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J Bacteriol, July 1998, p. 3570-3577, Vol. 180, No. 14
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Department of Animal Sciences, University of Kentucky, Lexington, Kentucky 40546-0215
Received 3 February 1998/Accepted 15 May 1998
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ABSTRACT |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Immediately downstream from the Thermoanaerobacter ethanolicus xylAB operon, comprising genes that encode D-xylose isomerase and D-xylulose kinase, lies a 1,101-bp open reading frame that exhibits 61% amino acid sequence identity to the Escherichia coli D-xylose binding periplasmic receptor, XylF, a component of the high-affinity binding-protein-dependent D-xylose transport. The 25-residue N-terminal fragment of the deduced T. ethanolicus XylF has typical features of bacterial leader peptides. The C-terminal portion of this leader sequence matches the cleavage consensus for lipoproteins and is followed by a 22-residue putative linker sequence rich in serine, threonine, and asparagine. The putative mature 341-amino-acid-residue XylF (calculated molecular mass of 37,069 Da) appears to be a lipoprotein attached to the cell membrane via a lipid anchor covalently linked to the N-terminal cysteine, as demonstrated by metabolic labelling of the recombinant XylF with [14C]palmitate. The induced E. coli avidly bound D-[14C]xylose, yielding additional evidence that T. ethanolicus XylF is the D-xylose-binding protein. On the basis of sequence comparison of XylFs to other monosaccharide-binding proteins, we propose that the sequence signature of binding proteins specific for hexoses and pentoses be refined as (KDQ)(LIVFAG)3IX3(DN)(SGP)X3(GS)X(LIVA)2X2A. Transcription of the monocistronic 1.3-kb xylF mRNA is inducible by xylose and unaffected by glucose. Primer extension analysis indicated that xylF transcription initiates from two +1 sites, both situated within the xylAB operon. Unlike in similar transport systems in other bacteria, the genes specifying the membrane components (e.g., ATP-binding protein and permease) of the high-affinity D-xylose uptake system are not located in the vicinity of xylF in T. ethanolicus. This is the first report of a gene encoding a xylose-binding protein in a gram-positive or thermophilic bacterium.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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D-Xylose is nature's second-most-abundant carbohydrate. The initial steps of D-xylose metabolism in bacteria typically involve transport, isomerization to D-xylulose, and phosphorylation to D-xylulose-5-phosphate. The second and third steps of this pathway are catalyzed by D-xylose (D-glucose) isomerase (XylA) and xylulose kinase (XylB), respectively (4), while xylose uptake is mediated via at least two distinct transport systems: low-affinity ion-linked symport and the binding protein-dependent transport system, also referred to as ABC-type transport (ATP-binding cassette). Low-affinity xylose transport requires an electromotive gradient and is mediated by a single membrane protein, XylE, as established by genetic and molecular evidence in Escherichia coli (6, 24) and Bacillus megaterium (42). ABC-type transport of xylose, shown to function so far only in E. coli and Salmonella typhimurium (1, 43, 48), involves a periplasmic protein, XylF, which binds xylose with high affinity. Two additional components are postulated to participate in binding protein-dependent xylose uptake on the basis of DNA sequence homology with other ABC transporters of monosaccharides, i.e., a membrane-spanning permease, XylH, which receives the sugar from XylF and translocates it to the cytoplasm and an ATPase, XylG, that energizes the substrate translocation process (46).
In thermophilic anaerobic bacteria, xylose utilization has been studied mostly at the biochemical level. In the past few years, xylA gene products from several thermoanaerobes have been cloned and characterized for possible application in the production of high-fructose corn syrup (7, 25, 27, 31). However, virtually nothing is known about molecular aspects of xylose transport in these interesting organisms. We recently reported that xylA and xylB in Thermoanaerobacter ethanolicus, a gram-positive xylanolytic thermophilic anaerobe, constitute a xylose-inducible, bicistronic operon (8). In this study, we show that the T. ethanolicus xylF, encoding D-xylose-binding protein, lies downstream from the xylAB operon and that its expression is also transcriptionally regulated. In addition, we provide evidence that the T. ethanolicus XylF is a lipoprotein that has sequence similarities with other monosaccharide-binding proteins and several transcriptional regulators of carbon metabolism.
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Bacterial strains, plasmids, and growth conditions.
T.
ethanolicus 39E (ATCC 33223) was grown as previously described
(9). Plasmids pUC18 (Life Technologies, Gaithersburg, Md.)
and pBluescript II KS (Stratagene, La Jolla, Calif.) were used as
cloning vectors in Escherichia coli DH5
(Life
Technologies, Gaithersburg, Md.). The E. coli strains were
grown in Luria-Bertani medium (39) supplemented with
ampicillin (100 µg/ml) or carbenicillin (50 µg/ml) as needed.
Construction and screening of genomic library.
A T. ethanolicus genomic library was prepared as previously described
(9). Probes for chromosome walking were prepared by random
hexamer labelling of the appropriate restriction fragments with
[-32P]dATP (39). Colony hybridization and
washes, as well as recombinant DNA manipulations, were carried out by
standard techniques (39).
DNA sequencing and analysis. Dideoxy-termination DNA sequencing was performed by following the Sequenase 2.0 kit (Amersham) protocol with double-stranded plasmid templates isolated by a boiling minipreparation procedure (39). Oligonucleotides were synthesized by Integrated DNA Technologies (Coralville, Iowa). Sequence analyses were performed by using the Lasergene biocomputing software package (DNASTAR, Madison, Wis.). BLAST search engines were employed for sequence homology searches (2).
PCR. Amplifications were performed as described previously (9), with the following modifications: pF-28 DNA (5 ng per reaction) was used as a template, the total number of cycles was 30, and the annealing temperature for the xylF-specific PCR product was 59°C. The oligonucleotides used for PCR of the xylF fragment were 5'AAT CTA GAT TCA AAC AAA ATT TTA GGA AGG AG and 5' AAG AAT TCA CTA TTA GCC GAT TGA ACT AAC.
RNA isolation and analyses.
Cells were harvested during the
logarithmic growth phase, and washed once in 50 mM Tris-Cl (pH 7.5),
and RNA was isolated with RNeasy Total RNA miniprep kits (Qiagen,
Chatsworth, Calif.). For Northern analysis, aliquots of total RNA (5 µg) were fractionated in a 1% agarose-formaldehyde gel, blotted,
and hybridized to the [-32P]dATP-labelled
xylF DNA internal fragment according to standard protocols
(39). The xylF probe was a PCR-amplified 323-bp
fragment from xylF. Transcript sizes were determined by
using the 0.24- to 9.5-kb RNA ladder (Life Technologies).
-32P]dATP and Klenow fragment by
following a standard protocol (39). The DNA template for the
antisense riboprobe was constructed by subcloning the 3'-terminal
SpeI-EcoRI fragment from pXI-10 (Fig. 1 in
reference 8; the EcoRI site was from the
vector) into pBluescript II KS. The SpeI-linearized template
was transcribed in vitro with T3 RNA polymerase in the presence of
[-32P]CTP (39), yielding a 608-nucleotide
antisense RNA.
Primer extension analysis was performed as previously described
(8) by using the oligonucleotide 5' ATG CAT ATG GAT TGT TTG
ATT TTG GTC CTT C, which is complementary to the sequence beginning 57 nucleotides downstream from the xylF translation initiation
site. For dot blot analysis, 1.5-µl aliquots of various dilutions of
total RNA isolated from T. ethanolicus 39E cells grown in
the presence of different carbon sources were spotted onto a membrane
which was hybridized to the same radiolabelled xylF-specific
probe used for Northern analysis. A standard hybridization procedure
was used (39).
Cloning and expression of the recombinant XylF.
The
xylF open reading frame (ORF) was PCR amplified by using
oligonucleotides 5' AGG AGA ATA GAC CAT GGT TAA AAA AGT CTC
and 5' GGC AAC AGT GGA TCC AGT TTT TCA AGA G, containing NcoI and BamHI sites (shown in boldface),
respectively. The pET15b expression vector (Novagen, Madison, Wis.) was
cut with NcoI and BamHI and dephosphorylated with
calf intestine alkaline phosphatase (New England Biolabs, Beverly,
Mass.) according to the manufacturer's instructions. Both the plasmid
and the NcoI-BamHI-cleaved xylF ORF
PCR product were then purified with GeneClean (Bio101, Vista, Calif.),
and the appropriate amounts were ligated with T4 DNA ligase. An aliquot
of the ligation mix was electroporated into E. coli JM109
(Promega, Madison, Wis.) and the recombinant transformants were
selected after restriction analysis of plasmid minipreparations. A
positive clone, pXFe, was then transformed into the expression host,
E. coli HMS174(DE3), by the CaCl2 procedure
(39). E. coli cells containing pXFe were grown in
Luria-Bertani medium supplemented with 50 µg of carbenicillin per ml.
Expression of the recombinant protein was induced by adding
isopropyl-
-thiogalactoside (IPTG [1 mM]) to liquid cultures that
reached an optical density at 600 nm (OD600) of
approximately 0.6.
Localization of the recombinant XylF and binding assay. Periplasmic fractions were isolated from cultures (16 ml) by a cold osmotic shock procedure, as previously described (3). Inner (cytoplasmic) membranes were fractionated from outer membranes by a sucrose gradient procedure (32).
D-Xylose binding activity was assayed by a modified filter binding method as described by Richarme and Kepes (36). Assays (100 µl) contained 50 mM Tris-HCl (pH 7.5), 6.9 µM D-[U-14C]xylose (250 mCi/mmol), and the various isolated fractions. After incubation at 70°C for 30 s, the mixture was placed in an ice bath, and 2 ml of ice-cold 50 mM Tris (pH 7.5) saturated with ammonium sulfate was immediately added. After 10 min, the mixture was filtered through 0.45-µm-pore-size nitrocellulose filters which had been soaked in 50 mM Tris (pH 7.5). The filtered material was washed with an additional 2 ml of the Tris-ammonium sulfate solution. Filters were dried for 20 min at 110°C, and radioactivity was determined after the addition of scintillation fluid. Preliminary experiments demonstrated that less than 0.5% of the radiolabelled xylose bound to filters in the absence of cellular protein.Metabolic radiolabelling of the recombinant XylF. Two cultures of E. coli cells (10 ml each) carrying pXFe were grown until the OD600 reached 0.5, when [14C]palmitic acid (specific activity, 52 mCi/mmol) was added to a final concentration of 0.75 µCi/ml. Cell growth was continued until an OD600 of 0.6 was reached, when IPTG was added at 1 mM to one of the cultures. The cells were grown for an additional 90 min and then harvested by centrifugation (10,000 × g, 5 min). Cell pellets were washed twice in 1 ml of 50 mM Tris (pH 7.5), and final pellets were resuspended in 100 µl of sodium dodecyl sulfate (SDS) extraction buffer (50 mM Tris [pH 7.5], containing 2% SDS, and 0.1% 2-mercaptoethanol). Cell extracts were then incubated at 70°C for 15 min, and cell debris was removed by centrifugation. Supernatant aliquots (5 µl) were run in an SDS-10% polyacrylamide gel, which was stained with Coomassie blue, destained, dried, and exposed to film for 4 weeks at room temperature.
Nucleotide sequence accession number. The complete xylF DNA sequence is available in GenBank under accession no. AF043466.
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Cloning and nucleotide sequence analysis. The ORF analysis of the T. ethanolicus genomic clone pXI-10 containing the xylAB operon, characterized in a previous study (8), revealed an N-terminal portion (93 amino acid residues) of a putative polypeptide 3' to the xylB ORF. A homology search for its sequence was performed with combined protein sequence databases and yielded the periplasmic D-xylose-binding protein precursor, XylF, from E. coli (48) as having the sequence with the highest similarity score (data not shown). Therefore, the 3'-terminal SpeI-EcoRI fragment from pXI-10 was used to screen the T. ethanolicus 39E genomic library for overlapping clones homologous to xylF. Two positive clones were identified, one of them carrying the complete ORF.
The putative 1,101-bp xylF ORF begins 89 bp downstream of the xylB termination codon with an ATG, preceded by a possible ribosome-binding sequence complementary to the 3' end of the T. ethanolicus 39E 16S rRNA (35). The coding region is flanked at its 3' terminus by the TGA triplet, specifying a translation termination codon (data not shown). A palindromic sequence was found downstream of the ORF 3' end that may serve as a transcription termination signal (data not shown). The G + C content of this ORF was 34.9 mol%, which matches the value of 35 mol%, experimentally determined for T. ethanolicus 39E total DNA (28). The deduced peptide contains 366 amino acid residues, giving a calculated molecular mass of 39,809 Da. The database homology search against the complete ORF confirmed that its sequence was homologous to the E. coli XylF (48) and a putative XylF from Haemophilus influenzae (11), with 61 and 60% amino acid sequence identity, respectively. The next consecutive ORF was located 426 bp downstream of the xylF ORF, and it had the opposite polarity. However, given the lack of sequence homology to any known proteins, no function could be assigned to this hypothetical peptide (data not shown). Three more ORFs were identified in the contiguous sequence of pF-28, all showing high similarities with genes encoding enzymes of the histidine biosynthesis pathway (10).Amino acid sequence analysis.
The 25-residue amino-terminal
fragment of the T. ethanolicus XylF has three distinct
domains: i.e., a positively charged N-terminal region, followed by a
highly hydrophobic central region which ends with a stretch of short
side chain neutral amino acids (data not shown). Such a sequence
structure is typical of signal peptides in bacterial lipoproteins which
are cleaved off at the cysteine residue (52), thus rendering
Cys-26 the N terminus of the mature T. ethanolicus XylF
protein, with a calculated molecular mass of 37,069 Da. The sequence
LSGC, corresponding to residues 23 to 26 in T. ethanolicus
XylF (data not shown), perfectly matches the four-residue sequence
consensus L(S,A)(A,G)
C defined for lipoprotein leader sequences
(49, 52). Taken together, these observations strongly
suggested that the processed, mature form of T. ethanolicus
XylF is a lipoprotein. The putative signal peptide is followed by a
22-residue stretch, rich in polar amino acids, e.g., serine, threonine,
and asparagine (7, 5, and 4 residues, respectively [Fig.
1]).
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Characterization of transcription.
In order to perform
Northern analysis, equal amounts of RNA from cells cultivated with
xylose or glucose were hybridized against a 323-bp fragment from
xylF. A prominent band, approximately 1.3 kb in size, was
seen only in RNA from xylose-grown cells (Fig. 2A). Two other faint bands (approximately
5 and 4 kb long) were detected when xylose was the energy source. DNA
sequence analysis (reference 8 and this study)
showed that an inverted repeat (
G = 
10.5
kcal/mol), followed by a poly(dT) stretch, is located in the
xylB-xylF intercistronic spacer (Fig. 3B). Northern analysis suggested that this sequence is likely to function as a 
-independent termination hairpin of xylAB transcription; therefore, the
majority of xylF mRNA appeared to be monocistronic.
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Expression of the recombinant XylF. SDS-PAGE was carried out to analyze the expression of the T. ethanolicus XylF in E. coli (Fig. 5). A highly abundant protein band migrating at approximately 37 kDa was observed in cell lysates of induced cells, but not in uninduced cells or cells carrying only the vector. The isolation of the periplasmic fraction by cold osmotic shock showed that the recombinant enzyme was not present in the host periplasm (data not shown). To test the functionality of the recombinant XylF, a D-xylose binding assay was performed with crude extracts from host cells harvested 2 h after induction. The induced cells had 40-fold-higher D-xylose binding activity than the uninduced cells, e.g., 1.58 versus 0.04 nmol of D-[14C]xylose bound per mg of protein by induced versus uninduced cells. Similar specific activities of D-xylose binding were found in both inner and outer membranes (data not shown).
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Metabolic radiolabelling of the recombinant XylF. The amino acid sequence analysis suggested that the native T. ethanolicus XylF is a lipoprotein. Biochemical evidence to support this hypothesis could be provided by covalently linking the recombinant XylF to a radiolabelled fatty acid. A similar approach has been used to identify lipoproteins in other gram-positive bacteria (49). In an attempt to accomplish this, the host cells harboring the recombinant clone were grown in the presence of [1-14C]palmitic acid prior to induction. Cell lysates of radiolabelled cells were then subjected to SDS-PAGE, followed by autoradiography (Fig. 6). The result clearly showed the presence of a radioactively labelled protein corresponding in size to the recombinant XylF, and this protein was absent in the control (uninduced) cells. Thus, E. coli performed posttranslational fatty acyl modification of the recombinant XylF.
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DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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To our knowledge, the molecular analysis of the T. ethanolicus xylF presented here is the first report of a gene encoding D-xylose-binding protein in a gram-positive bacterium and in a thermophilic organism. We have provided evidence strongly suggesting that the T. ethanolicus XylF is a lipoprotein: (i) the sequence begins with a putative signal peptide that contains the lipoprotein-scission consensus site (52); (ii) metabolic labelling with [14C]palmitate yielded a radiolabelled protein of the size corresponding to XylF; and (iii) the recombinant XylF was associated with cell membrane fractions, as is typical of bacterial lipoproteins (33). The last observation is particularly interesting in light of the fact that the entire xylF coding region, including the signal sequence, was present in the recombinant construct. Clearly, the cleavage sequence of T. ethanolicus XylF was recognized by the E. coli enzymatic machinery responsible for translocation, processing, and localization of lipoproteins.
There have been several reports that overproduction of heterologous lipoproteins is harmful for E. coli hosts (49). We have demonstrated that the T. ethanolicus XylF was not only highly expressed in E. coli, but also that it was functional, as could be inferred from the high D-xylose binding activity observed in induced cells. Since T. ethanolicus is gram-positive, it is likely that the native XylF is anchored to the external surface of the cell membrane by a lipid moiety thioacylated to the amino-terminal cysteine of the mature protein, as has been demonstrated in ligand-binding proteins from other gram-positive bacteria (49).
The signal peptide of the T. ethanolicus XylF is abutted by
a sequence region rich in serine, threonine, and asparagine. A similar
sequence was also observed in the N terminus of another mature
lipoprotein, an -amylase of a hyperthermophile, Thermotoga maritima (29). These sequences, dubbed "linkers,"
are also found in immunoglobulin 1A, a pullulanase, xylanases, and
cellulases, where they join different domains within an enzyme
(13, 26). It has been postulated that a linker in a cell
membrane-anchored lipoprotein enhances enzyme performance by serving as
an extended spacer relative to the cell surface (29). The
noticeable lack of linkers in periplasmic monosaccharide-binding
proteins (Fig. 1) supports this view. Further work is needed to
determine whether the linker facilitates interactions of XylF with
membrane-associated transport proteins during D-xylose
transport.
The marked binding of D-xylose by E. coli carrying the recombinant XylF suggested that the protein also functions in vivo in T. ethanolicus. Our preliminary transport studies indicate that a high-affinity D-xylose uptake system does operate in T. ethanolicus (10). These observations imply the existence of additional components needed for binding protein-dependent transport of D-xylose in T. ethanolicus, i.e., a permease, and an ATP-binding protein. In E. coli, genes encoding these two enzymes (XylH and XylG, respectively) are clustered together with xylF in the xylFGHR operon (48), where xylR codes for a transcriptional regulator of xylose utilization (47). In H. influenzae, D-xylose transport genes also constitute an operon, xylFGH (11). The operon organization is characteristic of genes encoding ABC transporters of other mono- and disaccharides (12), metals, ions, and peptides (12, 17). However, our finding that no sequences homologous to either xylG or xylH lie in the same genomic locus with xylF in T. ethanolicus represents an exception to this paradigm. Similarly, it was recently reported that genes encoding ATP-binding proteins which mediate maltose transport in Streptomyces reticuli (41) and Thermoanaerobacterium thermosulfurigenes (38) are not situated within operons. It remains to be elucidated how the regulation of expression of these remote cistrons is coordinated.
The solitary location of xylF on the T. ethanolicus chromosome relative to putative xylG and xylH is also reflected in the monocistronic nature of the xylF mRNA. Our RNA analyses indicated that the inverted repeat, located in the xylB-xylF intercistronic spacer (Fig. 3B), is likely to function as an efficient transcriptional terminator, yielding barely detectable xylABF read-through transcripts. Both xylF +1 sites are situated within the xylAB operon. The question as to how the transcription of xylAB is coupled with xylF expression, with respect to the two internal xylF promoters, awaits further study.
As the RNA dot blot data demonstrated, transcription of T. ethanolicus xylF is inducible by xylose and is not repressed by glucose. Such a phenomenon, also observed in regulation of xylAB transcription in T. ethanolicus (8), is markedly different from those in other xylose-utilizing bacteria, where glucose exerts strong inhibition of xylose utilization via several distinct mechanisms, most frequently, catabolite repression (21). Previously, a palindromic sequence was identified in the vicinity of the xylAB +1 site (8) and was postulated to serve as a T. ethanolicus xylose operator (xylO) on the basis of its striking sequence similarity to xylO palindromes, with the sequence consensus TTNGTTTNNNNNNNAAACNAA (5), mediating negative regulation of xylose catabolism in bacilli, Staphylococcus xylosus, and Lactobacillus pentosus (23, 30, 37, 45). In this respect, it was intriguing to find that an inverted repeat, TTTGTTTGATTT-23 bp-AATTCAAACAAA, with half-sites perfectly matching corresponding portions in the xylO consensus sequence, lies adjacent to the downstream transcription initiation site of xylF (Fig. 3B). In B. subtilis, an oligomeric xylose repressor, XylR, was shown to bind two tandemly repeated overlapping palindromes spaced 4 bp apart (5). Notably, the xylO sites do not have to overlap for binding to occur (i.e., XylR can bind isolated palindromes as single sites) (5). However, without experimental evidence, it is difficult to explain how an XylR homolog in T. ethanolicus would achieve simultaneous binding of the xylF palindromes spaced by the 23-bp loop. Future studies should show whether a looping mechanism, analogous to that observed in L-arabinose operon regulation by AraC (40), may be involved in regulation of xylF expression in T. ethanolicus. Nevertheless, the presence of conserved palindromes adjacent to both xylAB and xylF promoters and similar expression patterns of the two operons with respect to the carbon sources suggest that both xylAB and xylF operons may be controlled by a similar mechanism of negative regulation. Interestingly, the inverted repeat implicated in the xylAB transcription termination coincides with the putative xylF operator sequence. Hence, this might serve as an example of versatility of cis-acting elements in transcriptional regulation of bacterial carbon metabolism.
A recent study showed that XylFs from E. coli and H. influenzae are more closely related to the A. tumefaciens multiple-sugar-binding protein ChvE than to the E. coli periplasmic receptors of L-arabinose, D-glucose or D-galactose, or D-ribose (22). Our inclusion of T. ethanolicus XylF in the multiple sequence comparison confirmed this observation. Significantly, our sequence analysis indicated that most residues involved in protein-sugar interactions in E. coli monosaccharide-binding transporters (i.e., AraF, MglB, and RbsB) appear to be either fully conserved or replaced by isofunctional residues in D-xylose-binding proteins. In E. coli AraF and MglB, they include residues that sandwich sugar molecules inside the protein cleft by stacking interactions and those forming hydrogen bonds with sugars, which confer substrate specificity (34).
We also noted, for the first time, that XylF sequences possess a region closely matching a sequence pattern of binding proteins specific for hexoses and pentoses, the so-called cluster 2 signature. This consensus was defined as K(LIVFAG)3IX3D(SGP)X3(GS)X(LIVA)2X2A, where boldface letters indicate invariant residues in all of the relevant sequences available at the time (50). Our inclusion of XylFs in multiple sequence alignment revealed two residues in XylFs that deviate from this consensus (Fig. 1). Thus, we propose that the cluster 2 sequence signature be refined as (KDQ)(LIVFAG)3IX3(DN)(SGP)X3(GS)X(LIVA)2X2A, where boldface letters reflect the changes introduced. This may facilitate future sequence analyses of sugar-binding proteins.
At present, it is not clear which residues and/or interactions are responsible for the presumed thermostability of XylF in the thermophilic bacterium T. ethanolicus. The amino acid composition analysis of its predicted sequence (data not shown) compared to that of mesophilic XylFs did not reveal any obvious differences, with one exception: there are three cysteines in the peptide chain of the T. ethanolicus XylF, unlike in the other two XylFs, which completely lack cysteine residues. Now that the recombinant T. ethanolicus XylF is available, it will be possible to examine if a disulfide bridge is present in the mature, properly folded protein, and, if so, whether such a conformation is required for the protein thermostability, as has been documented for numerous other thermostable enzymes (14).
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ACKNOWLEDGMENT |
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This work was supported by the U.S. Department of Agriculture under agreement 95-37500-1793.
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FOOTNOTES |
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* Corresponding author. Mailing address: 212 W. P. Garrigus Building, Department of Animal Sciences, University of Kentucky, Lexington, KY 40546-0215. Phone: (606) 257-7554. Fax: (606) 257-5318. E-mail: strobel{at}pop.uky.edu.
Published with the approval of the Director of the Kentucky
Agricultural Experiment Station as journal article no. 98-07-80.
Present address: Department of Biochemistry, Chandler Medical
Center, University of Kentucky, Lexington, KY 40536-0084.
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REFERENCES |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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