Two-dimensional NMR Spectroscopy and Structures of Six Lipid A Species from Rhizobium etli CE3. DETECTION OF AN ACYLOXYACYL RESIDUE IN EACH COMPONENT AND ORIGIN OF THE AMINOGLUCONATE MOIETY

doi:10.1074/jbc.M004009200

Two-dimensional NMR Spectroscopy and Structures of Six Lipid A Species from Rhizobium etli CE3

DETECTION OF AN ACYLOXYACYL RESIDUE IN EACH COMPONENT AND ORIGIN OF THE AMINOGLUCONATE MOIETY^*^,

Nanette L. S. Que, Anthony A. Ribeiro^§, and Christian R. H. Raetz^¶

From the Department of Biochemistry and the ^§ Duke NMR Spectroscopy Center and Department of Radiology, Duke University Medical Center, Durham, North Carolina 27710

Received for publication, May 10, 2000

ABSTRACT

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The chemical structures of six lipid A species (A, B, C, D-1, D-2, and E) purified from Rhizobium etli CE3 were investigatedby one- and two-dimensional NMR spectroscopy. The R. etli lipidA subtypes each contain an unusual acyloxyacyl residue at position2' as part of a conserved distal glucosamine moiety but differin their proximal units. All R. etli lipid A species lack phosphategroups. However, they are derivatized with an $alpha$ -linked galacturonicacid group at position 4', as shown by nuclear Overhauser effectspectroscopy. Component B, which had been not been reported inprevious studies, features a $beta$ , 1'-6 linked disaccharide of glucosamineacylated at positions 2, 3, 2', and 3' in a pattern that is typicalof lipid A found in other Gram-negative bacteria. D-1 containsan acylated aminogluconate unit in place of the proximal glucosamineresidue of B. C and E lack ester-linked $beta$ -hydroxyacyl chains atposition 3, as judged by their H-3 chemical shifts, and may besynthesized from B and D-1, respectively, by the R. etli 3-O-deacylase.D-2 is an isomer of D-1 that forms nonenzymatically by acyl chainmigration. A may be an elimination product derived from D-1 duringhydrolysis at 100 °C (pH 4.5), a step needed to release lipidA from lipopolysaccharide. Based on these findings, we proposea biosynthetic scheme for R. etli lipid A in which B is generatedfirst by a variation of the E. coli pathway. The aminogluconateunit of D-1 could then be made from B by enzymatic oxidation ofthe proximal glucosamine. As predicted by our hypothesis, enzyme(s)can be demonstrated in extracts of R. etli that convert ¹⁴C-labeled B to D-1.

INTRODUCTION

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
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DISCUSSION
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Gram-negative bacteria, such as Rhizobium etli and Rhizobium leguminosarum, belong to a family of select microbes that fixnitrogen during symbiosis within the roots of leguminous plants(1, 2). Lipopolysaccharides (LPS),¹ which coat the outer membranes of the Rhizobiaceae, may playimportant role(s) in this process (3, 4). Mutants of R.leguminosarum and R. etli that lack O-antigen cannot generatefunctional nodules (5-8), and LPS undergoes subtle structuralmodifications during symbiosis, possibly reflecting adaptationsto the root microenvironment (9, 10).

Whether or not the lipid A portion of LPS also plays an important role in symbiosis is unknown. Well characterized R. etlior R. leguminosarum mutants with altered lipid A structures havenot been described. The important studies of Carlson and co-workers(11, 12) have demonstrated that the chemistry of lipid A inR. etli and R. leguminosarum is remarkably different from thatof most other lipid A molecules, suggesting the possibility ofunique biological function(s). Interesting features of R. etlilipid A include the absence of phosphate moieties, the presenceof a galacturonic acid residue at position 4', substitution ofthe proximal glucosamine residue by a 2-aminogluconate unit, andthe presence of an unusual C28 acyl chain (11, 12).

A single R. etli lipid A structure lacking an acyloxyacyl unit was previously proposed (11, 12). We have now developednew chromatographic methods, described in the accompanying article(13), that resolve R. etli CE3 lipid A into six related components,designated A, B, C, D-1, D-2 and E (see Fig. 1). The lipid A speciesof R. leguminosarum 3855 (14, 15) are very similar to thoseof R. etli CE3, as judged by thin layer chromatography.² Chemical analyses and mass spectrometry (13, 16) show thatall six lipid A species of R. etli contain glucosamine but thataminogluconate is present only in components D-1, D-2, and E (seeFig. 1) (13). The masses of the distal units of all six componentsare identical, suggesting a conserved structure (see Fig. 1) (13).The MALDI/TOF mass spectrometry studies furthermore show thatcomponents C and E are 3-O-deacylated versions of B and D-1, respectively(Fig. 1) (13), and may be formed by the 3-O-deacylase presentin R. etli membranes (17).

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Fig. 1. Proposed structures of species B, C, D-1, E, and A isolated from R. etli CE3. Species B and C contain a glucosamine disaccharide unit typical of lipid A molecules found in most other Gram-negative bacteria, including E. coli. D-1 and E feature an aminogluconate unit in place of the proximal glucosamine. All lipid A species of R. etli contain a galacturonic acid substituent at position 4' and an unusual C28 chain that is further substituted at C27, the position labeled as ( $omega$ -1)'2'. Dashed bonds show microheterogeneity with respect to acyl chain lengths or the presence of the $beta$ -hydroxybutyrate substituent. The uniform numbering scheme used to label the key sugar and lipid positions for the NMR analysis (Table I) is indicated in the structure of species B. Roman numerals indicate spin systems. Component A appears to be a chemical degradation product of D-1, and it may contain an aminogluconolactone residue (A. Ribeiro, C. Raetz, and N. Que, manuscript in preparation). D-2 (not shown) is an isomer of D-1 resulting from nonenzymatic acyl chain migration of the ester-linked chain at position 3 to position 5 of the aminogluconate moiety.

We now present the first high resolution NMR structural studies of intact lipid A species purified from R. etli CE3. The R.etli lipid A molecules all yield strong ¹H NMR signals diagnostic of an acyloxyacyl moiety, consistentwith the mass spectrometry discussed in the accompanying article(13, 16). Homo- and heteronuclear one- and two-dimensionalNMR studies reveal that the six lipids feature a conserved distalglucosamine unit with a $beta$ anomeric glycosidic linkage to the proximalunit. The proximal sugar residues of B and C display an anomericproton signal, whereas those of D-1, D-2, and E do not, consistentwith the proposal that B and C contain a conventional glucosaminedisaccharide backbone, as seen in lipid A of most other Gram-negativebacteria. The NMR spectra validate the previously proposed $alpha$ -linkedgalacturonic acid moiety attached to the 4' position of the distalglucosamine in all components (11, 12). Our NMR studies alsodemonstrate that position 3 of the proximal unit in componentsC and E is not acylated. Based on our discovery and structuralcharacterization of B, we propose an enzymatic pathway for theorigin of the aminogluconate moiety, and we present evidence fornovel enzyme(s) in crude extracts of R. etli that rapidly convert¹⁴C-labeled B into D-1.

EXPERIMENTAL PROCEDURES

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INTRODUCTION
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Materials-- Glass backed 0.25-mm Silica Gel 60 thin layer chromatography plates were from Merck. Deuterated solvents (CD₃OD, CDCl₃ with0.1% tetramethylsilane, and D₂O) and 5-mm NMR tubes were purchasedfrom Aldrich. Chloroform, ammonium acetate, and sodium acetatewere obtained from EM Science, whereas pyridine, methanol, andformic acid were from Mallinckrodt. [U-¹⁴C]acetate was purchased from Amersham PharmaciaBiotech.

Bacterial Strains-- R. leguminosarum 3855 (14) was grown at 30 °C in TY broth supplemented with 10 mM CaCl₂. R. etli CE3 (5, 11) was likewisegrown on TY broth supplemented with 10 mM CaCl₂ but with the furtheraddition of 20 µg/ml nalidixic acid and 200 µg/ml streptomycinsulfate.

Isolation and Purification of R. etli Lipid A Components-- The individual lipid A species were purified as described in the preceding paper. To make [¹⁴C]acetate-labeled component B, a 5-ml culture of CE3 was grownto A₅₀₀ = 1 in the presence of 50 µCi of [U-¹⁴C]acetate (50 mCi/mmol). The purification of ¹⁴C-labeled B was achieved by a combination of DEAE-cellulose columnchromatography (18) and preparative thin layer chromatography,as described for nonradioactive B in the accompanying article(13). Approximately 0.05% of the [U-¹⁴C]acetate added to the culture was incorporated intoB.

NMR Spectroscopy-- NMR spectra were recorded on Varian Unity 500 or 600 NMR spectrometers, each equipped with a Sun Sparc 2 data system. Proton-detectedspectra were obtained with a 5-mm Varian inverse probe in theUnity 500 and a 5-mm triple probe in the Unity 600. Proton andcarbon chemical shifts in CDCl₃/CD₃OD/D₂O (2:3:1 v/v/v) are reportedrelative to internal tetramethylsilane at 0.00 ppm with the residualsignal of CD₃OD serving as the secondary reference at 49.5 ppmfor carbon spectra. ¹H spectra at 500 MHz were obtained with a spectral width of 5kHz, a 67° pulse flip angle (6 µs), a 4.8-s acquisition time,and a 2-s relaxation delay (RD) and digitized using 48,000 pointsto obtain a digital resolution of 0.208 Hz/pt.

¹H spectra at 600 MHz were obtained with a 5.4 kHz spectral width, a 67° pulse field angle (4.5 µs), a 4.3-s acquisition time,and a 1-s RD. The spectra were digitized using 48,000 points toobtain a digital resolution of 0.225 Hz/pt.

The two-dimensional sequences from Varian (COSY, TOCSY, and NOESY) were modified to include a long, low power transmitterpulse for solvent signal elimination at a frequency differentfrom nonselective high power pulses at the quadrature detectionfrequency.

The following two-dimensional NMR experiments were performed at 600 MHz. COSY (19, 20) were recorded in the absolute valuemode with a 5.4 kHz spectral width, 2,000 points, a 1-s RD, and160 scans/increment. In these experiments 512 time incrementswere collected and zero-filled to 2,000 points with sine-bellweighting in both dimensions before Fourier transformation, followedby symmetrization of the two-dimensional matrix. TOCSY (21)and NOESY (22) were recorded in the hypercomplex phase-sensitivemode using two sets of 200 time-incremented spectra, 160 scans/increment,a 1-s RD, and a mixing time of 100 ms in TOCSY and 500 ms in NOESY.The final two-dimensional matrices were 2,000 × 2,000 with Gaussianweighting in both dimensions and were notsymmetrized.

Proton-detected single bond ¹H,¹³C two-dimensional chemical shift correlation spectra were recorded using the HMQC method (23,24) with ¹³C decoupling during acquisition. Two sets of 256 time incrementswere obtained in the hypercomplex phase-sensitive mode with 2,000points in t₂. Four hundred scans were recorded per time increment,and the RD was 1.2 s. The two-dimensional data were processedusing Gaussian functions and zero-filled to a final size of 2,000× 2,000.

Conversion of ¹⁴C-Labeled B to ¹⁴C-Labeled D-1 in Crude Cell Extracts-- The reaction mixture (10 µl) consisted of 5 µM ¹⁴C-labeled B (~700 cpm/tube), 0.5-1 mg/ml CE3 membranes, 1 mM MgCl₂, and 50mM MES buffer, pH 6.5. Reactions were stopped after incubationat 30 °C at the indicated times by spotting 4-µl samples ontoa silica gel thin layer plate, which was developed in the solventchloroform/methanol/water/pyridine (40:25:4:2 v/v/v/v). Afterdrying the plate, conversion of B to D-1 was detected and quantifiedusing a Molecular Dynamics Storm PhosphorImager, equipped withImageQuantsoftware.

RESULTS

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

High Resolution ¹H NMR Spectra of Purified R. etli Lipid A Species-- The intact lipid A components of R. etli CE3 have not been available previously for study by high resolution ¹H NMR spectroscopy. The 600 MHz ¹H NMR spectra of components B, C, D-1, E, and A dissolved in CDCl₃/CD₃OD/D₂O(2:3:1 v/v/v) (25) reveal remarkably sharp and well resolvedsugar and acyl resonances, which can be divided into four generalregions (Fig. 2). The downfield signals between 4.5-5.3 ppm correspondto anomeric and acylated oxymethine protons. The resonances between3.5 and 4.5 ppm arise from unsubstituted oxymethine protons, predominantlythose of sugars. The complex multiplets between 2.2 and 2.6 ppmoriginate mainly from the $alpha$ -methylenes of the $beta$ -hydroxyacyl chains,whereas the broader signals around 1.4-1.6 ppm are characteristicof their $gamma$ -methylenes. The 0.9-1.3 ppm upfield resonances areattributed to terminal methyl groups and bulk methylenes, respectively.Solvent resonances between 4.5-4.8 ppm (arising from HOD and CD₃OH)may obscure the anomeric H-1' signal (as with component C in Fig.2) but can be removed with appropriate presaturation pulses (B,D-1, E, and A in Fig. 2) (25).

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Fig. 2. High resolution ¹H NMR spectra at 600 MHz of species B, C, D-1, E, and A purified from R. etli. The NMR spectra were recorded at 25 °C in the solvent, CDCl₃/CD₃OD/D₂O (2:3:1 v/v/v). Sample sizes were typically 1-4 mg in 0.6 ml.

Presence of an Unusual Acyloxyacyl Residue in B and Other R. etli Lipid A Components-- ¹H NMR assignments for B, C, D-1, and E (Table I) were derived from two-dimensional COSY experiments using the anomeric protonsas entry points to elucidate the networks of coupled spin systems.The COSY results (Fig. 3) furthermore provide unequivocal evidencefor the presence of an unusual acyloxyacyl moiety in B and inall other R. etli lipid A components (supplementary figures).The $beta$ -oxymethine protons of the $beta$ -hydroxyacyl chains in lipidA molecules resonate around 3.7-4.2 ppm (like those of sugars),provided the $beta$ -OH moiety is unsubstituted, but are detected near5.2 ppm if the $beta$ -OH is further acylated (26-29). The number andsubstitution of the $beta$ -hydroxyacyl chains present in a lipid Amolecule can be estimated from the number of cross-peak pairsbetween the $alpha$ -methylene (2.2-2.6 ppm) and the $beta$ -oxymethine protons,as well as the $gamma$ -methylene (1.4-1.6 ppm) and the $beta$ -oxymethineprotons. The COSY of B (Fig. 3) displays five $alpha$ / $beta$ and $gamma$ / $beta$ cross-peakpairs.³ The cross-peaks near 2.4 ppm/4.0 ppm (designated $alpha$ 2/ $beta$ 2, $alpha$ 3/ $beta$ 3,and $alpha$ 3'/ $beta$ 3' in Fig. 3) and near 1.5 ppm/4.0 ppm (designated $gamma$ 2/ $beta$ 2, $gamma$ 3/ $beta$ 3, and $gamma$ 3'/ $beta$ 3' in Fig. 3) correspond to what is expected for $alpha$ - and $gamma$ -methylene protons, respectively, adjacent to $beta$ -oxymethinesof unsubstituted $beta$ -hydroxyacyl chains. However, the cross-peakpairs designated $alpha$ 2'/ $beta$ 2' and $gamma$ 2'/ $beta$ 2' in Fig. 3 are considerablyfarther downfield than the others, indicating that this particular $beta$ -oxymethine group is acylated. This pattern of cross-peaks at(2.38, 2.54)/5.12 and (1.6)/5.12 ppm is in fact diagnostic forthe presence of an acyloxyacyl unit in component B of R. etlilipid A. The COSY spectra for the other five purified componentsof R. etli lipid A (A, C, D-1, D-2, and E) reveal identical $alpha$ 2'/ $beta$ 2'and $gamma$ 2'/ $beta$ 2' cross-peaks, as observed in B (Fig. 3), indicatingthat each lipid A component features one acyloxyacyl residue (seesupplementary figures). Similar downfield $alpha$ / $beta$ and $gamma$ / $beta$ cross-peaksare also seen in the COSY of E. coli lipid A, in which two acyloxyacylgroups are known to be present (25).

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Table I
Selected ¹H NMR chemical shifts of CE3 lipid A components
The chemical shifts are taken from COSY experiments. Chemical shifts for B are from Fig. 3, whereas others are from Supplementary Figs. 2-5. Slightly different chemical shifts are seen for certain residues in other experiments (TOCSY, NOESY, and HMQC), most likely arising from small changes in pH or solvent ratios. The numbering is shown in Fig. 1.

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Fig. 3. A 600 MHz two-dimensional ¹H-¹H COSY analysis of species B highlighting the key acyl chain connectivities. The presence of an unusual acyloxyacyl chain is directly indicated by the cross-peaks to the downfield $beta$ -oxymethine designated $alpha$ 2'/ $beta$ 2' and $gamma$ 2'/ $beta$ 2', compared with the remaining $alpha$ / $beta$ and $gamma$ / $beta$ cross-peaks. The cross-peak pairs designated $alpha$ "2"/ $beta$ "2" and $gamma$ "2"/ $beta$ "2" arise from the couplings within the $beta$ -hydroxybutyrate residue. The cross-peaks designated with thick and thin arrows indicate the coupling from the C27 oxymethine to the C26 methylene and C28 methyl groups of the C28 fatty acyl chain in the presence or absence of the $beta$ -hydroxybutyrate substituent, respectively.

Evidence for a $beta$ -Hydroxybutyrate Moiety Esterified to the 27-OH Group in Component B-- The remaining cross-peak pairs designated $alpha$ "2'/ $beta$ "2' and $gamma$ "2'/ $beta$ "2' (Fig. 3) are attributed to the coupling between the $alpha$ -methyleneprotons and the $beta$ -oxymethine proton, and the $gamma$ -methylene protonsand the $beta$ -oxymethine proton of the $beta$ -hydroxybutyrate residue,respectively (Fig. 1). The $beta$ -hydroxybutyrate residue is attachedto the 27-OH group of the C28 acyl chain (11-13). The $gamma$ "2'/ $beta$ "2'cross-peak is seen to resonate significantly upfield relativeto the other $gamma$ / $beta$ cross-peaks (Fig. 3). This pattern is consistentwith that expected for a $beta$ -hydroxybutyrate residue, because its $gamma$ -carbon atom is a terminal methyl group rather than a methyleneunit.

The well resolved multiplet labeled ( $omega$ -1)'2' at 4.92 ppm in Fig. 3 is assigned to the oxymethine proton on C27 of the C28fatty acyl chain (Fig. 1). The downfield position of this protonindicates the C27-OH group must be acylated, presumably with the $beta$ -hydroxybutyrate moiety. There are no cross-peaks detected betweenthe ( $omega$ -1)'2' proton signal and the 2.5 ppm region, indicatingthat the ( $omega$ -1)'2' proton is not coupled to an $alpha$ -methylene group.Instead, the ( $omega$ -1)'2' proton shows cross-peaks near 1.5/1.6 and1.25 ppm (Fig. 3, thick arrows). These are interpreted as evidencefor the coupling of the ( $omega$ -1)'2' proton to the geminal protonson C26 and to the terminal methyl protons on C28, respectively.A minor lipid A species, presumably lacking the $beta$ -hydroxybutyratesubstituent at the 27-OH position, is revealed by the weaker cross-peaksat 3.7/(1.4, 1.3) and 3.7/1.2 ppm (Fig. 3, thin arrows). A specieslacking the $beta$ -hydroxybutyrate group is likewise seen by mass spectrometry(13).

The features of the ¹H NMR spectrum of B attributed to the $beta$ -hydroxybutyrate substituent and the ( $omega$ -1)'2' proton of the C28chain are also detected in species A, C, D-1, D-2, and E (supplementaryfigures). Likewise, the strong cross-peak near 2.4/1.6 ppm, assignedto the $alpha$ and the $beta$ methylene protons of the C28 chain (designated $alpha$ '/ $beta$ '2' in Fig. 3), is seen in the NMR spectra of the other R.etli lipid A components. The conclusion that the acyloxyacyl residueinvolving the unusual C28 chain with its $beta$ -hydroxybutyrate appendageis located at the 2' (rather than the 3') position (Fig. 1) restsprimarily on the mass spectrometry presented in the accompanyingarticle (13).

Sugar Spin Coupling and Assignments in Component B-- Spin coupling connectivities and detailed assignments for the sugar protons are shown in the expanded COSY of component Bfrom 3.5 to 5.5 ppm (Fig. 4). Two glucosamine units and one galacturonicacid residue are observed in the NMR spectra of B, consistentwith mass spectrometry and chemical analyses (13). Unlike lipidA of E. coli, the proximal glucosamine unit of B is not phosphorylated.The major anomeric H-1 (J = 3.4 Hz) of B resonates upfield at5.12 ppm compared with the H-1 of E. coli lipid A at 5.54 ppm(25). Because the proximal glucosamine is not phosphorylated,both $alpha$ and $beta$ anomeric forms are detected by NMR spectroscopy.Indeed, the COSY of B (Fig. 4) reveals four anomeric protons,resonating, respectively, at 5.12 ppm (the major $alpha$ anomeric formof H-1, designated 1), 4.75 ppm (J = 8.3 Hz; the minor $beta$ anomericform of H-1, designated 1 $beta$ ), 4.53 ppm (J = 8.1 Hz; H-1'), and5.23 ppm (unresolved J, estimate < 3 Hz; H-1"). The intensityof the H-1' signal at 4.53 ppm is much reduced because of thepresaturation pulses (25) used to eliminate the solvent lines,but it is nevertheless visible, and its identification is unambiguousfrom its chemical shift and connectivity pattern.

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Fig. 4. Partial 600 MHz two-dimensional ¹H-¹H COSY analysis of species B showing sugar ring connectivities. The labeled cross-peaks indicate the assignments for the two glucosamine and the single galacturonic acid residue. The proximal glucosamine is not phosphorylated, and both $alpha$ and $beta$ anomeric forms are detected. Integration gave estimates of 82% $alpha$ and 18% $beta$ anomeric forms.

The chemical shifts and vicinal coupling constants of the anomeric protons give insights into the configurations and conformationsof the sugar groups (28, 30). The glucosamine H-1 of B resonatesat a relatively low field position (5.12 ppm) and has a smallcoupling constant (J = 3.4 Hz), providing evidence that H-1 isequatorial and the proximal glucosamine unit of B is mostly inthe $alpha$ -anomeric form. Likewise, the relatively low field position(5.23 ppm) and small coupling constant of H-1" (<3 Hz) provideevidence that H-1" is equatorial and that the galacturonic acidmoiety of B has the $alpha$ -anomeric configuration. In contrast, H-1'of the distal glucosamine unit resonates further upfield (~4.53ppm) with an observed coupling constant of 8.1 Hz, consistentwith an axial H-1' and the $beta$ -anomeric configuration. NOESY analysisof B (see below) provides further evidence that H-1' is indeedaxially disposed, as the distal glucosamine of B is found to beattached via a $beta$ , 1'-6 linkage to the proximal glucosamine. H-1"is equatorially disposed with a distinct NOE to the axial H-4',as the galacturonic acid residue is attached via an $alpha$ , 1"-4' linkageto the distalglucosamine.

H-3 and H-3' (5.18 and 5.28 ppm, respectively) of the proximal and distal glucosamine residues of component B are shifteddownfield considerably relative to the other sugar oxymethines(Fig. 4). This indicates that the glucosamine 3 and 3' positionsof B are esterified with acyl chains (Fig. 1), as in lipidA of most other bacteria (25, 26, 31-33). The protons of thegalacturonic acid residue show chemical shifts (Fig. 4 and TableI) and small coupling constants, consistent with the stereochemistryof unsubstituted galacturonic acid. Similar to the case for H-1,H-4' of component B (3.92 ppm) resonates further upfield thanH-4' of E. coli lipid A (4.17 ppm) (25) because of the absenceof a phosphate moiety at position 4' inB.

TOCSY Analysis of Component B-- The two-dimensional TOCSY data confirm the presence of three major sugar spin coupling systems in B (designated I, II, andIII in Figs. 1 and 5), and an additional minor system (designatedI in Fig. 5). These observations strongly validate the assignmentsderived from the COSY experiment (Fig. 4 and Table I). Spin systemsI and I , respectively, correspond to the $alpha$ - and $beta$ -anomericforms of the proximal glucosamine residue, whereas II representsthe distal $beta$ , 1'-6 linked glucosamine. Spin system III arisesfrom the galacturonic acid moiety attached to the 4' positionon the distal glucosamine.

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Fig. 5. Partial 600 MHz two-dimensional ¹H-¹H TOCSY of species B showing sugar ring connectivities. Spin systems I and I correspond to the major $alpha$ -anomeric and minor $beta$ -anomeric forms of the proximal glucosamine unit. Spin system II represents the distal $beta$ , 1-6 linked distal glucosamine. Spin system III arises from the galacturonic acid moiety attached to the 4' position on the distal glucosamine unit.

Evaluation of the Carbon Structure of Component B by HMQC Spectroscopy-- Selection of multiple quantum coherence by two-dimensional HMQC spectroscopy eliminates large deuterated carbon solvent signalsand gives a two-dimensional map connecting protons to their directlybonded carbons. The key features revealed in the HMQC two-dimensionalmap for B (Fig. 6 and Table II) are the number and chemical shiftsof the anomeric carbons and of the C-2 atoms of the glucosamineunits. Three cross-peaks are clearly observed in the anomericregion (90-112 ppm). The resonance at 92 ppm correlates to thepredominant anomeric form of H-1 at 5.12 ppm (Fig. 4) and mustcorrespond to the C-1 of the proximal glucosamine unit. The chemicalshift of 92 ppm supports the $alpha$ -anomeric assignment (28). Thecross-peaks at 102 and 101 ppm, respectively, connect to the 4.6ppm H-1' and to the 5.2 ppm H-1" (both slightly shifted from thevalues in Table I because of gradual solvent evaporation). Theyare therefore identified as C-1' of the distal glucosamine andC-1" of the galacturonic acid residue. The observed chemical shiftsnear 102 and 101 ppm for C-1' and C-1" are consistent with the $beta$ configuration for the distal glucosamine and the $alpha$ form forthe galacturonic acid moieties, respectively (28).

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Fig. 6. Partial two-dimensional HMQC spectrum of species B, showing direct bond ¹H-¹³C correlations within the sugar ring region. The assigned cross-peaks are labeled. Three anomeric cross-peaks are observed. The intensity of the C-1'/H-1' cross-peak is reduced because of the presaturation sequence to suppress the solvent resonances.

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Table II
Selected ¹³C NMR chemical shifts of CE3 lipid A components
The chemical shifts in ppm are taken from HMQC experiments (Fig. 6 for B and Fig. 8 for D-1). Only the predominant forms are reported. For D-1, this is the species with the 3-O-acylated aminogluconate residue. For D-2 it is the 5-O-acylated species. The numbering system is shown in Fig. 1.

The nitrogen-substituted carbons of amino sugars usually resonate near 52-54 ppm (25, 28). Two prominent cross-peaks near53 ppm (C-2) and 55 ppm (C-2') are seen in the HMQC spectrum ofB (Fig. 6), which correlate to the chemical shifts of H-2 at 4.08ppm and H-2' at 3.87 ppm, respectively (Fig. 4). H-2 and H-2'are part of spin systems I and II, respectively, in the TOCSYanalysis (Fig. 5). Spin systems I and II are therefore confirmedto arise from amino sugars (i.e. glucosamine units), based onthe chemical shifts of C-2 and C-2'.

NOESY Analysis of Component B-- A two-dimensional NOESY expansion for B in the sugar region is shown in Fig. 7. H-1' near 4.6 ppm (part of spin system IIof the TOCSY in Fig. 5) displays strong, well resolved intraresidueNOEs to H-3' and H-5'. The multiple intramolecular 1,3-diaxialNOE enhancements seen within the distal sugar are diagnostic ofa $beta$ -linked glucopyranose (25). In addition, H-1' shows strongNOE signals to H-6a and the resolved H-6b of the proximal sugar,providing unequivocal evidence for the $beta$ , 1'-6 linkage. Additionalevidence is seen in the downfield location of C-6 near 68.6 ppm(Table II and Fig. 6) (25, 34, 35) relative to the C-6'signal at 61.6 ppm (Fig. 6 and Table II), which is consistentwith the view that 6'-OH is not glycosylated.

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Fig. 7. Partial 600 MHz ¹H-¹H two-dimensional NOESY analysis of species B. With the diagonal phased negatively, the two-dimensional NOE cross-peaks phased negatively. Diagnostic NOEs are detected from H-1" (5.23 ppm) to H-2" (3.77 ppm) within the galacturonic acid moiety and to H-4' (3.92 ppm) in the distal glucosamine unit (interglycosidic). In addition, cross-peaks are seen between H-1' (4.53 ppm) and H-3' (axial), and H-5' (axial) within the distal glucosamine sugar, and to H-6a and H-6b in the proximal glucosamine unit (interglycosidic). A NOE from H-1 to H-2 is also detected within the proximal glucosamine. The mixing time was 500 ms.

H-1 of the proximal glucosamine and H-1" of the galacturonic acid moiety display strong NOE signals to their respective H-2and H-2". A single intramolecular (axial-equatorial) anomericH-1 to H-2 NOE of this kind is diagnostic for $alpha$ -linked gluco-and galactopyranoses. H-1" shows one additional strong NOE signal(Fig. 7) that can be attributed to H-4', providing evidence foran $alpha$ , 1"-4' glycosylation of the distal glucosamine by the $alpha$ -galacturonicacid residue. In addition, the C-4' signal at 75.7 ppm is significantlydownfield of the C-4 resonance at 68.8 ppm, consistent with theproposed glycosylation of the 4'-OH group (Fig. 6 and Table II).

Overall, the NOESY data provide strong NMR evidence for the locations and configurations of the glycosidic linkages in R.etli component B to be $alpha$ -GalUA(1 $right-arrow$ 4)- $beta$ -GlcN(1 $right-arrow$ 6)- $alpha$ / $beta$ -GlcN.Our findings confirm the GalUA attachment site deduced previouslyby methylation analysis of the unresolved R. etli lipid A mixture(11).

Absence of a Proximal Glucosamine Unit in Species D-1, D-2, and E-- The HMQC spectra of D-1 (Fig. 8), D-2 (not shown), and E (not shown) reveal only two anomeric carbon/proton cross-peaks. Theseare C-1'/H-1' (102/4.55 ppm) from the distal $beta$ -glucosamine unitand C-1"/H-1" (101/5.21 ppm) from the $alpha$ -galacturonic acid residue.In fact, scrutiny of the cross-peaks assigned to the galacturonicacid moiety, the distal glucosamine unit, and the C28 chain withits appended $beta$ -hydroxybutyrate group reveals them to be essentiallythe same in both D species and B. The strong C-1/H-1 cross-peak(92/5.12 ppm) arising from the proximal glucosamine unit of B(Fig. 6) is not observed in D-1, D-2, and E, which contain a proximalaminogluconate unit (Fig. 8 for D-1). The presence of a carbonylgroup at C-1 in the proximal unit of the two D species and E issupported by the +4 to 5 ppm downfield ¹³C shift of the C-2/H-2 cross-peak from 53/4.08 ppm in B (Fig.6) to 57-58/4.42 ppm in the D species and E (Fig. 8 and TablesI and II). As in component B, the C-6 signals of D-1, D-2, andE (69-71.8 ppm) are downfield relative to their respective C-6'resonances (61-62 ppm) (Fig. 8 and Table II) indicative of glycosylationof the 6-OH group. The HMQC data thus provide the initial evidencefor the presence of a $beta$ , 1'-6 linkage between the distal glucosamineand the aminogluconate unit of the D-1, D-2, and E species.

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Fig. 8. Partial two-dimensional HMQC spectrum of species D-1, showing direct bond ¹H-¹³C correlations within the sugar ring region. The assigned cross-peaks are labeled. Comparison with Fig. 6 reveals that the C-1'/H-1', C-1"/H-1", and C-2'/H-2' cross-peaks in D-1 resonate at almost identical shifts as those in B. However, the C-2/H-2 cross-peak at 53.0/4.08 ppm in B is shifted to 57.0/4.42 ppm in D-1, and the C-1/H-1 cross-peak is not seen in D-1, consistent with the presence of a proximal aminogluconate unit in D-1.

As discussed in the accompanying article (13), D-1 and D-2 display identical positive and negative ion MALDI/TOF mass spectra,suggesting that they are isomers. NMR spectroscopy directly showsthat D-1 and D-2 differ in an unusual positional isomerizationspecifically localized in the proximal aminogluconate residue(Supplementary Figs. 3 and 4). However, the COSY cross-peaks arisingfrom the distal glucosamine and the galacturonic acid moiety inD-1 and D-2 are quite similar and closely match their correspondingsignals inB.

The COSY analysis for the proximal aminogluconate unit is found to be considerably more complicated. Expansion of the COSY(Fig. 9a) of a freshly isolated preparation of D-1 reveals a distinctdouble-doublet (H-3 at 5.03 ppm; short arrow in Fig. 9a) withresolved J couplings = 3.7 and 7.4 Hz and strong COSY cross-peaksto H-2 (4.42 ppm) and H-4 (4.00 ppm). This indicates that themajor isomer D-1 can be assigned as a 3-O-acylated aminogluconateunit. An adjacent, nearly resolved, less intense multiplet (5.05ppm; long arrow in Fig. 9a) reveals a different connectivity pattern(Fig. 9a, D-2 subscript), with less intense COSY cross-peaks tononequivalent H-6 resonances (3.78 and 4.16 ppm) and to H-4 (3.81ppm) (Fig. 9b, upper spectrum, diagonal arrows). This findingindicates that a small amount of the D-2 isomer can be detectedin fresh D-1 preparations and that D-2 can be assigned as a 5-O-acylatedaminogluconate unit. Integration gave relative ratios of 70:30for the 5.03 ppm double-doublet and 5.06 ppm multiplet, and theirsum approaches that of the singly resolved H-1" (5.20 ppm) andthe $beta$ -oxymethine proton (5.12 ppm) (Fig. 9b).

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Fig. 9. Partial 600 MHz two-dimensional ¹H-¹H COSY analyses of freshly isolated D-1 and D-2 samples, showing sugar ring connectivities. a, the COSY cross-peaks arising from the galacturonic acid and the distal glucosamine unit in D-1 are similar to those observed for B (Fig. 6) and for D-2 (full spectrum not shown). However, even in a fresh sample of D-1, the proximal aminogluconate unit is revealed by NMR spectroscopy to be a mixture of a major 3-O-acylated form (authentic D-1) and a minor 5-O-acylated aminogluconate species (likely to be D-2, as labeled), which arises by a slow intramolecular trans-esterification. b, expansion of the acylated aminogluconate resonances of fresh D-1 and D-2 samples. The expanded D-1 spectrum reveals a prominent double-doublet at 5.03 ppm (H-3), which correlates to H-2 and H-4 in the COSY, providing evidence that this represents a 3-O-acylated species. A less prominent multiplet at 5.07 ppm (assigned to H-5 of the contaminating D-2 in the D-1 sample) correlates to H-6a, H-6b, and H-4 of the D-2 form in the COSY (indicated by the diagonal arrows). Integration of the D-1 spectrum yields estimates of 70% 3-O-acylated (D-1) and 30% 5-O-acylated (D-2) species in the fresh D-1 sample. Expansion of the acylated aminogluconate resonances in a fresh D-2 sample reveals a prominent multiplet at 5.04 ppm, which overlaps and obscures a less intense double-doublet (because of contaminating D-1). COSY reveals the prominent multiplet to correlate to H-6a, H-6b, and H-4 (indicated by the diagonal arrows) in D-2, thus indicating that the 5-O-acylated species is dominant in this sample. However, the COSY analysis also reveals "weaker" cross-peaks to H-2 and H-4, suggesting that the minor species present as an impurity in D-2 is in fact the 3-O-acylated isomer (contaminating D-1).

Upon standing, the D-1 sample equilibrated to a 55% D-1 and 45% D-2 mixture (not shown). The proximal aminogluconate thusbehaves as a mixture of major and minor isomers that presumablyarise by a slow intramolecular trans-esterification reaction betweenC-3 and C-5, which occurs during the time required for sampleisolation and NMR analysis. Hence, we conclude that the predominantform of the proximal sugar in D-1 is 3-O-acylated, which is likelyto be the physiologically relevantspecies.

Further Studies of the Nonenzymatic Interconversion of D-1 and D-2-- The relationship between D-1 and D-2 as equilibrating species was further documented by the following experiments: 1) A freshlyprepared solution of D-2 exhibited the reciprocal NMR behaviorof D-1, revealing a dominant broad multiplet at 5.06 ppm, whichoverlaps and obscures a small double-doublet at 5.04 ppm (Fig.9b). COSY analysis (Fig. 9b, lower spectrum) of this fresh D-2solution now reveals less intense cross-peaks to the double-doubletand more dominant cross-peaks to the broad multiplet. This findinggives evidence that D-2 consists predominantly of the 5-O-acylatedaminogluconate unit, with a minor contribution from the 3-O-acylatedD-1. 2) When fresh D-1, dispersed in 50 mM aqueous MES, pH 6.5,and 0.1% Triton X-100, is incubated overnight at room temperature,TLC analysis in the system CHCl₃/pyridine/formic acid/methanol/H₂O(60/35/10/5/2 v/v/v/v/v) reveals the gradual formation of D-2(Fig. 10). Conversely, fresh D-1 gradually forms from D-2 incubatedunder similar conditions at room temperature (Fig. 10). The sameslow interconversions occur in the ternary solvent used for theNMR experiments.

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Fig. 10. TLC analysis of the nonenzymatic interconversion of D-1 and D-2 after overnight incubation. Following incubation overnight in 50 mM aqueous MES, pH 6.5, and 0.1% Triton X-100, D-2 gradually appears in freshly isolated sample of D-1 (lane 1), whereas D-1 is generated in a sample of D-2 (lane 2). The 3-O-deacylated species E remains unchanged under these conditions (lane 3). The interconversion of D-1 and D-2 presumably occurs by a slow intramolecular acyl chain migration.

Component E-- Results from MALDI/TOF spectrometry showed that component E is related to D-1/D-2 but is missing one fatty acyl chain fromthe proximal sugar (13). The mass spectrometry methods werenot able to establish whether the 2- or 3-position is deacylatedin E. The two-dimensional COSY of E (Supplementary Fig. 5), however,shows that the downfield H-3 peak observed in B and D-1 is absentin E. Instead, H-2 of the aminogluconate residue of E displaysa distinct COSY connectivity with an upfield resonance at 4.21ppm, which is assigned as the H-3 of E. Thus, E is the 3-O-deacylatedderivative of D-1. Likewise, C is not acylated at the 3-position(H-3 at 3.68 ppm in Supplementary Fig. 2) but is otherwise thesame as B by NMRanalysis.

A striking difference between the COSY analysis of E and D-1/D-2 is that the proximal aminogluconate of E displays a verysimple spectrum (Supplementary Fig. 5). This result strengthensthe interpretation of the complexities in the spectra of D-1 andD-2 as arising from fatty acyl migration within the proximal aminogluconateunit. Once the 3-position is deacylated in E, acyl chain migrationon the aminogluconate moiety is no longerpossible.

Origin and Properties of Component A-- MALDI/TOF mass spectrometry does not readily reveal the relationship of A to the other species. The [M $-$ H] signal of A cannot be explained by a simple deacylation of eitherB or D-1. However, upon subjecting D-1 to hydrolysis at pH 4.5,under the same conditions needed to release the lipid A componentsfrom R. etli LPS (100 °C), a more rapidly migrating species similarto A is formed (data not shown). No band corresponding to A isobserved when B or D-2 are hydrolyzed at pH 4.5. Thus, A appearsto originate from D-1 as a consequence of the conditions usedto cleave the 3-deoxy-D-manno-octulosonic acid-lipid A linkage.The COSY analysis of A is shown in Supplementary Fig. 1. Evidencefor the proposed structure of A (Fig. 1) will be presentedelsewhere.

Conversion of B to D-1 by R. etli or R. leguminosarum Membranes-- When ¹⁴C-labeled, purified component B is incubated with R. etli or R. leguminosarum membranes, TLC analysis at various timepoints demonstrates robust conversion of B to a more polar speciesthat migrates with purified ¹⁴C-labeled D-1 (Fig. 11). This observation lends credence to ourproposal (Fig. 12) that the aminogluconate residue in D-1 is generatedby the oxidation of the proximal glucosamine of B and supportsthe view that components B and D-1 are both physiologically importantspecies.

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Fig. 11. Rapid enzymatic conversion of B to D-1 by R. etli membranes. Upon incubation with R. etli or R. leguminosarum membranes, ¹⁴C- labeled B is converted to a more polar ¹⁴C- labeled species that migrates with purified standard of D-1.

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Fig. 12. A hypothetical pathway for the biosynthesis of the aminogluconate moiety of R. elti lipid A species D-1. Following the formation of component B, by the indicated pathway, a novel oxidation of the proximal glucosamine residue is proposed. If the reaction proceeds through a lactone intermediate (not shown), an additional lactonase would be needed to generate D-1. All the enzymes needed to generate component B have been detected (36, 37, 44), with the exception of the reactions that incorporate the galacturonic acid and the $beta$ -hydroxybutyrate residues.

	DISCUSSION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

The lipid A species of R. etli and R. leguminosarum are strikingly different from those of other Gram-negative bacteria (Fig.1). We are studying the biosynthesis of R. etli lipid A to identifynovel lipid A-modifying enzymes and the genes encoding them. Sofar, we have discovered a 4'- and a 1-phosphatase (36, 37),a C28 acyltransferase (38), and a 3-O-deacylase (17), allof which appear to be unique to the R. etli system when comparedwith E. coli. However, the enzyme(s) that incorporate the 4'-galacturonicacid residue and the proximal aminogluconate unit of R. etli lipidA (Fig. 1) are not yet known, in part because of uncertaintiessurrounding the structure of R. etli lipid A. Consequently, wedecided to reinvestigate R. etli lipid A, using new conditionsfor lipid A purification (13) and improved procedures for highresolution NMR spectroscopy (25).

In this and the accompanying paper (13), we have presented a more complete structural picture of R. etli lipid A than previouslyproposed (Fig. 1). Our analyses of intact lipid A molecules isolatedfrom whole cells by hydrolysis at pH 4.5 have revealed that lipidA of R. etli consists of a mixture of at least six structurallyrelated but distinct components rather than a single species.Four of these (B, C, D-1, and E) appear to be physiologicallyrelevant, whereas A and D-2 are probably formed during hydrolysisandpurification.

In the current study, the substitution patterns and glycosidic linkages of the lipid A species of R. etli were directly analyzedby NMR methods without the need for cumbersome chemical modificationsand/or fragmentation. Our NMR procedures enable the study of lipidA molecules in their intact state and provide independent validationof conclusions derived from destructive methods. Indeed, our NMRdata in conjunction with the mass spectrometry presented in theaccompanying article (13) are in complete accord and providea coherent proposal for the revised R. etli lipid A structuresshown in Fig. 1. The two-dimensional NMR methods that we haveemployed have also allowed identification of the sites of deacylationin components C and E. The 3-O-deacylase that has recently beendiscovered in R. leguminosarum and R. etli membranes (17) nicelyaccounts for these species as derivatives of B and D-1,respectively.

Most significantly, several specific cross-peaks are observed in the COSY analysis of all six lipid A components (Fig. 3 andsupplementary figures) that are diagnostic of the presence ofan unusual acyloxyacyl moiety in each of these molecules (Fig.1). In previous work, the absence of an acyloxyacyl residue wasexplicitly proposed based on the failure of R. etli lipid A torelease an acyloxyacyl unit following Kraska methylation (11).However, no direct physical studies of purified, intact R. etlilipid A molecules were reported prior to the presentinvestigation.

Establishing the presence or absence of an acyloxyacyl moiety in a lipid A molecule is critical, because this functionalityis often necessary for effective stimulation of the innate immunesystem of animals (39, 40). Whether or not certain types oflipid A can also induce innate immune responses in plants is unknown.Recent evidence supports the idea that plants may have evolvedsystems of innate immunity, perhaps analogous to the Toll-likereceptor system for lipid A in animals (41, 42). Interestingly,tobacco leaves develop disease resistance in response to certaintypes of infused lipopolysaccharides (43). We favor the viewthat the unusual structure of lipid A in R. etli somehow facilitatessymbiosis by masking the potential immuno-stimulatory activitythat might be associated with a more conventional (phosphate-containing)lipid A structure. Perhaps, the plant does not reject the R. etliendosymbiont because R. etli lipid A is not recognized by theinnate immune system of the plant. In this scenario, the plantcould still respond to infections by Gram-negative pathogens thatpossess a conventional phosphate-containing lipid A moiety, whileretaining the nitrogen-fixingendosymbiont.

The analytical methods that we have developed and the microheterogeneity that we have documented allow us to formulate forthe first time a specific hypothesis regarding the enzymatic originof the aminogluconate unit in D-1 and E (Fig. 12), a biochemicalentity that has not been described in other systems. Our abilityto test this hypothesis relies entirely upon our preparation ofa pure sample of ¹⁴C-laleled B (Fig. 11). This approach would not have been possiblewithout the identification and availability of a nonradioactivestandard of B, characterized by definitive structural criteria,as described above. Our initial in vitro experiment clearly revealsthat R. etli and R. leguminosarum membranes contain enzyme(s)capable of metabolizing ¹⁴C-labeled B to a product that migrates like D-1, as judged byTLC (Fig. 11). This membrane-bound activity is highly efficient(Fig. 11) and is likely to be the first example of an oxidationof a lipid A-like molecule. Further characterization of this interestingnew system isunderway.

The genes encoding the unique lipid A-modifying enzymes of R. etli have not yet been identified, but if available, they couldbe exploited in various important ways. For instance, they couldbe used in the production of hybrid lipid A structures in recombinantbacterial strains, possibly giving insights into the functionsof lipid A in outer membrane assembly and providing new systemsfor the development of vaccines and adjuvants. It will also beof great interest to determine how novel hybrid lipid A structuresprepared with specific R. etli enzymes affect the innate immuneresponses of animals or plants, in comparison with those thatthat are normally elicited by E. coli or Salmonella lipid A. Lastly,defined mutations in the biosynthesis of R. etli lipid A shouldpermit meaningful structure/function studies of lipid A duringthe establishment of symbiosis and nitrogen fixation in leguminousplants.

FOOTNOTES

^* This work was supported by National Institutes of Health Grant R37-GM-51796 (to C. R. H. R.). The Duke University NMR Centeris supported in part by National Institutes of Health Grant P30-CA-14236.NMR instrumentation was also funded by grants from the NationalScience Foundation, the National Institutes of Health, the NorthCarolina Biotechnology Center, and Duke University.The costs ofpublication of this article were defrayed in part by the paymentof page charges. The article must therefore be hereby marked "advertisement"in accordance with 18 U.S.C. Section 1734 solely to indicate thisfact.

The on-line version of this article (available at http://www.jbc.org) contains additionalfigures.

^¶ To whom correspondence should be addressed: Dept. of Biochemistry, Duke University Medical Center, Box 3711, Durham, NC 27710.Tel.: 919-684-5326; Fax: 919-684-8885; E-mail: raetz@biochem.duke.edu.

Published, JBC Papers in Press, June 15, 2000, DOI 10.1074/jbc.M004009200

² N. L. S. Que and C. R. H. Raetz, unpublishedresults.

³ The atom-labeling scheme is defined in Fig. 1. The pairs arise because of the nonequivalence of the magnetic environmentsof the geminal $alpha$ -methylene protons of the $beta$ -hydroxyacylsubstituents.

ABBREVIATIONS

The abbreviations used are: LPS, lipopolysaccharide; MALDI/TOF, matrix-assisted laser desorption ionization/time of flight; GalUA, galacturonic acid; COSY, correlation spectroscopy; TOCSY, total correlation spectroscopy; NOE, nuclear Overhauser effect; NOESY, NOE spectroscopy; HMQC, heteronuclear multiple-quantum coherence spectroscopy; RD, relaxation delay; MES, 4-morpholineethanesulfonic acid.

	REFERENCES

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

1.	Long, S. R., and Staskawicz, B. J. (1993) Cell 73, 921-935
2.	Spaink, H. P., Kondorosi, A., and Hooykaas, P. J. J. (1998) The Rhizobiaceae: Molecular Biology of Model Plant-associated Bacteria , Kluwer, Dordrecht, The Netherlands
3.	Kannenberg, E. L., and Brewin, N. J. (1994) Trends Microbiol. 2, 277-283
4.	Carlson, R. W., Bhat, U. R., and Reuhs, B. (1992) in Plant Bio/Technology and Development (Gresshoff, P. M., ed) , pp. 33-44, CRC Press, Boca Raton, FL
5.	Noel, K. D., Vandenbosch, K. A., and Kulpaca, B. (1986) J. Bacteriol. 168, 1392-1401
6.	Priefer, U. B. (1989) J. Bacteriol. 171, 6161-6168
7.	Kannenberg, E. L., Rathbun, E. A., and Brewin, N. J. (1992) Mol. Microbiol. 6, 2477-2487
8.	Perotto, S., Brewin, N. J., and Kannenberg, E. L. (1994) Mol. Plant Microbe Interact. 7, 99-112
9.	Sindhu, S. S., Brewin, N. J., and Kannenberg, E. L. (1990) J. Bacteriol. 172, 1804-1813
10.	Tao, H., Brewin, N. J., and Noel, K. D. (1992) J. Bacteriol. 174, 2222-2229
11.	Bhat, U. R., Forsberg, L. S., and Carlson, R. W. (1994) J. Biol. Chem. 269, 14402-14410
12.	Forsberg, L. S., and Carlson, R. W. (1998) J. Biol. Chem. 273, 2747-2757
13.	Que, N. L. S., Lin, S., Cotter, R. J., and Raetz, C. R. H. (2000) J. Biol. Chem. 275, 28006-28016
14.	Brewin, N. J., Wood, E. A., Johnston, A. W. B., Dibb, N. J., and Hombrecher, G. (1982) J. Gen. Microbiol. 128, 1817-1827
15.	Kadrmas, J. L., Allaway, D., Studholme, R. E., Sullivan, J. T., Ronson, C. W., Poole, P. S., and Raetz, C. R. H. (1998) J. Biol. Chem. 273, 26432-26440
16.	Que, N. L. S., Basu, S. S., White, K. A., and Raetz, C. R. H. (1998) FASEB J. 12, 1284 (abstr.)
17.	Basu, S. S., White, K. A., Que, N. L., and Raetz, C. R. (1999) J. Biol. Chem. 274, 11150-11158
18.	Raetz, C. R. H., and Kennedy, E. P. (1973) J. Biol. Chem. 248, 1098-1105
19.	Bax, A., R., F., and Morris, G. A. (1981) J. Magn. Reson. 42, 164-168
20.	Bax, A., and Freeman, R. (1981) J. Magn. Reson. 44, 542-561
21.	Bax, A., and Davis, D. G. (1985) J. Magn. Reson. 65, 355-360
22.	Jeener, J., Meier, B. H., Bachmann, P., and Ernst, R. R. (1979) J. Chem. Phys. 71, 4546-4552
23.	Summers, M. F., Marzili, L. G., and Bax, A. (1986) J. Am. Chem. Soc. 108, 4285-4294
24.	Bax, A., and Subramanian, S. (1986) J. Magn. Reson. 67, 565-569
25.	Ribeiro, A. A., Zhou, Z., and Raetz, C. R. H. (1999) Magn. Res. Chem. 37, 620-630
26.	Takayama, K., Qureshi, N., Mascagni, P., Nashed, M. A., Anderson, L., and Raetz, C. R. H. (1983) J. Biol. Chem. 258, 7379-7385
27.	Takayama, K., Qureshi, N., Mascagni, P., Anderson, L., and Raetz, C. R. H. (1983) J. Biol. Chem. 258, 14245-14252
28.	Agrawal, P. K. (1992) Phytochemistry 31, 3307-3330
29.	Agrawal, P. K., Bush, C. A., Qureshi, N., and Takayama, K. (1994) Adv. Biophys. Chem. 4, 179-236
30.	van Halbeek, H. (1996) in Encyclopedia of NMR (Grant, D. M. , and Harris, R. K., eds), Vol. 2 , pp. 1107-1137, Wiley, Chichester
31.	Takayama, K., Qureshi, N., and Mascagni, P. (1983) J. Biol. Chem. 258, 12801-12803
32.	Strain, S. M., Armitage, I. M., Anderson, L., Takayama, K., Qureshi, N., and Raetz, C. R. H. (1985) J. Biol. Chem. 260, 16089-16098
33.	Zähringer, U., Lindner, B., and Rietschel, E. T. (1999) in Endotoxin in Health and Disease (Brade, H. , Opal, S. M. , Vogel, S. N. , and Morrison, D. C., eds) , pp. 93-114, Marcel Dekker, Inc., New York
34.	Masoud, H., Perry, M. B., and Richards, J. C. (1994) Eur. J. Biochem. 220, 209-216
35.	Karunaratne, D. N., Richards, J. C., and Hancock, R. E. (1992) Arch. Biochem. Biophys. 299, 368-376
36.	Price, N. J. P., Jeyaretnam, B., Carlson, R. W., Kadrmas, J. L., Raetz, C. R. H., and Brozek, K. A. (1995) Proc. Natl. Acad. Sci. U. S. A. 92, 7352-7356
37.	Brozek, K. A., Kadrmas, J. L., and Raetz, C. R. H. (1996) J. Biol. Chem. 271, 32112-32118
38.	Brozek, K. A., Carlson, R. W., and Raetz, C. R. H. (1996) J. Biol. Chem. 271, 32126-32136
39.	Raetz, C. R. H. (1996) in Escherichia coli and Salmonella: Cellular and Molecular Biology (Neidhardt, F. C., ed), 2nd Ed., Vol. 1 , pp. 1035-1063, American Society for Microbiology, Washington, D.C.
40.	Rietschel, E. T., Kirikae, T., Schade, F. U., Mamat, U., Schmidt, G., Loppnow, H., Ulmer, A. J., Zähringer, U., Seydel, U., Di Padova, F., Schreier, M., and Brade, H. (1994) FASEB J. 8, 217-225
41.	Medzhitov, R., and Janeway, C. A., Jr. (1998) Curr. Opin. Immunol. 10, 12-15
42.	Borregaard, N., Elsbach, P., Ganz, T., Garred, P., and Svejgaard, A. (2000) Immunol. Today 21, 68-70
43.	Graham, T. L., Sequeira, L., and Huang, T. S. (1977) Appl. Environ. Microbiol. 34, 424-432
44.	Price, N. P. J., Kelly, T. M., Raetz, C. R. H., and Carlson, R. W. (1994)

Two-dimensional NMR Spectroscopy and Structures of Six Lipid A Species from Rhizobium etli CE3 DETECTION OF AN ACYLOXYACYL RESIDUE IN EACH COMPONENT AND ORIGIN OF THE AMINOGLUCONATE MOIETY*,

Two-dimensional NMR Spectroscopy and Structures of Six Lipid A Species from Rhizobium etli CE3

DETECTION OF AN ACYLOXYACYL RESIDUE IN EACH COMPONENT AND ORIGIN OF THE AMINOGLUCONATE MOIETY^*^,