized using 514-nmexcitation and a 530- to 560-nm bandpass emission filter. Greenfluorescent protein (GFP) fluorescence was visualized using488-nm excitation and either a 505- to 550-nm bandpass or a505-nm longpass emission filter. Root tissues were stained in10 µM rhodamine123 solution (dissolved in water) for 5min at room temperature and washed with distilled water. Confocalimages of rhodamine123 were collected using 543-nm excitationand a 560- to 615-nm bandpass emission filter. Roots were treatedwith MitoTracker Orange CMTMRos for 20 min, and images werecollected using 543-nm excitation and a 560-nm long-pass emissionfilter.

Differential interference contrast (DIC) and fluorescent microscopiesof hypocotyl epidermal cells was performed on an Olympus XI81inverted scope platform (Olympus America, Mellville, NY) usingNomarski optics, and images captured with a Cascade II charge-coupleddevice (Roper, Scientific, Trenton, NJ) and analyzed using IPLaband NIH Image 1.61 software. Seedlings were grown for 2 d inthe dark on 1/2 MS medium supplemented with 1% glucose and thencleared in chloral hydrate. Average cell length was made fromfive cells at each position using multiple hypocotyls.

The Col-0 transgenic seeds bearing with pHW138 (35S::SGB1-GFP)were germinated in the dark at 23°C on 1/2 MS medium with1% sucrose. Six-day-old seedlings were stained with ice-cold1 µM BODIPY 558/568 brefeldin-A (BFA) (Invitrogen) atroom temperature for 20 min. The root hairs were observed usinglaser-scanning confocal microscopy. Root hairs had good penetrationfor BODIPY 558/568 BFA; however, the proper concentration ofthe dye and the age of the root hairs of a seedling are criticalto avoid any effect of the de-esterified BFA, to obtain optimalpenetration, and to avoid background fluorescence.

Assays
The histochemical staining method for $beta$ -glucuronidase (GUS) activityis described by Malamy and Benfey (1997). Briefly, except for2-d-old seedlings, all samples for histochemical analysis inGUS solution were gently degassed for 5 min for plants. Afterstaining overnight, the samples were washed three times andcleared in 75% ethanol, in which samples were also stored.

For yeast growth assays, three independent colonies of eachtransformed yeast strain were cultured overnight on a rotaryshaker at 30°C until the stationary stage (OD₆₀₀ > 1.0)in 5 ml of minimal medium (YNB supplemented with histidine,leucine, and methionine [uracil dropout], containing 2% glucoseand 200 µg/ml Geneticin). The cultures were then dilutedto OD₆₀₀ $~$ 0.1 and grown to an OD₆₀₀ 0.5–1.0. Tenfold serialdilutions were spotted onto minimal medium for plate assays.The plates were cultured for 3 d, and the colonies representingliving cells were counted for comparisons. The hexose transporterdeletion strain EBY.VW4000 was transformed with SGB1 and grownon SD medium (ura dropout) containing 2% glucose for 4 d.

For sugar sensitivity, assays were performed essentially asdescribed by Arenas-Huertero et al. (2000). Sterilized, dryseeds were sown on 1/2 MS medium supplemented with 0–7%D-glucose. Seedlings were grown for 10 d in constant dim light,and the numbers of green plants were scored.

Xenopus Oocyte Expression and Glucose Uptake Assays, SGB1 Antiserum
Construction of plasmids pHW136 through 139 is described inSupplemental Table S3. The plasmid containing the constitutivelyactive human glucose transporter pGLUTX1(LL-AA) construct, togenerate RNA for oocyte injection, was obtained from Dr. MaryCarayannopoulos (Washington University, St. Louis, MO). Thisplasmid harbors mutations in the GLUT coding region, which changeLL amino acids to AA, causing the loss of insulin dependencefor high-level glucose transport. Plasmids were linearized usingEcoRI for pHW137 and pHW139, SacI for pHW137, and SalI for pGLUTX1(LL-AA). Stage V–VI oocytes were injected with 50 ng ofRNA prepared from SGB1 sense and antisense, respectively, andhmGLUTX1 (LL-AA) cDNA. 2-Deoxy-D-glucose (2-DOG) uptake assayswere conducted 3 d after injection of oocytes as described byIbberson et al. (2000), except the amount of injected RNA inthe present study was doubled. Briefly, the oocyte cells wereincubated with 2 mM 2-DOG and 10 µCi of [1,2-³H]deoxy-D-glucose(Sigma-Aldrich, St. Louis, MO) in a volume of 0.5 ml at 23°Cfor 50 min. 2-DOG uptake remains linear at 45 min. Cells werewashed, lysed, and the radioactivity was measured by scintillationcounting.

Antiserum against the SGB1 peptide MRGRHIDKRVPSKEFLSALC conjugatedto keyhole limpet hemocyanin was generated in rabbits. The antiserum(#661) was used at a dilution of 1:5000 for immunoblot analyses.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Screen for Dominant Extragenic Alleles that Suppress agb1-2 Phenotypes
To identify new components required in G protein signaling inplants, we screened $~$ 20,000 T1 seedlings for dominant extragenicalleles (Weigel et al., 2000) that suppress the etiolated hypocotyland hook phenotypes of the G $beta$ null mutant agb1-2 (Figure 1).Eight independent suppressor candidates, designated here assgb-1^D-8^D for Suppressor of G Beta, were found to display, todifferent degrees, both an elongated hypocotyl and a closedhook after 2 d in darkness relative to agb1-2. One of these,sgb-1^D, is the subject of this study. As shown in Figure 1,A and B, the short hypocotyl of agb1-2 at 2 d was partiallysuppressed in the hemizygous sgb1-1^D/homozygous agb1-2 background,whereas the agb1-2 hook phenotype was completely suppressed(Figure 1C).

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Figure 1. sgb1-1^D restores some agb1-2 (G $beta$ ) mutant phenotypes to wild type. (A) Two-day-old etiolated seedlings with the indicated genotype. Wild type Col-0 has a long hypocotyl and closed hook, the parental G $beta$ loss-of-function mutant agb1-2 has a short hypocotyl and opened hook. The suppressor mutant SGB1-1^D, generated in the mutant agb1-2 background fully and partially restored the agb1-2 hook phenotype and hypocotyl phenotypes, respectively. Bar, 1 mm. A minimum of 10 seedlings were used to determine the mean of the hypocotyl length (B) and hook angle degree (C) and corresponding SE of the mean. (D) Rosette size of mature SGB1-1^D/agb1-2 plants is restored to wild-type, whereas leaf shape and serration (E) is (T2) partially restored. Bar, 1 cm.

In addition, the larger rosette size of agb1-2 was also suppressed(Figure 1D) but other agb1-2 phenotypes such as leaf shape (Figure 1F)were only partially suppressed, and others such as silique shape(our unpublished data) were not suppressed at all by the sgb1-1^Dmutation.

Suppressor of G Beta
The sgb1-1^D agb1-2 line contained a single copy T-DNA insertionlocated at position 30,032,723 of chromosome 1, $~$ 1 kb 5' to thestart codon of At1g79820. Four genes were found within a 20-kbregion flanking the insertion (Figure 2A). Therefore, to identifywhich gene was activated, the steady-state mRNA levels of thesefour adjacent genes were analyzed using RT-PCR. Only At1g79820showed an enhanced steady-state mRNA level compared with theparent agb1-2 (Figure 2A).

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Figure 2. Identification of the SGB1 locus and recapitulation of the SGB1-1^D mutant phenotype. (A) The insertion site of a tandem 4X 35S enhancer element in the SGB1-1^D/agb-2 mutant plant (T1) was determined by plasmid rescue. The relative steady-state transcript levels of four genes flanking the T-DNA insert ( $~$ 10-kb length each side) were estimated by semiquantitative PCR using RNA from 2-wk-old rosette leaves (constant light; 22°C) of agb1-2 single and the SGB1-1^D agb-2 double mutants. An elevated steady-state RNA level was found for locus At1g79820, a putative hexose transporter in Arabidopsis. Longer PCR cycling revealed an At1g79820 band in agb1-2. The $beta$ -actin 2 gene served as the normalization control. (B) The steady-state At1g79820 RNA levels in plants harboring a transgene driven by the constitutive 35S promoter-driven were measured by RT-PCR in three independent transformed lines in the agb1-2 genotype (lanes 3–5, lines 1 $->$ 3). Shown for comparison are the steady-state At1g79820 RNA levels in the Col-0 wild-type and agb1-2 genotypes. (C) Recapitulation of the wild-type phenotype in the agb1-2 mutant was performed using 2-d-old seedlings grown in dark. Arabidopsis (agb1-2) was transformed with a 35S CaMV viral promoter driving the expression of the SGB1 cDNA (pHW101). Lines 1 $->$ 3 mimicked the phenotype of the suppressor sgb1–1^D agb1-2 with partially elongated hypocotyl and closed hooks. (D) Quantitation of hypocotyl lengths as a function of D-glucose is shown for wild type (solid diamonds), agb1-2 expressing SGB1 (closed circles), and agb1-2 (open squares). The data are from one experiment repeated twice with the same results. (E) sgb1–1^D/– (hemizygous), agb-2/+ (heterozygous) did not display additional phenotypes. (F) Ectopic expression of SGB1 (35S::SGB1) in agb1-2 has increased cell numbers in developing hypocotyls. ${diamondsuit}$ , Col-0; ${square}$ , agb1-2; $bullet$ , 35S:SGB1,agb1-2. The number and length of epidermal cells of the hypocotyl were determined as described in Materials and Methods. Cell number begins with the basal cell at the root–shoot junction and increases apically toward the hook of the 2-d-old etiolated seedling. The average of the SEM for cell length measurement was ±26 µm.

To confirm that the dominant suppressor phenotypes was a consequenceof overexpression at this locus, the full-length cDNA encodedby the At1g79820 locus was placed under the control of the cauliflowermosaic viral 35S promoter and transformed into the parent agb1-2mutant. Hypocotyl and hook phenotypes of agb1-2 mutant wererestored to wild type in three independent transgenic linesoverexpressing the At1g79820 cDNA in agb1-2 (Figure 2, B andC, lines 1–3, and D). The D-glucose hypersensitivity ofagb1-2 hypocotyls was also rescued when At1g79820 was overexpressed(Figure 2D). These results support our conclusion that enhancedexpression of At1g79820 causes suppression of the agb1 phenotypesin sgb1-1^D agb1-2 and based on these, we designate At1g79820as SGB1. Seedlings that were hemizygous for the SGB1-1^D locusand heterozygous for the agb1-2 allele (i.e., Agb1⁺) exhibitedthe wild-type phenotype (Figure 2E). Because agb1/+, SGB1-1^Dseedlings behaved similarly to wild-type seedlings, this resultsuggests that SGB1-1^D only affects hypocotyl and hook formationin the agb1-2 loss-of-function background. Consistent with thisobservation, overexpression of the SGB1 cDNA (35S::SGB1) inwild-type seedlings did not confer an obvious phenotype in theseassays, nor did it alter morphology or development of adultplants (our unpublished data).

The underlying cause for restoration of the short hypocotylsof agb1-2 seedlings to wild-type hypocotyl lengths when expressionof SGB1 is elevated is due to an increase in cell number (Figure 2F).There were on average 23 cells along a file on the hypocotylepidermis of wild-type seedlings in contrast to 12 cells foragb1-2 hypocotyls similar to values published by Ullah et al.(2003). Seedlings expressing SGB1 under the 35S promoter havefiles comprised of 20 cells. The maximum and minimum cell lengthsfor all three genotypes are similar, indicating that the celldivision defect occurring during early development in agb1-2is restored by SGB1.

Taken together, the dependence of a loss of AGB1 for a phenotypewhen SGB1 is overexpressed suggests that SGB1 lies on the samegenetic pathway as AGB1. It also suggests that AGB1 acts asa positive regulator of SGB1.

SGB1 Encodes a Putative Hexose Transporter
The SGB1 protein, composed of 495 amino acids, has a predictedmolecular mass of 52.4 kDa and an isoelectric point of ${approx}$ 9 foran unphosphorylated form and 6 for a predicted fully phosphorylatedform. The majority of protein topology servers (http://aramemnon.botanik.unikoeln.de)return a prediction for SGB1 having 10–12 transmembrane(TM) domains (Figure 3A, overlying dark lines), a central cytosolicloop and N- and C-terminal internal domains, and two sugar transportsignatures (Figure 3A, double-arrow lines). A 12-TM topologyis typical of sugar transporters in human, yeast, and plants(Marger and Saier, 1993; Buttner and Sauer, 2000; Wood and Trayhurn,2003). SGB1 is most similar to a plastidic glucose transporterin plants (46% identical, 66% similar), to the human glucosetransporter GLUT8 (28% identical, 48% similar), and to YBR241C,a putative transporter in budding yeast (28% identical, 48%similar).

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Figure 3. The architecture of SGB1, a putative hexose transporter and a comparison to yeast and vertebrate homologues. (A) The SGB1 open reading frame encodes 495 amino acids. Partial sequences of SGB1 (At1g79820), a putative plastidic glucose transporter (pGlcT, At5g16150), and a rat glucose transporter 4 (GLUT4, NP_036883), and full-length sequences of human glucose transporter 8 (GLUT8, NP_055395 and an unknown protein from yeast (YBR241C) are aligned using DNA STAR Mega alignment. Regions of SGB1 with high probability to be membrane spanning are indicated by bold horizontal lines. A transmembrane domain hidden Markov model was used for transmembrane prediction. Sugar transporter signature 1 and 2 predicted for SGB1 are indicated by the double-headed arrows. The N-terminal extensions of SGB1 and pGlcT are truncated as is the C-terminal extension on rGLUT4 for space consideration. (B) SGB1 is a member of the monosaccharide transporter (-like) family. There are 49 proteins shown to be similar to SGB1 above a cut-off of 4 x 10^–16 for Arabidopsis. These were analyzed cladistically as described in Materials and Methods. The family is composed of six clades of which functionality has either been determined experimentally for at least one submember or inferred bioinformatically. Arabidopsis SGB1 (designated in this figure as AtSGB1 for cross-genome comparison) is a member of a small group of plastidic glucose transporters. Although none of the Arabidopsis pGlcT have been shown experimentally to transport a monosaccharide, a pGlcT from spinach having high similarity to AtSGB1 has experimental proof (Weber et al., 2000

). Other clades are designated accordingly (http://www.biologie.uni-erlangen.de/mpp/TPer/index_TP.shtml): STPs are sugar transpoters. ERD6 homologues are the early responsive to dehydration stress proteins. PolyolT, XyloseT, and InositolT are transporters of polyol, xylose, and inositol transporters, respectively. (C) Among 31 expressed yeast hexose transporters and glucose sensors having sequence identity to AtSGB1 (cut-off E value = 4.8 x 10^–10), AtSGB1 is most similar to a subgroup of proteins with unknown function. The largest group is the hexose transporter family of S. cerevisiae, composed of 18 proteins (Hxt1–17, Gal2). These proteins and other three maltose transporters (MPH2, MPH3, and MAL11) are essential for metabolic glucose consumption. RGT2 and SNF3 are glucose sensors that generate an intracellular signal inducing expression of glucose transporter (HXT) genes (Ozcan and Johnston, 1999

). A hexose transport deficient strain (EBY.VW4000) was generated through deletions in the 21 genes marked with an asterisk and used for genetic complementation by SGB1. Accession numbers for the yeast homologues are provided in the following Web site with GBS1 protein sequence as a query: http://seq.yeastgenome.org/cgi-bin/nph-blast2sgd. (D) Comparison of Arabidopsis SGB1-16 human hexose transporters. The E value cut-off for selecting the vertebrate sequences was 8 x 10^–11. Accession numbers for the human homologues are provided in the following Web site with GBS1 protein sequence as a query: http://www.ncbi.nlm.nih.gov/blast/Blast.cgi.

SGB1 belongs to a large superfamily of known and putative hexosetransporters with at least 50 members in Arabidopsis (Figure 3B).This superfamily, designated monosaccharide-H+ transporter-like(MST-like) proteins (http://www.biologie.uni-erlangen.de/mpp/TPer/index_TP.shtml),is one of the largest gene families in Arabidopsis, with mostmembers having unknown functionality. The exceptions are theknown sugar transporters (STP1-14, STP clade; Figure 3B) thathave essential function throughout plant development (Saueret al., 1990

; Truernit et al., 1996

, 1999

; Sherson et al., 2000

;Schneidereit et al., 2003

, 2005

; Scholz-Starke et al., 2003

).The large family of Arabidopsis MST-like proteins is composedof several clades. One large clade (STP) is composed of knownand putative glucose transporters. Other clades contain putativeinositol transporters, anion transporters, polyol transporters,and glucose transporters. SGB1 (At1g79820) is a member of theplastidic glucose transporter clade (pGlcT) composed of fouruncharacterized proteins and is annotated as such solely onprotein similarities to a spinach plastid glucose translocator(Weber et al., 2000

). Only one member of pGlcT (At5g16150) hasa predicted chloroplast transit peptide (ChloroP = 0.83). SGB1has a higher probability for mitochondrial targeting (TargetP:mtSP= 0.48) than for chloroplast targeting (ChloroP = 0.23), butneither prediction score strongly supports a mitochondrial orplastidic subcellular location.

SGB1 is similar to putative and known hexose transporters inyeast and humans. Yeast has 32 sugar transporters that fallinto three major clades (Figure 3C). A comparison of ArabidopsisSGB1 (AtSGB1, Figure 3) to the Saccharomyces cerevisiae proteindatabase with a cut-off E value of 4.8 x 10^–10 placesAtSGB1 among a group of unknown proteins, and it is most closelyrelated to YBR241C and VPS73. Cladistic analyses using a clustermodel places SGB1 within the 16 most similar glucose transportersin humans (cut-off E value of 8 x 10^–11). Human GLUT8is the most similar to AtSGB1 (Figure 3, A and D).

SGB1 Transports 2-Deoxy D-Glucose
Heterologous expression in oocytes in conjunction with 2-DOGuptake assays support the predicted hexose transport activityof SGB1. The oocyte assay is a well established in vivo assaysystem for heterologous hexose transport (Gould et al., 1991).Expression levels of SGB1 in oocytes after mRNA injection wasdemonstrated by immunoblot analysis using antisera directedto a 19-amino acid peptide located near the amino terminus ofSGB1, which is predicted to be surface exposed and extracellular.SGB1 was detected in oocytes injected with sense mRNA but notthe negative or positive controls (Figure 4, inset). Two negativecontrols were incorporated. As shown in Figure 4, [³H]2-DOGuptake into oocytes injected with antisense SGB1 RNA and SGB1RNA containing a frame-shift mutation were not significantlydifferent from oocytes injected with buffer alone and were atvalues similar to the nontransport controls reported by Ibbersonet al. (2000) on a per oocyte basis. In contrast, SGB1 senseRNA resulted in 10-fold greater transport than controls andat values similar to the positive control, injection of a constitutivelyactive glucose transporter 1 (Ibberson et al., 2000).

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Figure 4. Deoxyglucose transport. Glucose uptake in oocyte cells overexpressing Arabidopsis SGB1 protein. The indicated RNA (50 ng) was injected into oocyte cells. Glucose uptake was carried out on the third day as described in Materials and Methods. Two negative controls were antisense SGB1 RNA and a frame-shifted mutant RNA of SGB1, which introduces a premature stop codon. The positive control was a constitutively active human glucose transporter designated GLUTX1'LL-AA. The inset shows the immunoblot analysis of oocyte extracts probed with serum directed against SGB1 as described in Materials and Methods.

Complementation analysis with SGB1 tested with several yeastsingle and multiple deletion mutations (Supplemental Table S2)in known and putative hexose transporters (Figure 3C) was performed.However, despite extensive effort, rescue of either strong orweak phenotypes of hexose transporter null lines was not convincing(our unpublished data).

SGB1 Recessive Mutants Mimic agb1-2 Etiolated Phenotypes
A T-DNA-insertion mutant allele of locus At1g79820, designatedhere as sgb1-2 in the Col-0 ecotype was isolated from the SalkInstitute sequence-indexed insertion mutant collection (Alonsoet al., 2003). The T-DNA insertion is located in the highlyconserved region of the penultimate exon (Figure 5A). SemiquantitativePCR revealed the absence of full-length SGB1 transcript, althougha truncated transcript was detectable (Figure 5B). Neither theabsence nor excessive amount of SGB1 had an effect on AGB1 geneexpression (Supplemental Figure S2). The transcript levels ofgenes encoding the other known G protein elements, GCR1 (Pandeyand Assmann, 2004), GPA1 (Ullah et al., 2001), RGS1 (Chen etal., 2003), or the GPA1-interacting protein THF1 (Huang et al.,2006) were not changed by altered expression of SGB1 (SupplementalFigure S2).

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Figure 5. SGB1 recessive mutants have overlapping phenotypes to agb1-2. (A) The sgb1-2 allele contains a T-DNA insertion in the SGB1 gene in the penultimate exon (T-DNA insert not drawn to scale). Arrows represent position of gene primers and arrowheads are T-DNA right border primers. (B) SGB1 mRNA was analyzed in young leaves by using RT-PCR as described in Materials and Methods. Lanes 1 and 2 represent RT-PCR using the 5' and 3' SGB1 primers (arrows). Lane 3 shows the RT-PCR product using the 5' gene primer (left arrow) and the RB primer (arrowhead, Supplemental Table S1). Actin 2 primers in the same reactions were used for normalization (product = 0.9 kb). The SGB1 PCR product is 1.5 kb. The sgb1-2 PCR product is 1.6 kb. (C) sgb1-2 showed similar morphology to agb1-2 with shorter hypocotyls and open hooks. Red arrows mark the positions of the root–shoot transition zone (left arrow) and hook apex (right arrow), respectively, for hypocotyl length comparison. Seedlings were grown on 1/2 MS medium in dark for 2 d. (D) The sgb1-2 mutant was genetically complemented with a 35S driven SGB1 cDNA (D) or a SGB1 promoter-driven SGB1-YFP translational fusion cDNA (E). (F) The agb1-2 sgb1-2, double mutant showed similar 2 d-phenotypes as the parents with open hook and short hypocotyl; no additive or synergistic phenotypes were observed.

Similar to the agb1-2 mutant, 2-d-old etiolated sgb1-2 seedlingsexhibited short hypocotyls and open hooks (Figure 5C). The sgb1-2allele conferred phenotypes that behaved recessively (our unpublisheddata). To confirm that the mutant phenotypes were caused bythe T-DNA insertion at the SGB1 locus, we genetically complementedsgb1-2 mutant plants. Transgenic sgb1-2 plants expressing SGB1(Figure 5D), or the fusions SGB1-YFP or SGB1-GUS (our unpublisheddata), displayed wild-type phenotypes. The observation thatthe sgb1-2 mutant had deficiencies in early development similarto the agb1-2 mutant suggests an associate role of SGB1 withAGB1 in cell division and elongation. Moreover, similar morphologicalphenotypes implicate SGB1 and AGB1 in the same pathway of Gprotein signaling, consistent with the results from the SGB1-1^Dgain-of-function mutants. To test the genetic relationship further,epistasis analysis was performed between the agb1-2 and sgb1-2alleles. The 2-d-old seedlings of the agb1-2 SGB1-2 double mutantgrown on 1% sucrose showed a similar phenotype to agb1-2 orSGB1-2 with short hypocotyls and open hooks (Figure 5F); neitheran additive nor synergistic phenotype was observed.

Together, the recessive sgb1-2 phenotype and the epistasis betweenloss-of-function alleles of agb1 and sgb1-2 suggests that AGB1acts as a positive regulator of SGB1 in the early seedling development.

SGB1 Protein Is Predominantly Expressed in Tissues with Active Cell Division
SGB1 RNA was detected in various tissues of wild-type plantsby RT-PCR (Figure 6A). Consistent with these RT-PCR results,an analysis of gene expression profiling data deposited in theGENEVESTIGATOR database (https://www.genevestigator.ethz.ch)showed that SGB1 mRNA was detectable in a wide range of tissues.No single treatment or tissue type tested to date in the publicdatabase displayed altered SGB1 RNA levels over controls oraverage by more than two-fold. Of particular interest, D-glucosealtered SGB1 expression only 1.3-fold (Genevestigator, versionSeptember 2005). Therefore, to elucidate the differences insteady-state levels of SGB1 protein in various cells due topossible posttranslational control, we transformed both agb1-2and Col-0 with a construct containing the SGB1 promoter drivingthe SGB1 cDNA translationally fused with the GUS gene. Overexpressionof SGB1-GUS in the agb1-2 mutant conferred wild-type hypocotyllength and hook angle, indicating that the SGB1-GUS fusion proteinis active (our unpublished data). High steady-state levels ofSGB1 protein were observed for various sink tissues both inthe presence (wild-type Col-0) and absence (agb1-2) of AGB1protein. The apical and lateral root meristems (Figure 6, Band C), displayed high SGB1 levels. SGB1 protein was also highin anthers/pollen (Figure 6D), embryos, and specific cells ofthe siliques, including the abscission zone of the floral organs(Figure 6E). Dividing, but not mature, leaf cells containedhigh SGB1 levels (cf. Figure 6, F and G). A specific set ofnewly formed cells of vascular traces in expanding leaves wasshown to contain SGB1 (Figure 6H, arrowheads). The SGB1-GUSpattern greatly overlaps the AGB1 expression pattern (Ullahet al., 2003).

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Figure 6. Steady-state levels of SGB1 protein are highest in sink tissues. (A) RT PCR using primers amplifying the full-length 1.5-kb SGB1 cDNA (Figure 5A, arrows), generated from total RNA isolated from the indicated organs. "Leaf" means young leaves only. The $beta$ -actin 2 level was used for normalization. (B–H). Transgenic Col-0 plants expressing a SGB1-translational GUS fusion protein driven by the SGB1 promoter (pHW130) are stained for $beta$ -glucoronidase activity as described in Materials and Methods. (B) Fifteen-day-old root with apical root meristem shown as inset (C) Lateral root. (D) Flower showing anther and pollen staining. (E) Silique showing abscission zone staining (left and right), seed staining (center). (F) Newly divided cells of young leaves of 15-d-old light-grown plants; SGB1-GUS was detectable only in sink/young leaves rather in source/mature leaves. (G) Young leaf. (H) Vascular cells of a young leaf. Mature leaves lacked any detectable GUS activity. At least three lines were analyzed with the representative results shown here. (I). Glucose is a trigger for SGB1 expression in hypocotyls and hooks. Two-day-old transgenic seedlings, bearing the native promoter-driven SGB1-GUS were used to monitor SGB1 responses to sugars. Seeds of transgenic plants bearing pSGB1:SGB1-GUS were grown on 1/2 MS medium supplemented with 0 or 1% glucose, sucrose, sorbitol, inositol, or fructose. Two-day-old etiolated seedlings were stained for GUS activity as described in Materials and Methods. Glucose and sucrose increased the steady-state levels of SGB1 in hypocotyls, hooks, and the entire roots.

Because SGB1 may function in AGB1-dependent sugar sensing (Figures 2Dand S1) and because most signal networks contain feedback regulation,the effect of D-glucose on SGB1 protein level in planta wastested using an SGB1-GUS translational fusion driven by theSGB1 promoter (Figure 6I). Etiolated seedlings grown withoutsugars express SGB1 in root meristems. Application of D-glucosegreatly increased the steady-state level of the SGB1-GUS fusionprotein and its distribution pattern. The D-glucose-inducedincrease was observed predominantly in the hypocotyl and rootapices (Figure 6I, brackets). Similarly, sucrose increased thesteady-state level of SGB1-GUS but with less efficacy. Sorbitol,inositol, and fructose did not alter the levels or distributionpattern of SGB1 over the no-sugar control.

SGB1 Is a Golgi-localized Protein
Arabidopsis plants expressing an SGB1-YFP translational fusiondriven by the SGB1 promoter enabled the determination of thesubcellular localization of SGB1 (Figure 5E). We first experimentallyruled out the predicted (in silico) mitochondrial and/or plastidiclocalizations of SGB1. Root tip cells of transgenic plants bearingpSGB1::SGB1-cyan fluorescent protein (CFP) and counterstainedwith MitoTracker, a mitochondrion-specific fluorescent dye (Invitrogen),revealed that mitochondrial fluorescence did not colocalizewith SGB1-CFP fluorescence (our unpublished data). In addition,chloroplast-containing mesophyll cells expressing an SGB1::GFP fusion protein, reveal no overlap between chlorophyll andGFP (our unpublished data).

SGB1-YFP driven by the native promoter in wild-type (Figure 7B)and agb1-2 null (Figure 7C) backgrounds showed that fluorescencewas observed in root tissues where the SGB1 promoter is active(Figure 6, B and C). Moreover, the fluorescence imaging wasobserved to be in multiple punctate compartments within eachcell, reminiscent of the size, distribution, and number of Golgiapparatus in plant cells (Boevink et al., 1998). Moreover, thedynamics of SGB1-GFP movement (our unpublished data) also matchedpublished Golgi dynamics (http://www.bio.utk.edu/cellbiol/iv/default.htm).Imaging a pSGB1::SGB1-YFP fluorescent construct in plants lackingfunctional AGB1 (Figure 7B) demonstrated that the localizationof SGB1 was not dependent on AGB1 as the fluorescence patternsin Figure 7, B and C, are identical. Finally, because the SGB1steady-state levels are higher in hypocotyl cells when grownon 1% D-glucose (Figure 6I), we examined hypocotyl epidermalcells and found the same punctate pattern for SGB1-YFP localizationas in root cells (our unpublished data).

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Figure 7. SGB1 is localized to the Golgi apparatus. (A) Wild type (Col-0) roots. (B) Imaging of SGB1 promoter-driven SGB1-YFP in the wild-type background. Individual Golgi stacks are seen as punctuate structures rapidly moving throughout the cytosol. (C) Imaging of native promoter driven SGB1-YFP in the agb1-2 background. (D) SGB1-GFP localization is sensitive to brefeldin-A (BFA). GFP imaging of the 35S promoter-driven SGB1-GFP before (untreated) and after (+100 µM BFA) treatment with BFA for 90 min, demonstrating the change in localization. (E) Z-stack reconstruction of 35S::SGB1- GFP expression in leaf tissues before (above) and after (below) 100 mM BFA treatment. (F) High-magnification imaging of a single BFA compartment in a leaf epidermal cell expressing SGB1-GFP. Left, DIC; middle, fluorescence; and right, merge.

To confirm that the observed fluorescence was the Golgi apparatus,BFA was used. BFA has been shown in plants to disrupt the integrityof Golgi stacks, resulting in the fusion of the endoplasmicreticulum (ER) and the Golgi stacks and the formation of socalled "BFA compartments" (Ritzenthaler et al., 2002

). Aftertreatment with brefeldin-A (Figure 7D, bottom), the GFP fluorescencewas observed to change from punctate structures representingthe Golgi to both a diffuse fluorescence representing the fusedER/Golgi compartments and larger punctate structures representingthe newly formed BFA compartments (Ritzenthaler et al., 2002

Z-stack reconstruction imaging of the young leaf epidermal cellsof SGB1-GFP plants before (Figure 7E, untreated) and after BFAtreatment (Figure 7D, +100 µM BFA) clearly demonstratethe effect of BFA on SGB1 localization. Higher magnificationimaging of an individual BFA compartment (Figure 7, F and G)demonstrated that the larger BFA compartments were made up offused smaller compartments, presumably individual Golgi stacks.Figure 7F is a three-dimensional reconstruction from a Z-stackacquisition of control and BFA-treated cells.

Bodipy-BFA has been previously shown to label the Golgi complexin living cells (Deng et al., 1995). We used Bodipy-BFA to stainGolgi in Arabidopsis seedlings expressing SGB1- GFP driven bythe cauliflower mosaic virus (CaMV) 35S promoter. In Arabidopsisroot hair cells, SGB1-GFP showed a predominant colocalizationwith Bodipy-BFA–labeled Golgi stacks that were dispersedin the cytoplasm (Figure 8A, arrowheads). Under these conditions,SGB1-GFP protein was also associated with vesicles typicallysmaller than the Golgi stacks and that did not stain with Bodipy-BFA(Figure 8A, arrow). To further elucidate the localization ofSGB1 and to understand the nature of the small non-Golgi vesicles,we used Arabidopsis seedlings expressing both SGB1-CFP drivenby the SGB1 promoter and the cis-medial Golgi marker ${alpha}$ -mannosidase-YFPdriven by the CaMV 35S promoter. As shown using the Bodipy-BFAGolgi reporter (Figure 8A), SGB1-CFP was observed in Golgi aswell as within rapidly moving small vesicles (Figure 8B andSupplemental Movies S1–3). Interestingly, the additionof 1% D-glucose caused within minutes a decrease in the smallerSGB1-CFP–labeled vesicles (Figure 8B, arrow, and SupplementalMovies S1–3). As can be seen in Figure 8B (bottom), nearlyall the SGB1-CFP fluorescence colocalizes with the Golgi markerafter a low concentration of D-glucose was applied. This redistributionwas most apparent in the supplemental movies where the ratesof movement of the smaller vesicles and the SGB1-CFP–labeledGolgi were perceptively different. Concomitant and commensuratewith the D-glucose–induced decrease in the number of smallvesicles containing SGB1-CFP, the SGB1-labeled Golgi compartmentsincreased. This indicates that the Golgi is the predominantSGB1 compartment and further suggests that D-glucose regulatesthe SGB1 trafficking between the Golgi and as yet unidentifiedsmall vesicle compartments.

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Figure 8. SGB1 is trafficked via Golgi and other vesicles. (A) Imaging of Bodipy-BFA– labeled root hair cells in Arabidopsis plants expressing SGB1-GFP driven by the CaMV 35S viral promoter. Left, localization of SGB1. SGB1 displayed predominant but not exclusive localization to the Golgi Apparatus (middle and right, see arrowheads). However, SGB1 is also found in small vesicles (arrows). (B) Hypocotyl cells of Arabidopsis plants expressing SGB1-CFP (left, false colored magenta) driven by the native SGB1 promoter and the cis-medial Golgi marker ${alpha}$ -mannosidase-YFP ( ${alpha}$ -mann.-YFP, middle, false colored green). Right, merged images where white represents overlap of signals. Addition of 1% D-glucose caused the reduction of SGB1 localization in the rapidly cycling smaller vesicles with a commensurate increase in SGB1 within the Golgi (arrows and Supplemental Movies S1–3).

In summary, four lines of evidence indicate that the predominantbut not exclusive subcellular localization of SGB1 is the Golgiapparatus: 1) the SGB1 compartment share the size, morphology,and dynamics of plant Golgi; 2) BFA reversibly causes the SGB1-GFPfluorescence pattern to collapse into diffuse ER/Golgi punctuatestructures and the previously described BFA compartment derivedfrom the Golgi; 3) SGB1 colocalizes with the Golgi stain Bodipy-BFA;and 4) SGB1 colocalizes with the cis-medial Golgi enzyme ${alpha}$ mannosidase.Moreover, we have shown that SGB1 is found to various degrees,depending on the conditions, in smaller rapidly moving vesiclesand that the addition of D-glucose diminishes their abundancein the cortical region of the plant cell.

DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In metazoans, the G $beta$ ${gamma}$ dimer regulates the activity of phospholipaseC $beta$ , adenyl cyclase (AC), and G protein-coupled inwardly rectifyingpotassium channel potassium channels; however, Arabidopsis lacksthese candidate effectors. Therefore, without directly testablehypotheses for G $beta$ ${gamma}$ activation of plant targets, we sought to definenovel candidate plant effectors that are positively regulatedby the Arabidopsis G $beta$ subunit, AGB1, and/or downstream elementsin the G $beta$ ${gamma}$ signal network. Our approach used activation taggingin a G $beta$ -null genotype with the rationale that overexpressionof G $beta$ ${gamma}$ targets would compensate for the loss of AGB1 activation.Although activation tagging has been useful as a forward genetictool to dissect roles for genes in large families, only recentlyhas it become useful to identify genetic suppressors in Arabidopsis(Li et al., 2002). The emphasis in the present study is suppressionby a dominant allele of a hexose transporter gene of etiolatedhypocotyl length conferred by loss of AGB1.

One of the high D-glucose sensing pathways in yeast uses a G ${alpha}$ subunit (GPA2) to activate AC and ultimately protein kinaseA (Lemaire et al., 2004). Evidence suggests that the activatedform of Arabidopsis GPA1 is also involved in sugar sensing becausergs1 mutants (Chen et al., 2003, 2006b; Chen and Jones, 2004)and GTPase-deficient GPA1 mutants (Huang et al., 2006) are D-glucosetolerant, whereas gpa1 null mutants are hypersensitive to D-glucose(Ullah et al., 2002). However, this does not involve AC activation,and a direct role for the G $beta$ ${gamma}$ subunit has not been demonstrated.We have shown that agb1-2 mutants are severely hypersensitiveto applied D-glucose (Supplemental Figure S1), suggesting thateither the G $beta$ ${gamma}$ dimer is required for G ${alpha}$ recruitment/action or thatthe G $beta$ ${gamma}$ dimer plays a direct role in sugar signal transduction.The latter possibility is favored because D-glucose hypersensitivityin the agb1 mutant (Supplemental Figure S1) is much greaterthan observed for the gpa1 mutants. The greater D-glucose hypersensitivityof the agb1 mutants makes the agb1-2 genotype more suitablefor a robust suppressor screen and thus was our rationale forthe selection of agb1 over gpa1 mutants.

Upon receptor activation, the released G $beta$ ${gamma}$ dimer modulates theactivities of effectors in concert or opposition to the activatedG ${alpha}$ subunit. This action is nearly always constrained to the plasmamembrane, although there are a few examples of G $beta$ ${gamma}$ localizationat a subcellular membrane (Brunk et al., 1999). Because G $beta$ ${gamma}$ ispredominantly found at the plasma membrane and SGB1 is in theGolgi, the genetic interaction between G $beta$ ${gamma}$ and SGB1 is indirectbiochemically. The most likely mechanism involves a secondarymessenger whose production is initiated at the plasma membranebut has a site of action distally, possibly on SGB1.

We have shown that overexpression of a Golgi-localized hexosetransporter is able to restore some phenotypes that result fromthe loss of AGB1. This suggests that the action or subcellulartranslocation of SGB1 is a consequence of AGB1 function or asubset of AGB1-mediated signaling networks. There is a rolefor a mammalian heterotrimeric G protein in the translocationof glucose transporters, although the mechanism is unconventional,and the G ${alpha}$ subtype remains controversial (Patel, 2004; Duganiand Klip, 2005). Nonetheless, these studies raise the possibilityof D-glucose regulation of SGB1 translocation in Arabidopsisand point to future experimentation.

The purpose for D-glucose signaling in plants remains to beelucidated, but it has been suggested that D-glucose controlsenergy carbon homeostasis (Zhou et al., 1998; Sheen et al.,1999; Xiao et al., 2000; Leon and Sheen, 2003; Gibson, 2005)as is known for mammals. We propose here an additional possibility,namely, that external D-glucose may signal growth strategiesin plants as is well known for yeast (Versele et al., 2001;Tamaki et al., 2005). Specifically, we hypothesize that D-glucose,a recognized regulator of cell cycle gene expression in plants(discussed above) and yeast (Vanoni et al., 2005), togetherwith AGB1, already shown to be involved in cell proliferation(Ullah et al., 2003), operate on the same pathway to modulatecell proliferation rates in apical and intercalary meristems.It is most likely that there are many targets to the heterotrimericG protein complex subunits, each resulting in the control ofsome aspect of cell proliferation such as control of the nuclearcycle and cell wall synthesis. A role for a Golgi-localizedhexose transporter is a likely control element for the latter.

The mechanism of sugar sensing in plants may be unique (Sheenet al., 1999; Gibson, 2005); however, as in yeast, downstreamfrom sugar perception lie controls for plant cell proliferationthrough the stability of cyclins, other cell cycle regulators(Riou-Khamlichi et al., 2000; Menges and Murray, 2002; Lorenzet al., 2003; Planchais et al., 2004), and transcription (Thumet al., 2004). Exogenous sugar, especially D-glucose, has profoundeffects on Arabidopsis development, and many of these are knownto involve light perception by the phytochrome photoreceptor.For example, in the etiolated seedling, sugars and phytochromeregulate hypocotyl length and hook angle (Misera et al., 1994;Short, 1999; Ullah et al., 2002; Takahashi et al., 2003; Laxmiet al., 2004). During and after de-etiolation, sugar and lightregulate cotyledon expansion, hypocotyl growth, anthocyaninlevel, and lignin biosynthesis (Dijkwel et al., 1997; Borisjuket al., 1998; Salchert et al., 1998; Rogers et al., 2005).

The concentration of extracellular D-glucose in plants is unknown.It is therefore difficult to evaluate whether applications ofD-glucose above 3%, as shown in Supplemental Figure S1 and inpublished work (Arenas-Huertero et al., 2000), are physiologicallyrelevant or instead induce a neomorphic response through, forexample, a stress mechanism. Extremely high D-glucose levels(molar) are found in tissues such as in fruit, but the levelsof extracellular D-glucose in different tissues have yet tobe determined. The role for high glucose in signaling is anextraordinarily complicated problem to solve, because it musttake into consideration that D-glucose is rapidly taken up,a high concentration of sucrose occurs in apoplastic transportand must encounter localized invertases within their cell walls,cells may have desensitization mechanisms operating as a functionof concentration and exposure time, and there are no physiologicalassays for D-glucose responses with response times in minutesto assess this (current sugar sensitivity assays are in daysusing organ growth acclimated in applied glucose concentrations).In vivo extracellular sensors for D-glucose (Deuschle et al.,2005) are required to answer unequivocally this question, butthese are not yet available. However, indirect measurementshave been applied to address this problem, and estimates ofapoplastic levels of D-glucose at 150 mM (3%) or higher havebeen suggested (McLaughlin and Boyer, 2004; Makela et al., 2005).For example, sorghum embryos develop in as high as 6% apoplasticD-glucose (Maness and McBee, 1986).

Nonetheless, could the suppression by SGB1-1^D be a means tocounter the inability to cope with a glucose stress conferredby the loss of AGB1? Although not to be ruled out, two linesof evidence do not support this. First, the etiolated phenotyperescued by SGB1-1^D and by the overexpression of SGB1 is apparentunder normal physiological conditions (i.e., 1% D-glucose orsucrose; Figures 1 and 2). Second, the increased SGB1 expressiondoes not confer a sugar phenotype when this hypothetical stressis relieved (Figure 2E).

How can increased hexose transport into the Golgi rescue hypocotyllength in the agb1-2 mutant and what is a possible mechanismfor AGB1 action? Hypocotyl growth occurs by cell expansion froma limited set of cells laid down during embryogenesis. agb1-2hypocotyls have a reduced number of cells; consequently, thehypocotyl length is reduced (Ullah et al., 2003). During mitosis,plants build a wall through the secretion and translocationof membrane and wall materials. This type of wall formationrequires de novo wall synthesis of which some components areassembled in the Golgi, most notably the pectins and xyloglucans(Munoz et al., 1996; Baydoun et al., 2001). One possible explanationis that wall synthesis is increased as a consequence of elevatedglucose in the Golgi. Pectins and xyloglucans are internalizedin root cells and subsequently are deposited into the nascentcell plate during division (Baluska et al., 2005). As discussedabove, sugars control the rate of cell division by multiplemeans from control of cell cycle machinery to wall synthesis.Thus, one of the modes of action of AGB1 may be to control glucosetransport into the Golgi directly or indirectly through SGB1,which consequently affects division wall synthesis.

In conclusion, although several hexose transporters have todate been characterized, SGB1 represents the first in the unknownpGlcT clade and the first in plants shown to be localized tothe Golgi apparatus. SGB1 and AGB1 are found in tissues withhigh cell division activity. Most importantly, SGB1 and AGB1genetically operate in the pathway, extending the current evidencethat a heterotrimeric G protein complex plays a role in modulatingcell proliferation in Arabidopsis.

ACKNOWLEDGMENTS

We thank Dr. Jin-Gui Chen for generating the screening populations,Jing Yang for experimental assistance, Dr. Mary Carayannopoulosfor the hGLUTX1 plasmid, the Salk Institute Genomic AnalysisLaboratory and Arabidopsis Stock Center for the T-DNA line materials,and Dr. Boles for the yeast strain EBY.VW4000. We also greatlyappreciate helpful discussions with Drs. N. Allen, P. Morgan,and Z. Chen. Work in A.M.J.'s laboratory on the ArabidopsisG protein is supported by National Institute of General MedicalSciences Grant GM-65989-01, Department of Energy Grant DE-FG02-05ER15671,and National Science Foundation Grant MCB-0209711.

Footnotes

The online version of this contains supplementalmaterial at MBC Online (http://www.molbiolcell.org).

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E06-01-0046)on July 19, 2006.

Address correspondence to: Alan M. Jones (alan_jones{at}unc.edu)

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