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J. Biol. Chem., Vol. 279, Issue 24, 25411-25419, June 11, 2004

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Enzymatic Synthesis of Lipid A Molecules with Four Amide-linked Acyl Chains

LpxA ACYLTRANSFERASES SELECTIVE FOR AN ANALOG OF UDP-N-ACETYLGLUCOSAMINE IN WHICH AN AMINE REPLACES THE 3''-HYDROXYL GROUP^*

Charles R. Sweet¶, Allison H. Williams||, Mark J. Karbarz, Catherine Werts**, Suzanne R. Kalb, Robert J. Cotter, and Christian R. H. Raetz

From the Department of Biochemistry, Duke University Medical Center, Durham, North Carolina 27710, the ^**Unité de Bactériologie Moléculaire et Médicale, Institut Pasteur, Paris, 75015, France, and the Middle Atlantic Mass Spectrometry Laboratory, Department of Pharmacology and Molecular Sciences, The Johns Hopkins University School of Medicine, Baltimore, Maryland 21205

Received for publication, January 20, 2004 , and in revised form, March 1, 2004.

	ABSTRACT

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
LpxA of Escherichia coli catalyzes the acylation of the glucosamine 3-OH group of UDP-GlcNAc, using R-3-hydroxymyristoyl-acyl carrier protein (ACP) as the donor substrate. We now demonstrate that LpxA in cell extracts of Mesorhizobium loti and Leptospira interrogans, which synthesize lipid A molecules containing 2,3-diamino-2,3-dideoxy-D-glucopyranose (GlcN3N) units in place of glucosamine, do not acylate UDP-GlcNAc. Instead, these LpxA acyltransferases require a UDP-Glc-NAc derivative (designated UDP 2-acetamido-3-amino-2,3-dideoxy--D-glucopyranose or UDP-GlcNAc3N), characterized in the preceding paper (Sweet, C. R., Ribeiro, A. A., and Raetz, C. R. H. (2004) J. Biol. Chem. 279, 25400–25410), in which an amine replaces the glucosamine 3-OH group. L. interrogans LpxA furthermore displays absolute selectivity for 3-hydroxylauroyl-ACP as the donor, whereas M. loti LpxA functions almost equally well with 10-, 12-, and 14-carbon 3-hydroxyacyl-ACPs. The substrate selectivity of L. interrogans LpxA is consistent with the structure of L. interrogans lipid A. The mechanism of L. interrogans LpxA appears to be similar to that of E. coli LpxA, given that the essential His¹²⁵ residue of E. coli LpxA is conserved and is also required for acyltransferase activity in L. interrogans. Acidithiobacillus ferrooxidans (an organism that makes lipid A molecules containing both GlcN and GlcN3N) has an ortholog of LpxA that is selective for UDP-GlcNAc3N, but the enzyme also catalyzes the acylation of UDP-GlcNAc at a slow rate. E. coli LpxA acylates UDP-GlcNAc and UDP-GlcNAc3N at comparable rates in vitro. However, UDP-GlcNAc3N is not synthesized in vivo, because E. coli lacks gnnA and gnnB. When the latter are supplied together with A. ferrooxidans lpxA, E. coli incorporates a significant amount of GlcN3N into its lipid A.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Many Gram-negative bacteria contain a 2,3-diamino-2,3-dideoxy-D-glucopyranose (GlcN3N)¹ unit in place of one or both glucosamine residues in their lipid A molecules (Fig. 1) (1–3). As explained in the preceding manuscript (4), these lipid A variants may be generated from the sugar nucleotide UDP-2-acetamido-3-amino-2,3-dideoxy--D-glucopyranose (UDP-GlcNAc3N). The enzymes GnnA and GnnB are responsible for the biosynthesis of UDP-GlcNAc3N from UDP-GlcNAc in Acidithiobacillus ferrooxidans (4). GnnA catalyzes the oxidation and GnnB catalyzes the subsequent transamination of the glucosamine 3-OH group of UDP-GlcNAc to generate UDP-GlcNAc3N (4).

View larger version (19K): [in this window] [in a new window]   FIG. 1. Structure of the lipid A backbone in E. coli versus A. ferrooxidans, L. interrogans, or M. loti. A, this is the predominant E. coli lipid A molecule found in cells grown at pH 7.4 (3). The cyan O atom at positions 3 and 3' are characteristic of a GlcN disaccharide. B, the A. ferrooxidans lipid A backbone contains both GlcN and GlcN3N (3 and/or 3'-nitrogen atoms of GlcN3N in red and corresponding oxygen atoms of GlcN in cyan). This lipid A is likely a mixture of four species. Limited structural data suggest that it contains five acyl chains (5). The 1- and 4'-positions (X and Y, respectively) lack phosphate moieties (5). C, L. interrogans and M. loti lipid A contain GlcN3N exclusively (3- and 3'-nitrogen atoms in red). The structure of M. loti lipid A is not fully characterized (6). That of L. interrogans is presented in the following paper (7). In lipopolysaccharide, 3-deoxy-D-manno-octulosonic acid would be attached at position 6'.

	EXPERIMENTAL PROCEDURES

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Materials—All growth media, materials, and fine chemicals were the same as in the preceding manuscript (4) or were purchased from Sigma-Aldrich. PerkinElmer Life Sciences was the source of [-³²P]UTP. The LpxC inhibitor L-573,655 was kindly provided by Dr. A. Patchett (Merck Research Laboratories) (14).

Bacterial Strains and Plasmids—A. ferrooxidans ATCC 23270 and M. loti ATCC 700743 were purchased from the American Type Culture Collection. A. ferrooxidans cells were grown on modified 9K medium (15). M. loti cells were grown on yeast mannitol agar or liquid medium (6). E. coli XL1-Blue (Stratagene) was used for cloning and maintenance of plasmids. E. coli BL21(DE3)/pLysS (Stratagene) was used for overexpression of cloned genes, typically using the Novagen plasmids pET23c+ and pET30a+. The E. coli temperature-sensitive mutant RO138 (lpxA2 recA rpsL Tet^r), a recA derivative of SM101 (12), was provided by Dr. M. Anderson (Merck Research Laboratories). The vector pBluescript II SK(+) (Stratagene) was used to express foreign genes in R0138, as described below. Plasmid constructs are summarized in Table I.

Recombinant DNA Techniques—Transformation of competent cells, nucleic acid purification, and electrophoresis were carried out according to established procedures (19, 20). The plasmids were purified using the Qiaprep miniprep spin column kit (Qiagen). Digested PCR products and plasmid DNA were purified by phenol/chloroform/isoamyl alcohol extraction and ethanol precipitation (19, 20) or by agarose gel electrophoresis in conjunction with the Qiagen Qiaquick gel extraction kit (4).

Isolation and Cloning of the lpxA Gene from A. ferrooxidans— Genomic DNA was prepared from A. ferrooxidans as described (4). The lpxA gene was PCR-amplified with the Pfu polymerase using the oligonucleotide primers 5'-GGA ATT CCA TAT GAC GGT GCA GAT TCA TCC GCT GG-3' (N-terminal primer) and 5'-CGG GAT CCC CCC GAT GAC CCC GGT TCT CAT ATG G-3' (C-terminal primer). The NdeI and BamHI sites, respectively, are underlined. The PCR product of AflpxA DNA was purified and digested with NdeI and BamHI in preparation for ligation into similarly treated pET23c+ vector. The desired derivative of pET23c+ bearing AflpxA was designated pCS311. The AfLpxA amino acid sequence is MTVQIHPLAI VDSSVQIGEG CTIGPFAVIG AGVEIGDHCR IGANTVIEGP CRLGAHNQIF QFASVGTAPQ DLGYAGEPTT LEIGSHNTIR EFVTINRGTV KGGGTTRIGH HNLLMAYCHV AHDCSIGDQV VMANAATLAG HVSVEDHAIL GGLSAVHQYA RVGAHAILGG GTMAPLDIPP FMMAAGNHAS LHGINVRGLA RRGIPRETIL QIKRAYRLLF RSGLRLEDAM DEVSQRGLNA PEVAYLLDFI RNSRRGITRP.

Generation of Plasmid Constructs Containing lpxA, gnnA, and gnnB from A. ferrooxidans—The AflpxA gene was subcloned from pCS311 along with the pET23c+ ribosome-binding site into pBluescript II SK(+) using XbaI and HindIII to generate pCS421 and then from this construct into pNGH100 (17) using SacI and BamHI to generate pCS449. The gnnA and gnnB genes were likewise cloned into pBluescript II SK(+) by insertion of the XbaI/HindIII fragment of the bicistronic construct pCS355 (4) into similarly treated pBluescript vector. The desired hybrid plasmid expressing the two genes was designated pCS411. In addition, a pBluescript II SK(+)-based construct was constructed bearing the A. ferrooxidans gnnA, gnnB, and lpxA genes. For this purpose, a PCR fragment bearing AflpxA was first generated using pCS311 as the template, and primers were designed to create a PCR product bearing the entire lpxA gene preceded by the pET23c+ ribosome-binding site. The N-terminal primer was 5'-CCC AAA AAG CTT GGG AGA CCA CAA CGG TTT CCC-3'. The C-terminal primer was 5'-CCC GCC TCG AGG TCG ACG GAG CTC GAA TTC GGA TCC-3'. This fragment was then cloned into pCS411 using HindIII and XhoI digestion, which inserts the lpxA fragment behind the gnnA and gnnB genes. As noted above, these genes are themselves behind a ribosome-binding site from pET23c+ (subcloned from pCS355). The hybrid plasmid derived from this ligation was designated pCS439.

Cloning of lpxA from L. interrogans Serovar Icterohemeorrhagiae (Strain Verdun)—The whole genome sequence of the L. interrogans serovar Lai (21) revealed one gene (LilpxA) of 780 bp that displayed 41% identity and 59% similarity at the protein level with E. coli LpxA (9). The LilpxA gene of L. interrogans serovar Icterohemeorrhagiae (strain Verdun, virulent isolate) (22) was PCR-amplified with the Pfu polymerase using the oligonucleotide primers 5'-GGA ATT CCA TAT GAA AAT ACA TCC GAC TGC TAT TA-3' (N-terminal primer) and 5'-GCG GAT CCT CAC CTG TGA TTT GTA ACT CCCC-3' (C-terminal primer). The NdeI and BamHI sites, respectively, are underlined. The amplified gene was digested with NdeI and BamHI and then ligated with T4 DNA ligase into similarly digested pET30a+. The ligation mixture was transformed by electroporation into supercompetent XL1-Blue (Stratagene). Plasmid-containing transformants were selected at 37 °ConLB agar plates supplemented with kanamycin (30 µg/ml). Putative clones were repurified on LB kanamycin plates. Plasmid DNA was then isolated and screened for the presence of the desired insert by BamHI and NdeI digestion. One positive clone containing the LilpxA gene was designated pLP3 and confirmed by DNA sequencing. Only two silent changes, specific for the Verdun strain, were detected in comparison with the nucleotide sequence of lpxA from the Lai strain.

For preparation of cell extracts and assays, the LilpxA gene of pLP3 was overexpressed in E. coli BL21(DE3)/pLysS (Stratagene). The LilpxA gene was also subcloned from pLP3 into pBluescript II SK(+) using XbaI and XhoI to generate pCS611, as described for pCS421. The LilpxA gene was subcloned into the low copy vector pNGH100 to make pCS623, using SacI and BamHI as described for pCS449.

Preparation of Cell-free Extracts—To prepare E. coli extracts for assays, the constructs were grown at 30 °C in 50 ml of LB broth with 100 µg/ml ampicillin to A₆₀₀ = 0.5, shifted to 18 °C for 10 min, induced with 1 mM isopropyl-1-thio--D-galactopyranoside, and then grown overnight. The extracts were prepared by passage through a French pressure cell, as described (4). The protein concentrations were quantified using the Pierce bicinchoninic acid assay kit (23) with bovine serum albumin as the standard.

Cell-free extracts and membranes of L. interrogans strain Verdun (avirulent derivative) were prepared from a 4.3-g frozen cell pellet derived from a 10-liter culture (2 x 10⁹ bacteria/ml) grown at the Institut Pasteur (Paris, France) (22). All of the steps were conducted at 0–4 °C. The pellet was resuspended in 20 ml of 50 mM HEPES, pH 7.5, containing 10% glycerol. A 5-ml portion of the cell suspension was diluted to 10 ml with the same buffer, and the remaining 15 ml was stored at -80 °C for later use. The cells were broken by three passages through a French pressure cell at 10,000 p.s.i. The lysate was centrifuged at 12,600 x g for 10 min to remove unbroken cells and large debris. The protein concentration of this extract was 6.9 mg/ml (23). A 7-ml portion of the extract was centrifuged at 100,000 x g for 1 h. The soluble fraction was stored at -80 °C, and the membranes were homogenized in 1 ml of 50 mM HEPES, pH 7.5, to yield a final protein concentration of about 12 mg/ml. The membrane suspension was then divided into aliquots and stored at -80 °C.

Substrate Preparation—The [-³²P]UDP-GlcNAc and all of the acyl-ACP substrates were prepared as previously described (24). To make [-³²P]UDP-GlcNAc3N from [-³²P]UDP-GlcNAc, 250 µCi of [-³²P] UDP-GlcNAc was dissolved in 138 µl of deionized water. This radiolabeled substrate (final concentration, 1.5 µM) was incubated with an additional 48.5 µM UDP-GlcNAc carrier, 50 µM HEPES, pH 8.0, 100 mM L-glutamic acid, 1 mM NAD⁺, and 0.5 mg/ml pCS355 cell-free extract (4) in a reaction volume of 200 µl for 2.5 h at 30 °C. About 50% of the [-³²P]UDP-GlcNAc is converted to [-³²P]UDP-GlcNAc3N under these conditions. This reaction was then chilled on ice and diluted 3-fold with cold 100% ethanol. After 10 min, the debris was removed by centrifugation. The supernatant was diluted 4-fold with cold water.

To separate the [-³²P]UDP-GlcNAc and [-³²P]UDP-GlcNAc3N, anion exchange chromatography was performed using a 2-ml DEAE-cellulose column (Whatman DE52) equilibrated with 10 mM BisTris, pH 6.0. The diluted reaction mixture was loaded onto the column, which was washed with 8 ml of deionized water and then with 8 ml of 10 mM BisTris, pH 6.0. The column was eluted with increasing concentrations of BisTris, pH 6.0, according to the following scheme: 8 ml at 20 mM, 8 ml at 30 mM, 8 ml at 40 mM, 4 ml at 50 mM, and 12 ml at 80 mM. The fractions (2 ml) were analyzed by TLC on PEI-cellulose plates, developed with 0.2 M aqueous guanidine HCl. Most of the [-³²P]UDP-GlcNAc3N elutes with the 20 and 30 mM BisTris. The relevant fractions were pooled, diluted 4-fold with water, and loaded onto a second DEAE column to remove NAD⁺ (4).

In Vitro lpxA Assay Conditions—The LpxA-catalyzed conversion of [-³²P]UDP-GlcNAc or [-³²P]UDP-GlcNAc3N to [-³²P]UDP-(3-O-acyl)-GlcNAc and [-³²P]UDP-(3-N-acyl)-GlcNAc3N, respectively, is monitored by TLC on a silica plate because the acylated product migrates more rapidly than the substrate (8, 24, 25). Each 10-µl reaction tube contained 40 mM HEPES, pH 8.0, 1 mg/ml bovine serum albumin, 0.2 mg/ml LpxC inhibitor L-573–655 (14), and 10 µM acyl donor (as indicated). Either 10 µM [-³²P]UDP-GlcNAc or 10 µM [-³²P]UDP-GlcNAc3N was used as the acyl acceptor at 2 x 10⁵ dpm/tube. The reaction was started at 30 °C by the addition of an appropriate amount of cell-free extract. Conversion to product was analyzed by spotting 1 µl of each reaction mixture on a silica TLC plate. The plate was developed with chloroform/methanol/water/acetic acid (25:15:4:2, v/v) and analyzed with a PhosphorImager.

Site-directed Mutagenesis of LilpxA—Using pLP3 as the template, the QuikChange site-directed mutagenesis kit (Stratagene) was used to generate the H120A substitution, which corresponds to the H125A mutation in E. coli (11). The structure of the mutated plasmid, designated pLP3-1, was confirmed by DNA sequencing. The pLP3-1 plasmid was then transformed into competent cells of BL21(DE3)/pLysS.

Structural Analysis of Lipid A Species Isolated from Various E. coli Constructs—Lipid A was isolated from the E. coli lpxA2 mutant RO138 complemented with different sets of genes. The first construct expressed gnnA, gnnB, and AflpxA off of a single hybrid plasmid (RO138/pCS439) (4), whereas the second construct expressed gnnA, gnnB, and LilpxA on separate hybrid plasmids (RO138/pCS411/pCS623) (Table I).

For preparation of the lipid A, RO138/pCS439 was grown without shaking in 1 liter of LB medium for 48 h at 42 °C in the presence of 50 µg/ml ampicillin and 12 µg/ml tetracycline. A 100-ml culture of RO138/pCS411/pCS623 was grown with shaking at 250 rpm in LB medium at 30 °C. The latter construct was not viable at 42 °C. A 100-ml culture of RO138/pCS61 also was grown at 42 °C in LB medium with shaking, given that it grows normally and produces normal amounts of wild-type lipid A.

Extraction, hydrolysis at pH 4.5, and purification of lipid A 1,4'-bisphosphate species by DEAE-cellulose chromatography was carried out as previously described (17, 26). Prior to mass spectrometry, the purified lipid A was subjected to base hydrolysis by incubation in freshly made chloroform, methanol, 1.7 M NaOH (2:1:0.4, v/v/v) at room temperature (25 °C) for 2 h, with occasional mixing of the two phases (27). Following hydrolysis, the organic phase was dried under N₂, and the lipid was redissolved in chloroform, methanol (4:1, v/v). A portion was spotted onto a silica gel 60 TLC plate, developed in chloroform, pyridine, formic acid, water (50:50:16:5, v/v/v/v). After spraying with 10% sulfuric acid in ethanol, the lipids were visualized by charring.

Mass Spectrometry of Base-treated Lipid A Samples—MALDI-TOF mass spectra were acquired in the negative-ion linear modes using a Kratos Analytical (Manchester, UK) MALDI-TOF mass spectrometer, operated with a 337-nm nitrogen laser, a 20-kV extraction voltage, and time-delayed extraction (24).

	RESULTS

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Selectivity of LpxA Acyltransferases in Extracts of M. loti and L. interrogans—Of the three organisms used for studying the origin of GlcN3N-containing lipid A molecules, M. loti is easiest to grow (6). As shown in Fig. 2A and Table II, 10 µM [-³²P]UDP-GlcNAc is inactive as an acceptor substrate in extracts of M. loti when tested with either 10-, 12-, 14-, or 16-carbon 3-hydroxyacyl-ACP donors (each added at 10 µM). In contrast, [-³²P]UDP-GlcNAc3N is efficiently acylated in the presence of 10-, 12-, or 14-carbon 3-hydroxyacyl-ACPs under matched conditions (Fig. 2B and Table II). The specific activity of M. loti LpxA was the highest with 3-hydroxymyristoyl-ACP (Table II), consistent with the reported fatty acid composition of M. loti lipid A (6). Prolonged incubation (Fig. 2B, lanes 10 and 14) resulted in nearly quantitative conversion of [-³²P]UDP-GlcNAc3N to acylated product, indicating that N-acylation by M. loti LpxA is thermodynamically favorable. This contrasts with the 3-O-acylation of [-³²P]UDP-GlcNAc by E. coli LpxA, which is thermodynamically unfavorable (11, 28).

View larger version (73K): [in this window] [in a new window]   FIG. 2. Acylation of [-32P]UDP-GlcNAc3N but not [-32P]UDP-GlcNAc in extracts of M. loti. Cell-free extracts were assayed at 0.05 mg/ml protein with 10 µM each of donor and acceptor substrates, as indicated. The four time points for each indicated hydroxyacyl-ACP (lanes 3–6, 7–10, 11–14, and 15–18) were 5, 10, 20, and 30 min. Lanes 1 and 2 are no enzyme controls at 0 and 30 min. A, [-32P]UDP-GlcNAc as acceptor substrate. B, [-32P]UDP-GlcNAc3N as acceptor substrate. The arrows indicate RF values of monoacylated products formed with the indicated acyl-ACP donors.

View this table: [in this window] [in a new window]   TABLE II Sugar nucleotide and acyl-ACP selectivity of LpxA acyltransferases in extracts of E. coli, M. loti, and L. interrogans Cell-free extracts were assayed in the linear range with 0.05–0.5 mg/ml protein, as appropriate. Conversion of [ - 32P]UDP-GlcNAc or [-32P]UDP-GlcNAc3N to the corresponding acylated derivative was monitored by TLC, followed by analysis with a PhosphorImager. The standard deviation of the specific activities was approximately ± 20% for triplicate or quadruplicate determinations.

The quantification of LpxA specific activities observed in various cell extracts with different combinations of substrates is summarized in Table II. Unexpectedly, E. coli LpxA was found to acylate UDP-GlcNAc3N at a slightly faster rate than its natural substrate UDP-GlcNAc (10 µM acceptor and donor substrates).

Mild Alkaline Hydrolysis of Acylated [-³²P]UDP-GlcNAc3N— To confirm that LpxA acylates [-³²P]UDP-GlcNAc3N on the nitrogen atom at the pyranose 3-position, a portion of the LpxA product generated with either E. coli or L. interrogans LpxA was subjected to mild alkaline hydrolysis (27). In contrast to [-³²P]UDP-3-O-acyl-GlcNAc synthesized by E. coli LpxA, which is deacylated by a 30-min exposure to dilute NaOH at room temperature (27), the acylated [-³²P]UDP-GlcNAc3N generated either by E. coli or L. interrogans LpxA was unaffected. These observations, together with the thermodynamically favorable acylation seen with UDP-GlcNAc3N versus UDP-GlcNAc, are consistent with the formation of an amidelinked acyl chain at the 3-position of the pryanose ring of UDP-GlcNAc3N (Scheme 1 in Ref. 4).

Cloning of LpxA Orthologs from L. interrogans and A. ferrooxidans—The lpxA genes of L. interrogans (21) and A. ferrooxidans were identified by probing their genomes (www.ncbi.nlm.nih.gov/BLAST/) with the E. coli LpxA sequence (9). One 780-bp gene, designated LilpxA, encodes a predicted protein of 259 amino acids that displays 41% amino acid identity and 59% similarity with E. coli LpxA (21), with an E value of about 4 x 10^-51 in a pair-wise comparison (29). The nearly identical lpxA gene from L. interrogans strain Verdun (22) was cloned by PCR from its genomic DNA, inserted into pET30a+, and expressed in E. coli BL21(DE3)/pLysS. The lpxA gene of A. ferrooxidans encodes a protein of 260 amino acid residues with 49% amino acid identity, 69% similarity with an E value 3 x 10^-71 when compared with E. coli LpxA (29). This gene was first cloned into pET23c+ and also into pBluescript II SK(+), pNGH100, or pCS411, depending on the experiment (see below). A ClustalW alignment of EcLpxA, AfLpxA, and LiLpxA is shown in Fig. 3.

View larger version (53K): [in this window] [in a new window]   FIG. 3. Sequence comparison of AfLpxA, EcLpxA, and LiLpxA. This ClustalW alignment (www.embl-heidelberg.de/) shows the predicted protein sequences and conserved residues of AfLpxA, LiLpxA, and EcLpxA. The relatively conserved E. coli lysine 76 and the absolutely conserved E. coli histidine 125 residues are highlighted with arrows (11). In many but not all bacteria that make lipid A containing GlcN3N, the lysine 76 equivalent is substituted with glycine. Lysine 76 is in the vicinity of the E. coli LpxA active site and may contribute to substrate binding (11). However, the G71K substitution in LiLpxA had no effect on sugar nucleotide selectivity (not shown).

Site-directed Mutagenesis of L. interrogans LpxA—Previous studies demonstrated that His¹²⁵ of E. coli is required for catalysis (11), perhaps as a general base to activate the glucosamine 3-OH group of UDP-GlcNAc during acyl chain transfer (Fig. 4). His¹²⁵ is conserved and corresponds to His¹²⁰ in L. interrogans (Fig. 3, lower arrow). Substitution of His¹²⁰ with alanine inactivates the L. interrogans LpxA (Fig. 5), suggesting a similar function as in E. coli, despite the differences in acceptor and donor selectivity.

View larger version (13K): [in this window] [in a new window]   FIG. 4. Possible role of His125 in the catalytic mechanism of E. coli LpxA. In our previously published model (11), N1 of histidine 125 (in the alternative tautomeric representation from the one shown above) was proposed to function as the general base. However, the His125 side chain of LpxA was flipped in the published x-ray structure (9) (S. Roderick, personal communication). With the revised conformation, N2 of His125 is proposed to activate the glucosamine 3-OH group in the acceptor substrate, and the conserved Asp126 side chain would then be in a good position to orient and/or stabilize the His125 residue by hydrogen bonding the N1 proton.

View larger version (15K): [in this window] [in a new window]   FIG. 5. The H120A substitution inactivates L. interrogans LpxA. His120 of L. interrogans LpxA is the equivalent of His125 in E. coli (see Fig. 3) (11).

Biosynthesis of GlcN3N-containing Lipid A Molecules in RO138 Complemented with gnnA, gnnB, and AflpxA—Lipid A samples from RO138/pCS61 (EclpxA) and RO138/pCS439 (gnnA gnnB AflpxA) grown without shaking at 42 °C were isolated and purified by ion exchange chromatography on DEAE cellulose. Each lipid A preparation was subjected to mild alkaline hydrolysis to remove all of the ester-linked acyl chains. TLC analysis of the hydrolyzed samples suggested that a portion (30%) of the RO138/pCS439 (gnnA gnnB AflpxA) lipid A contained three base-resistant acyl chains (Fig. 6A, Band I) under conditions that degrade all of the RO138/pCS61 (EclpxA) lipid A to a single, diacylated derivative (Fig. 6B, Band II).

View larger version (79K): [in this window] [in a new window]   FIG. 6. Mild alkaline hydrolysis of lipid A from RO138/pCS61 (EclpxA) (A) and RO138/pCS439 (gnnA gnnB AflpxA) (B). The plate was developed in chloroform/pyridine/formic acid/water (50:50: 16:5, v/v/v/v). The lipids were visualized by spraying with 10% sulfuric acid in ethanol, followed by charring on a hot plate. Nonhydrolyzed lipid A controls are shown for RO138/pCS439 (lane 2) and RO138/pCS61 (lane 4). Corresponding base-treated samples are shown in lanes 1 and 3, respectively.

View larger version (24K): [in this window] [in a new window]   FIG. 7. Negative ion mode MALDI-TOF mass spectrometry of base-hydrolyzed lipid A from RO138/pCS61 and RO138/pCS439. A 10-fold excess of RO138/pCS61 (EclpxA) lipid A (A) was hydrolyzed, when compared with RO138/pCS439 (gnnA gnnB AflpxA) lipid A (B), to ensure that complete hydrolysis of all ester-linked acyl chains was taking place under all experimental conditions. The proposed structures of the mild alkaline hydrolysis products are indicated.

	DISCUSSION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
LpxA is an essential cytoplasmic enzyme in E. coli that catalyzes the first step of lipid A biosynthesis according to the reaction: UDP-GlcNAc + R-3-hydroxymyristoyl-ACP UDP-3-O-(R-3-hydroxymyristoyl)-GlcNAc + ACP (3, 8, 11, 30). The crystal structure of E. coli LpxA at 2.6-Å resolution suggests that the enzyme is homotrimer in which the active sites are situated between adjacent subunits (9–11). Each LpxA monomer is constructed around an unusual left-handed parallel -helix, which is conserved in all LpxA orthologs and in many other bacterial acetyl- and acyltransferases (9, 31–33). The crystal structure of E. coli LpxA has not been determined in the presence of bound substrates or substrate analogs, but site-directed mutagenesis has demonstrated that histidine 125 is crucial for activity and that adjacent basic residues may contribute to substrate binding (Fig. 4) (11). The recent structure of Helicobacter pylori LpxA with a detergent molecule bound at the proposed active site supports the above conclusions (34).

The acyl-ACP donor selectivity of LpxA has previously been studied in several systems (8, 17, 24, 35–37). In general, LpxA orthologs show strong preferences for acyl chain length and the presence of the R-3-hydroxyl group (8, 17, 24, 35–37). The corresponding coenzyme A thioesters are not substrates (8, 25). E. coli LpxA is highly selective for R-3-hydroxymyristoyl-ACP (8, 25), whereas the Pseudomonas aeruginosa enzyme strongly prefers R-3-hydroxydecanoyl-ACP (35, 36). The G173M substitution converts the E. coli enzyme from a 14- to a 10-carbon-specific acyltransferase, whereas the converse M169G substitution in P. aeruginosa LpxA does the opposite (10). These findings show that precise hydrocarbon rulers are present in the active sites of these LpxA orthologs (Fig. 4). Cocrystals of LpxA variants with various acyl-ACPs will be required to gain further insights.

Although E. coli and related LpxA proteins have been characterized as UDP-N-acetylglucosamine 3-O-acyltransferases (8, 28, 35), their sugar nucleotide specificity has not been examined in depth (8). As proposed in Scheme 1 of the preceding manuscript (4), lipid A biosynthesis in bacteria that make GlcN3N-substituted lipid A molecules might start with the conversion of UDP-GlcNAc to the analog UDP-GlcNAc3N, followed by selective N-acylation catalyzed by special LpxA orthologs present in those organisms. The results shown in Fig. 2 and Tables II and III demonstrate that LpxA orthologs from M. loti, L. interrogans, and A. ferrooxidans do indeed utilize UDP-GlcNAc3N in strong or absolute preference to UDP-GlcNAc.

L. interrogans and M. loti make lipid A molecules based exclusively on a -1',6-linked GlcN3N disaccharide (6, 7), whereas A. ferrooxidans lipid A contains both GlcN3N and GlcN units (5). The LpxA with the most stringent substrate specificity is that of L. interrogans (Tables II and III). In agreement with the absence of glucosamine in the lipid A backbone of this organism (7), LiLpxA does not utilize UDP-GlcNAc at a measurable rate with any acyl donor substrate (limit of detection <2 pmol/min/mg of extract). Furthermore, LiLpxA does not acylate UDP-GlcNAc3N with any donor other than 3-hydroxylauroyl-ACP. Although most other LpxA proteins display a high degree of specificity for a particular acyl chain length, they do in fact function with alternative acyl donors at slow rates (Tables II and III) (8, 17, 24, 35, 37).

A. ferrooxidans LpxA displays some activity with all of the 3-hydroxyacyl-ACP donors tested and with both sugar nucleotides (Table III). M. loti cell extracts (Fig. 2) and the Bordetella pertussis and B. bronchiseptica LpxA orthologs (24) are likewise very relaxed with regard to acyl chain length selectivity. In the bordetellae, structural studies indicate that the acyl chains at the 3- and 3'-positions of lipid A can be different under different conditions, explaining the need for a relaxed LpxA ortholog (38–40). Structural characterization of A. ferrooxidans lipid A shows no such heterogeneity (5); however, this work was done with A. ferrooxidans IFO 14262 and may not reflect the exact lipid A structure of A. ferrooxidans ATCC 23270 from which our AflpxA gene was cloned. In RO138/pCS439, grown at 42 °C (Fig. 7B), mainly 3-hydroxymyristate was incorporated into the lipid A 3- and 3'-positions by AfLpxA. AfLpxA may be more selective in vivo, or more R-3-hydroxymyristoyl-ACP may be available inside the cells.

The composition of the lipid A synthesized by AfLpxA in living cells may be affected by the relative sizes of the UDP-GlcNAc and the UDP-GlcNAc3N pools. Despite reports of a mixed lipid A backbone in A. ferrooxidans (5) and our demonstration of a mixed lipid A composition in RO138/pCS439 (Figs. 6A and 7B), AfLpxA is 100-fold selective for UDP-GlcNAc3N over UDP-GlcNAc when assayed in vitro at 10 µM of each donor and acceptor substrate (Table III). Consequently, one could argue that a 100:1 concentration ratio of UDP-GlcNAc to UDP-GlcNAc3N might be needed in vivo to yield a mixed lipid A backbone containing equal amounts of GlcN3N and GlcN, as suggested in the literature (5). Because GlcN3N is roughly one-sixth of the total lipid A sugar in RO138/pCS439 (Fig. 7B), the in vivo ratio of UDP-GlcNAc to UDP-GlcNAc3N present in this E. coli construct might be 300:1.

The specific activity of AfLxpA-expressing E. coli extracts (36 pmol/min/mg) was significantly lower than that of the empty vector control (51 pmol/min/mg), when assayed with UDP-GlcNAc and 3-hydroxymyristoyl-ACP (Table III). Apparent suppression of the background chromosomal activity by heterologous overexpression of foreign LpxA orthologs has been noted previously (10, 17). This phenomenon may be due to the formation of inactive heterotrimers between EcLpxA and the foreign LpxA proteins. Because there was no measurable chromosomal activity with any acyl donor other than 3-hydroxymyristoyl-ACP in the vector control extracts under these assay conditions (Table III), the low but significant activity seen with UDP-GlcNAc when AfLpxA-expressing extracts were assayed with C-12 and C-16 hydroxyacyl-ACPs (Table III) likely represents true AfLpxA catalytic function.

E. coli LpxA has robust activity with UDP-GlcNAc3N and can tolerate the presence of some GlcN3N in its lipid A, as in RO138/pCS439 grown on plates or in nonshaking liquid culture medium at 42 °C (Fig. 7B). However, the complementation of the lpxA2 phenotype was not complete. Very small colonies formed on plates, and the maximal A₆₀₀ reached in nonshaken liquid medium was only 0.2. It may be that lipid A substituted with GlcN3N is toxic to E. coli. Whatever the explanation for the slow growth of RO138/pCS439 at 42 °C, it might yet be possible to substitute E. coli lipid A completely with GlcN3N, either by using alternative GnnA, GnnB, and/or LpxA orthologs or by introducing second site suppressor mutations into constructs like RO138/pCS439. Engineered strains containing GlcN3N-based lipid A molecules might be useful for the preparation of new endotoxin antagonists (41, 42) or novel vaccines.

	FOOTNOTES

 
The nucleotide sequence(s) reported in this paper has been submitted to the DDBJ/GenBank^TM/EBI Data Bank with accession number(s) AY541060 [GenBank] .

^* This work was supported by National Institutes of Health Grants GM-51310 and GM-51796 (to C. R. H. R.), and GM-54882 (to R. J. C.) and by Grant PTR94 form the Institut Pasteur (to C. W.). The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Supported by National Institutes of Health Training Grant GM-08558 in Biological Chemistry to Duke University.

^¶ Present address: Div. of Infectious Diseases, University of Massachusetts Medical Center, Worcester, MA 01655.

^|| Supported by National Institutes of Health Training Grant GM-07184 in Cellular and Molecular Biology to Duke University.

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

¹ The abbreviations used are: GlcN3N, 2,3-diamino-2,3-dideoxy-D-glucopyranose; BisTris, 2,2-bis(hydroxymethyl)-2,2',2''-nitrilotriethanol; ACP, acyl carrier protein; UDP-GlcNAc3N, UDP-2-acetamido-3-amino-2,3-dideoxy--D-glucopyranose; MALDI-TOF, matrix-assisted laser desorption ionization time-of-flight.

	ACKNOWLEDGMENTS

 
We thank Dr. Nanette Que for preparing the cell-free extracts of L. interrogans serovar Icterohemeorrhagiae (strain Verdun).

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