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Previous Article | Next Article 
Journal of Bacteriology, February 2001, p. 1133-1139, Vol. 183, No. 4
Department of Microbiology, University of
Hawaii, Honolulu, Hawaii 96822,1 and
Institute for Genetics and Microbiology, University of
Munich, Munich, Germany2
Received 16 August 2000/Accepted 6 November 2000
Listeria monocytogenes serotype 4b strains account for
about 40% of sporadic cases and many epidemics of listeriosis.
Mutations in a chromosomal locus resulted in loss of reactivity with
all three monoclonal antibodies (MAbs) which were specific to serotype 4b and the closely related serotypes 4d and 4e. Here we show that this
locus contains a serotype 4b-4d-4e-specific gene cassette (3,071 bp)
which consists of two genes, gltA and gltB, and
is flanked by palindromic sequences (51 and 44 nucleotides). Complete loss of reactivity with the three serotype-specific MAbs resulted from
insertional inactivation of either gltA or
gltB. The gltA and gltB mutants
were characterized by loss and severe reduction, respectively, of
glucose in the teichoic acid, whereas galactose, the other
serotype-specific sugar substituent in the teichoic acid, was not
affected. Within L. monocytogenes, only strains of
serotypes 4b, 4d, and 4e harbored the gltA-gltB cassette,
whereas coding sequences on either side of the cassette were conserved among all serotypes. Comparative genomic analysis of a serotype 1/2b strain showed that the 3,071-bp gltA-gltB cassette was
replaced by a much shorter (528-bp) and unrelated region, flanked by
inverted repeats similar to their counterparts in serotype 4b. These
findings indicate that in the evolution of different serotypes of
L. monocytogenes, this site in the genome has become
occupied by serotype-specific sequences which, in the case of serotype
4b, are essential for expression of serotype-specific surface antigens
and presence of glucose substituents in the teichoic acids in the cell wall.
Numerous serotypes of Listeria
monocytogenes have been identified using the antigenic scheme of
Seeliger and Hoehne (16). However, three serotypes, 1/2a,
1/2b, and 4b, account for more than 95% of clinical isolates
(5). Serotype 4b is of special interest, as it is
implicated in about 40% of sporadic cases and the majority of
epidemics of food-borne listeriosis reported in Europe and North
America during the past 20 years (1, 7, 15). This may
reflect relatively high virulence of serotype 4b strains for humans,
although unique pathogenesis attributes of this serotype have not yet
been identified.
The somatic component of the serotypic designation in
Listeria resides primarily in the anionic polymer, teichoic
acid (TA), which consists of polyribitol phosphate and is covalently
linked to peptidoglycan (4, 6, 18). Glycosidic
substitution(s) of the ribitol phosphate units render the TA variable,
structurally and antigenically, among different serotypes. In serogroup
1/2 (e.g., serotypes 1/2a and 1/2b), N-acetylglucosamine and
rhamnose are present as substituents on the ribitol, whereas in
serogroup 4, N-acetylglucosamine is integral to the TA
chains. A unique glycosidic substitution pattern is present in serotype
4b, where the integral N-acetylglucosamine bears both
galactose and glucose substituents (4, 18).
In an effort to develop tools useful for the identification of
antigenic and genetic attributes unique to serotype 4b bacteria, we
have used monoclonal antibodies (MAbs) (c74.22, c74.33, and c74.180)
which reacted with strains of serotypes 4b, 4d, and 4e (referred to
collectively as serotype 4b-4d-4e) (8) to identify serotype-specific genomic regions. One such region was shown to harbor the serogroup 4-specific gene gtcA, which has been
recently described (14). Insertional inactivation of
gtcA resulted in loss of reactivity with one of the MAbs
(c74.22), loss of galactose, and marked reductions in the glucose in
the TA of the cell (14). A different genomic
region was found to be specific to serotypes 4b, 4d, and 4e, and
mutants in this region lacked reactivity with all three MAbs
(10). Here we report the cloning and characterization of
the genes composing this region and provide genetic evidence for their
involvement in serotype-specific surface antigen expression and TA
glycosylation in L. monocytogenes serotype 4b.
Bacterial strains and media.
Listeria and
Escherichia coli strains were grown and preserved as
described before (14). Antibiotics used for
Listeria and for E. coli were as described before
(14). Generation of transposon mutants of the serotype 4b
strain 4b1 and screening of the mutants with the MAbs have been
described elsewhere (10).
Biochemical analysis of cell wall composition.
Cell wall
composition was determined as described by Fiedler et al.
(4). TA from Listeria was prepared and analyzed
as previously described (4, 6).
Molecular procedures.
Procedures for extraction of plasmid
DNA from E. coli and genomic DNA from
Listeria and for nonradioactive labeling and detection of
DNA were previously described (10). Fragment XL7-1, which flanks the single transposon insertion in mutant XL7, has been described elsewhere (10). This fragment was sequenced, and
inverse PCR (13) was employed to obtain genomic
fragments on either side, using as template genomic DNA of the
wild-type strain 4b1 digested with EcoRI or
Sau3A, purified from low-melting-point agarose with
phenol-chloroform extractions (2), and self-ligated. Amplified fragments were cloned in pCR2.1 (Invitrogen) and sequenced. Sequence information was used to design new primers at the end of the
known sequence for additional inverse PCRs. Transposon-flanking fragments from other mutants were amplified using the Tn916
terminal primer OTL (5'-CGG AAT TCC GTG AAG TAT CTT
CCT ACA G-3') with a 5'-end EcoRI site (underlined)
and primer cP1 (5'-CAC AGA AGC GAT ACG ATG A-3').
Probe construction.
Probe locations are shown in Fig.
1. Probe XL7-1 (1.1 kb), which flanks the
transposon insertion in mutant XL7, has been described elsewhere
(10). Probe XL7-4 (0.6 kb) is internal to open reading frame Z (ORFZ) and consists of a 0.6-kb Sau3A fragment
cloned into pUC19. Probe XL7-5 (1.6 kb), which includes ORFP and part of ORFO, was obtained as a PCR fragment with primers
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.4.1133-1139.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
A Novel Serotype-Specific Gene Cassette (gltA-gltB) Is
Required for Expression of Teichoic Acid-Associated Surface
Antigens in Listeria monocytogenes of Serotype
4b
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
1F5 (5' CCG
ACT GTA TCT TCT TTT CC 3') and 1R9 (5' TTT GCT ACT CAA CGG AGC CAC 3') and 4b1 DNA as the template. The XL7-AB probe (2.9 kb), which includes both gltA and gltB, was
obtained as a PCR fragment using primers 2P3 (5'-GTA ACG TCT CAT
ATA GGG AG-3') and 1R5 (5'-GTA GAA CAA TTG TAG TAC CG-3').
DNA fragments were isolated from low-melting-point agarose gels,
purified by phenol-chloroform extractions (2), and labeled
with a Genius kit.
View larger version (18K):
[in a new window]
FIG. 1.
Genomic organization of the region harboring the
transposon insertion in mutant XL7. Open arrows indicate ORFs and
predicted direction of transcription. Slashes at the borders indicate
that ORFW and ORFO are partial; lollipops represent putative stem-loop
structures. The location of the Tn916 
E insertion in
gltA (Tn) is indicated by a triangle. Thick lines represent
DNA fragments used as probes in Southern blots, and arrowheads at the
bottom indicate primers used in RT-PCR. RT-PCR was done as described in
Materials and Methods with -1R1 as the primer for cDNA synthesis.
The gel shows products of PCRs with cDNA as the template and the
primer pairs -1R1-PCT1-1 (lane 1), cP1-3-2P3 (lane 2), 3R2-3F2 (lane
3), and 4R2-3F2 (lane 4). Negative controls (using RNA instead of
cDNA as the template and the same pairs of primers) were devoid of
any product (data not shown).
RT-PCR. Procedures for RNA extraction from Listeria, construction of cDNA, and reverse transcription PCR (RT-PCR) were as described elsewhere (14).
Construction of integration mutant in gltB.
To
construct an integration mutant in gltB, an internal
fragment of the gene was cloned in the temperature-sensitive shuttle vector pKSV7 (17), and integrants were selected by growth
at the restrictive temperature (43°C) in medium containing
chloramphenicol (CM medium) as follows. The internal fragment was
amplified with primers 1F2 (5'-TTG GTA ACT CAC TAG TAC GT)
and 1R4 (5'-ACA AGC ACA AAC AAA GAC GC), cloned in
pCR2.1, recovered by EcoRI digestion, and subcloned into
EcoRI-digested and dephosphorylated pKSV7. The resulting
recombinant was electroporated into electrocompetent cells of the
parental strain 4b1 as previously described (14), and
transformants were isolated on CM medium after 48 h at 30°C. Integrants were isolated following four consecutive passages in CM
medium at the restrictive temperature (43°C) and confirmed by
Southern blotting. For colony immunoblots, the cultures were grown at
room temperature.
Construction of pKA and pKAB.
Listeria DNA
fragments harboring gltA and gltA-gltB were
amplified from DNA of the parental strain 4b1 by PCR using High
Fidelity enzyme (Roche). Fragment A (containing gltA) was
obtained by PCR using primers 2P3 and 1R1 (5'-CAA GGC AAG AGT
ACA GCT AC-3'). Fragment AB (containing gltA-gltB) was
amplified using primers 2P3 and 1R5 (described above for construction
of the gltA-gltB probe XL7-AB), which had a
HindIII site and a BamHI site, respectively, at the 5' end. The PCR fragments were excised from low-melting-point agarose gels, purified with phenol-chloroform, and cloned into pCR2.1.
Fragment A was isolated following digestion of the recombinant plasmid
with EcoRI and was subcloned into pKSV7 which had been digested by EcoRI and dephosphorylated. Fragment AB was
obtained following digestion of the plasmid with BamHI and
HindIII and directionally cloned into pKSV7 digested
with the same enzymes. The resulting plasmids, consisting of pKSV7 with
inserts of gltA and gltA-gltB, were named pKA and
pKAB, respectively. Upon electroporation, 100 µl of the cells was
plated on CM medium, and the plates were incubated at 30°C for 3 to 4 days.
Cloning of serotype 1/2b sequences.
Primers 2P2 (5'-
GAC CAT ATC GTC GTG CTA CA-3') and 1R65 (5'-CGA GCA TAC
AAG TGC TCG TT-3') were used to amplify a 1.1-kb DNA fragment
with DNA of strain F4242 (serotype 1/2b) as the template. The 1.1-kb
PCR product was directly cloned into pCR2.1 and sequenced on both strands.
DNA sequencing and sequence analysis. Nested deletions were generated using the Erase-a-Base system (Promega) as suggested by the vendor. DNA was sequenced and analyzed as previously described (14).
Nucleotide sequence accession number. The nucleotide sequence data for L. monocytogenes serotypes 4b and 1/2b have been deposited in GenBank under accession numbers AF033015 and AF033016, respectively.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Mutants negative for serotype-specific MAbs.
The
single-insertion Tn916E mutant XL7 lacked reactivity with
all three serotype-specific MAbs (C74.22, C74.33, and C74.180) but had
no readily detectable phenotypic differences from its wild-type
counterparts in terms of growth at 20 and 35°C, motility, sensitivity to serotype-specific phage 2671 or
Listeria-specific phage A511, hemolytic activity, and colony
or cellular morphology. Furthermore, four additional independent
transposon mutants (33N1, 33N2, 33N3, and 8A3) phenotypically identical
to XL7 were found to harbor transposon insertions in the same
EcoRI and HindIII genomic fragment as
XL7 (10), suggesting that the MAb-negative phenotype of
XL7 was associated with the Tn916E insertion. DNA sequence analysis of XL7-1 and of the additional fragments derived by
inverse PCR showed that the transposon was inserted in an ORF termed
gltA (for glucose in teichoic acid). The transposon
insertion sites in mutants 33N1, 33N2, 33N3, and 8A3 were within a
10-nucleotide (nt) region in gltA, which also harbored the
insertion in XL7. The target sequence for the transposon insertions
conformed to the consensus target sequence
(T[T/A]TTTTNNNNNNAAAAA[A/T]A)
for Tn916 (11).
Genomic organization and ORF analysis of the
gltA-gltB region.
Sequence analysis revealed six
complete ORFs (ORFX, ORFY, ORFZ, gltA, gltB, and ORFP) and
two partial ORFs (ORFW and ORFO) in this region (Fig. 1). ORFW
(partial), ORFX, ORFY, ORFZ, gltA, and gltB were
transcribed in the same direction and convergently to ORFP and ORFO
(partial). Two palindromic sequences with the potential to form
pronounced stem-loop structures flanked the gltA-gltB
region. The palindrome for putative stem-loop I (51 nt; calculated free
energy of formation, 46 kcal/mol) was in the region between ORFZ and
gltA, 55 nt downstream of ORFZ and 279 nt upstream of
gltA, whereas that for putative stem-loop II (44 nt;
calculated free energy of formation also 46 kcal/mol) was 8 and 27 nt
downstream of gltB and ORFP, respectively (Fig. 1). The
organization of the region suggests that stem-loops I and II may serve
as transcription terminators for ORFZ and ORFP, respectively.
gltA-gltB region.
The transposon-harboring
ORF (gltA) (1,647 bp) was 386 nt downstream of ORFZ.
We were unable to identify sequences upstream of gltA with
detectable similarity to the canonical Shine-Dalgarno ribosome
recognition sequences. A putative 10 promoter element (TATTAT)
was identified 92 nt upstream of the putative start codon of
gltA. The coding sequence of gltA appears to be
novel, as screens of the nucleotide and protein databases failed to
identify sequences with significant homology to either the gene or the
deduced gene product. The latter (548 amino acids, calculated
Mr of 62,755, pI 9.0) may be membrane associated
in L. monocytogenes, as hydrophobicity analysis of the
deduced polypeptide revealed 11 putative transmembrane segments (data
not shown).
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Coding sequences upstream of gltA-gltB (ORFW to ORFZ). BLAST and motif search analysis of the deduced amino acid sequences of ORFW (partial), ORFX, ORFY, and ORFZ suggested that all had characteristics of ABC (ATP-binding cassette) transporters (3). A putative ATP/GTP-binding site motif A (P loop) was identified in the deduced sequences of ORFX (residues 217 to 225) and ORFZ (residues 368 to 375). The ORFW-ORFX and ORFX-ORFY intergenic spaces were 2 and 21 nt, respectively, whereas the stop codon of ORFY overlapped by one nucleotide with the putative start codon of ORFZ, suggesting that ORFY and ORFZ are translationally coupled.
Coding sequences downstream of gltA-gltB (ORFP and
ORFO).
FASTA and BLAST analysis of ORFP, located downstream of
gltB and transcribed convergently, suggested that the
deduced product may be a penicillin-binding protein (PBP), having 34 to
55% identity over the entire amino acid sequence with PBPs from
numerous other bacteria. Highest similarity (55% identity) was
observed with the D-alanyl-D-alanine
carboxypeptidase, PBP5, of Bacillus subtilis (accession no. P08750). ORFP was preceded by ORFO (partial), transcribed in the same orientation as ORFP and separated from it
by 214 nt. The deduced ORFO product had 49 and 46% identity over
its entire available length (189 amino acids) with the
7-
-(4-carboxybutanamido)cephalosporanic acid acylase
(glutaryl 7-amino cephalosporanic acid [7-ACA] acylase precursor) of Bacillus laterosporus and with the cocaine
esterase of Rhodococcus sp. strain MB1, respectively. These
similarities are difficult to evaluate at this time, as such enzymatic
activities have not been detected before in L. monocytogenes.
Transcriptional studies.
The quantitative levels of
gltA-gltB transcripts were too low for reliable detection
and size determination by Northern blotting (data not shown), and
RT-PCR was used for transcriptional studies. When primer 1R1 (located
in gltB) was used for reverse transcription, a PCR product
of the expected size was obtained using primers 1R1 and PCT1-1
(spanning gltB and gltA) (Fig. 1, lane 1),
suggesting that gltA and gltB were cotranscribed.
Furthermore, the transcript contained the 386-nt region between
gltA and ORFZ, which includes the palindromic sequence, as
suggested by a product of the expected size with primers cP1-3 and 2P3
(located in the region between ORFZ and gltA) (Fig. 1, lane
2). Surprisingly, cDNA produced by primer 1R1 could be amplified
by primer 3R2 (located in the 3' region of ORFX) and either 3R2 or 4R2
(Fig. 1, lanes 3 and 4), suggesting that ORFY and ORFZ were included in
the transcript as well. These and additional RT-PCR data (not shown)
suggest the presence of transcripts harboring not only
gltA-gltB but also extending through the relatively long
(386-nt) region between gltA and ORFZ, to at least 2,287 nt
upstream of gltA. gltB appears to be the last ORF
in this transcriptional unit.
Insertional inactivation of either gltA or
gltB results in absence of glucose in the TA, whereas
galactose is not affected.
Transposon mutants in gltB
were not identified, and an integration mutant (4b1-INTB) was
constructed, using the temperature-sensitive plasmid pKSV7. Similarly
to XL7, the mutant had normal growth and other phenotypic
characteristics but lacked reactivity with all three MAbs (data not
shown). Biochemical analysis of TA from XL7 and 4b1-INTB showed that
both mutants were severely deficient in glucose. In contrast to the
wild-type parental strain 4b1, which had both galactose and glucose as
substituents on the N-acetylglucosamine of the TA, as is
typical of serotype 4b (4), glucose was undetectable in
the TA of XL7 and present in only trace amounts in the TA of 4b1-INTB
(Fig. 3). Interestingly, the other
serotype-specific substituent, galactose, was present in normal amounts
in the TA of the mutants, as were the integral components of TA
(ribitol phosphate and N-acetylglucosamine) (Fig. 3). The
loss of glucose in the TA of XL7 was also seen with the independently
obtained gltA mutants 33N1, 33N2, 33N3, and 8A3 (data not
shown).
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The MAb-negative phenotype of XL7 can be partially complemented by gltA alone or in combination with gltB. The recombinant plasmids pKA and pKAB, harboring gltA alone and together with gltB, respectively, were electroporated into mutant XL7. Both plasmids included 219 nt upstream of the start codon of gltA, since a promoter may be contained within this region. The resulting strains were grown in the presence of chloramphenicol at 30°C, a temperature which permits both replication of the temperature-sensitive plasmid (17) and optimal expression of the serotype-specific surface antigens (8). Reactivity of the mutant with c74.22, c74.33, and c74.180 was restored partially and to the same levels by both plasmids, whereas XL7 harboring the shuttle vector pKSV7 alone remained negative with the MAbs (data not shown). Although pKA and pKAB partially restored reactivity with the MAbs, glucose in the TA of the mutant was not restored to detectable levels (data not shown).
gltB is needed for heterologous expression of the serotype-specific surface antigens in strains of serotypes 4a and 4c. Strains of serotypes 4a and 4c lacked reactivity with the gltA-derived probe XL7-1 (10). When transformed with pKAB, strains ATCC 19114 (serotype 4a) and ATCC 19116 (serotype 4c) were rendered reactive with at least two of the MAbs, c74.22 and c74.33 (data not shown). When transformed by pKA these strains remained MAb negative, suggesting that gltB was required for expression of c74.22- and c74.33-specific surface antigens in these heterologous hosts.
Within L. monocytogenes, only strains of serotype
4b-4d-4e harbored sequences with homology to gltA and
gltB, whereas ORFP and ORFZ were conserved among different
serotypes.
Hybridizations using probe XL7-AB, which contains both
gltA and gltB, showed that the genes were unique
to L. monocytogenes serotype 4b-4d-4e and could not be
detected in DNA from strains of other serotypes. The genes have also
been detected in a unique lineage (lineage I) of L. innocua
(9). EcoRI restriction fragment length
polymorphisms using XL7-AB as the probe could differentiate between
L. monocytogenes serotype 4b-4d-4e and L. innocua
lineage I (Table 1). Southern blot and
PCR data suggest that the gltA-gltB cassette was
flanked by ORFZ and ORFP in L. innocua lineage I, as in L. monocytogenes serotype 4b (data not shown). No
hybridization was observed with DNA from other L. innocua
strains or other Listeria species (Table 1).
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Serotype 1/2b L. monocytogenes harbors a novel locus
genomically equivalent to the gltA-gltB cassette of
serotype 4b-4d-4e.
The genomic equivalent of the region
flanked by the conserved ORFZ and ORFP was amplified from strain F4242
(serotype 1/2b) as described in Materials and Methods. In serotype
1/2b, ORFP and ORFZ flanked a region of 528 bp, in contrast to 3,071 bp
in serotype 4b (Fig. 6). Interestingly,
the region in serotype 1/2b was flanked by palindromic sequences with
significant sequence identity (72 and 84%) to their counterparts in
serotype 4b (Fig. 7). The remainder of
the 528-bp region, however, showed no detectable homology with the
serotype 4b sequences. The 1/2b sequence contained only a small
potential coding sequence (ORFC, 75 amino acids), which was
preceded by a putative Shine-Dalgarno sequence 7 nt upstream of the
putative start codon. The palindromic sequence between ORFC and
ORFP was followed by a string of eight T's, suggesting that it
may function as a rho-independent terminator. The G+C content of ORFC
was unusually low (26%), and no homologous sequences were identified
in searches of the DNA and protein databases.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The ca. 3-kb gene cassette described here represents a novel serotype-specific locus present in serotype 4b L. monocytogenes and the genetically closely related (albeit relatively rare) serotypes 4d and 4e but in no other serotypes of the species. In addition, a unique L. innocua lineage that reacts with the serotype 4b-4d-4e-specific MAbs (9) also harbors the cassette, in the same genomic location as serotype 4b L. monocytogenes. The distribution of the cassette in Listeria parallels precisely the pattern of reactivity of the serotype-specific MAbs (8).
The genes on either side of the cassette were found to be conserved among different serotypes of L. monocytogenes as well as other Listeria species (L. innocua, L. ivanovii, and L. seeligeri). On one side, at least one of these genes (ORFP) may be involved in cell wall biosynthesis, the deduced product being a putative PBP. On the other side, we identified four genes with homology to ABC transporters. It remains to be determined whether the products of these genes mediate transport of cell wall or TA precursors.
The serotype-specific distribution of the cassette and its unusually low (for Listeria) G+C content suggest the possibility that it may have been introduced to the L. monocytogenes serotype 4b-4d-4e lineage by horizontal transfer from some unidentified source. From there it could have been transferred to lineage I of L. innocua, as has been speculated for the gtcA locus recently identified in this lineage (9). The origin of the serotype-specific sequences may be elucidated by future identification of homologous sequences in other bacteria or bacteriophage. It is tempting to speculate that the inverted repeats flanking the serotype-specific sequences may represent remnants of a genetic system (e.g., a transposon or phage) that may have mediated this transfer. These palindromic sequences may have assumed novel functions in their current locations in serotype 4b L. monocytogenes, possibly related to transcriptional termination, message stability, or other regulatory mechanisms. Interestingly, these inverted repeats were similar to their counterparts in serotype 1/2b. In the latter, however, the genomic location of the ca. 3-kb serotype 4b-4d-4e-specific cassette was occupied by a much shorter (528-bp) region, which harbors a novel, unrelated ORF. Involvement of the 1/2b region (ORFC) in expression of surface antigen(s) in serotype 1/2b remains to be determined.
The integrated genetic, immunological, and biochemical results suggest that in L. monocytogenes serotype 4b, the gltA-gltB cassette is involved in expression of the surface antigens recognized by MAbs c74.22, c74.33, and c74.180 and in the addition of glucose substituents on the TA, but the precise biochemical functions of the two genes remain to be elucidated. The genes can be cotranscribed, and at this time we cannot exclude the possibility that the transposon insertion in gltA may have polar effects on gltB. The fact that the observed phenotypic complementation of XL7, albeit partial, was conferred equally by pKA and pKAB suggests that gltB was expressed to some extent in this mutant. Construction of alternative mutants in gltA (such as an in-frame deletion) and/or alternative complementation strategies will be needed to more precisely address the function(s) of gltA. Sequence analysis could not facilitate functional predictions in the case of gltA, as both the gene and the deduced gene product appeared to lack homologs in the databases. The deduced gltB product, however, had significant similarity with numerous glycosylases and dolichol phosphate mannosyltransferases, and a glycosylase function would be in agreement with the observed deficiency of glucose in the TA of the gltB mutant.
Complementation of MAb reactivity of XL7 by gltA or gltA-gltB was partial, for reasons that are not clear but may involve absence of possibly required cis elements or suboptimal copy number of the genes in the vector that was used. The low level of complementation may account for the lack of detectable restoration of glucose in the TAs. Such difficulties with complementation were not experienced with the previously studied gene gtcA, where both MAb reactivity and TA glycosylation were restored by the wild-type gene in trans (14). The mechanisms controlling regulation of expression of gltA and gltB are not understood but may be complicated, as suggested by the presence of the long and apparently transcribed region between ORFZ and gltA.
Glycosylated TA components have been shown to be important antigenic determinants in L. monocytogenes (6, 19), although their role in infection has not been elucidated. It is worthy of note that even though gltA or gltB mutants grew normally in the laboratory, our surveys of numerous serotype 4b field isolates (both food and clinical) failed to identify strains which had the XL7 or 4b1-INTB phenotype or which lacked gltA-gltB sequences. One may speculate that because of its surface exposure, abundance, and immunogenicity, properly decorated TA may be important in interactions between the bacteria and their host cells. Glycosylated TA may also affect physiological attributes of the bacteria in foods or in the environment, in response to environmental stresses, association with surfaces and with other organisms in biofilms, etc. Continuing studies in our laboratory aim toward further elucidation of the serotype-specific gene cassettes described in this report in terms of their evolution and potential roles in adaptive physiology and pathogenesis of the listerial lineages which harbor them.
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ACKNOWLEDGMENTS |
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This research was partially supported by U.S. Department of Agriculture Competitive Research Initiative AAFS grant 99-35201-8183 and by ILSI North America.
We are grateful to Huyen Le Tran for assistance with graphics and to Vladimir Lazarevic for exchange of information related to teichoic acid biosynthesis genes. We thank Nattawan Promadej, Wei Zheng, Edward Lanwermeyer, and all other members of our laboratories for valuable feedback and support throughout the course of this work.
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FOOTNOTES |
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* Corresponding author. Present address: Department of Food Science, Food Pathogens Laboratory, North Carolina State University, Raleigh, NC 27695. Phone: (919) 513-2075. Fax: (919) 515-7124. E-mail: skathar{at}unity.ncsu.edu.
Present address: Biolog, Hayward, CA 94545.
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REFERENCES |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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| 1. |
Anonymous.
1999.
Update: multistate outbreak of listeriosis United States, 1998-1999.
Morbid. Mortal. Wkly. Rep.
47:1117-1118[Medline].
|
| 2. | Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. D. Seidman, J. A. Smith, and K. Struhl (ed.). 1987. Current protocols in molecular biology. Greene Publishing Associates and John Wiley & Sons, Inc., New York, N.Y. |
| 3. |
Fath, M. J., and R. Kolter.
1993.
ABC transporters: bacterial exporters.
Microbiol. Rev.
57:995-1017 |
| 4. | Fiedler, F., J. Seger, A. Schrettenbrunner, and H. P. R. Seeliger. 1983. The biochemistry of murein and cell wall teichoic acids in the genus Listeria. Syst. Appl. Microbiol. 5:360-376. |
| 5. | Gellin, B. G., and C. V. Broome. 1989. Listeriosis. JAMA 261:1313-1320[CrossRef][Medline]. |
| 6. |
Kaminsango, K.,
H. Fujii,
H. Okumura,
I. Saiki,
Y. Araki,
Y. Yamamura, and I. Azuma.
1983.
Structural and immunochemical studies of teichoic acid of Listeria monocytogenes.
J. Biochem.
93:1401-1409 |
| 7. | Kathariou, S. 2000. Pathogenesis determinants of Listeria monocytogenes, p. 295-314. In J. W. Cary, J. E. Linz, and D. Bhatnagar (ed.), Microbial foodborne diseases. Technomics Publishing Co., Inc., Lancaster, Pa. |
| 8. |
Kathariou, S.,
C. Mizumoto,
R. D. Allen,
A. K. Fok, and A. A. Benedict.
1994.
Monoclonal antibodies with a high degree of specificity for Listeria monocytogenes serotype 4b.
Appl. Environ. Microbiol.
60:3548-3552 |
| 9. |
Lan, Z.,
F. Fiedler, and S. Kathariou.
2000.
A sheep in wolf's clothing: Listeria innocua strains with teichoic acid-associated surface antigens and genes characteristic of Listeria monocytogenes serogroup 4.
J. Bacteriol.
182:6161-6168 |
| 10. | Lei, X.-H., N. Promadej, and S. Kathariou. 1997. DNA fragments from regions involved in surface antigen expression specifically identify Listeria monocytogenes serovar 4 and a subset thereof: cluster IIB (serotypes 4b, 4d, and 4e). Appl. Environ. Microbiol. 63:1077-1082[Abstract]. |
| 11. |
Lu, F., and G. Churchward.
1995.
Tn916 target DNA sequences bind the C-terminal domain of integrase protein with different affinities that correlate with transposon insertion frequency.
J. Bacteriol.
177:1938-1946 |
| 12. |
Morona, R.,
M. Mavris,
A. Fallarino, and P. A. Manning.
1994.
Characterization of the rfc region of Shigella flexneri.
J. Bacteriol.
176:733-747 |
| 13. | Ochman, H., M. M. Medhora, D. Garza, and D. L. Hartl. 1990. Amplification of flanking sequences by inverse PCR, p. 219-227. In M. A. Innis, D. H. Gelfand, J. J. Sninsky, and T. J. White (ed.), PCR protocols. Academic Press, Inc., San Diego, Calif. |
| 14. |
Promadej, N.,
F. Fiedler,
P. Cossart,
S. Dramsi, and S. Kathariou.
1999.
Cell wall teichoic acid glycosylation in Listeria monocytogenes serotype 4b requires gtcA, a novel, serotype-specific gene.
J. Bacteriol.
181:418-425 |
| 15. |
Schuchat, A.,
B. Swaminathan, and C. V. Broome.
1991.
Epidemiology of human listeriosis.
Clin. Microbiol. Rev.
4:169-183 |
| 16. | Seeliger, H. P. R., and K. Hoehne. 1979. Serotypes of Listeria monocytogenes and related species. Methods Microbiol. 13:31-49. |
| 17. | Smith, K., and P. Youngman. 1992. Use of a new integrational vector to investigate compartment-specific expression of the Bacillus subtilis spoIIM gene. Biochimie 74:705-711[Medline]. |
| 18. |
Uchikawa, K.,
J. Sekikawa, and I. Azuma.
1986.
Structural studies on teichoic acids in cell walls of several serotypes of Listeria monocytogenes.
J. Biochem.
99:315-327 |
| 19. |
Ullmann, W. W., and J. A. Cameron.
1969.
Immunochemistry of the cell walls of Listeria monocytogenes.
J. Bacteriol.
98:486-493 |
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| ALL ASM JOURNALS |
HindIII-digested molecular size markers
(fragment sizes [from the top to bottom], 23, 9.4, 6.6, 4.4, 2.3, 2.0, and 0.56 kb); lanes 2 to 15, L. monocytogenes F2381
(4b), G2228 (1/2a), F4242 (1/2b), F4254 (1/2b), LM103 (1/2c), ATCC
19113 (3a), G3331 (3b), SLCC 2540 (3b), G4315 (3c), SLCC 2479 (3c),
ATCC 19114 (4a), ATCC 19117(4d), ATCC 19118 (4e), and G2940 (4ab),
respectively; lanes 16 and 17, B. subtilis 168 and B. subtilis W23, respectively. Lanes 10 and 11 contained relatively
low amounts of DNA.
