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Infection and Immunity, May 1999, p. 2103-2109, Vol. 67, No. 5
Division of Infectious Diseases,
Received 30 September 1998/Returned for modification 30 December
1998/Accepted 27 January 1999
Escherichia coli K1 is the most common gram-negative
organism causing neonatal meningitis, but the mechanism by which
E. coli K1 crosses the blood-brain barrier is incompletely
understood. We have previously described the cloning and
molecular characterization of a determinant, ibeA (also
called ibe10), from the chromosome of an invasive
cerebrospinal fluid isolate of E. coli K1 strain RS218
(O18:K1:H7). Here we report the identification of another chromosomal
locus, ibeB, which allows RS218 to invade brain
microvascular endothelial cells (BMEC). The noninvasive
TnphoA mutant 7A-33 exhibited <1% the invasive ability of
the parent strain in vitro in BMEC and was significantly less invasive
in the central nervous system in the newborn rat model of hematogenous
E. coli meningitis than the parent strain. The
TnphoA insert with flanking sequences was cloned and
sequenced. A 1,383-nucleotide open reading frame (ORF) encoding a
50-kDa protein was identified and termed ibeB. This
ORF was found to be 97% identical to a gene encoding a 50-kDa hypothetical protein (p77211) and located in the 13-min region of the E. coli K-12 genome. However, no homology was
observed between ibeB and other known invasion genes when
DNA and protein databases in GenBank were searched. Like the
TnphoA insertion mutant 7A-33, an isogenic ibeB
deletion mutant (IB7D5) was unable to invade BMEC. A 7.0-kb locus
containing ibeB was isolated from a LambdaGEM-12 genomic
library of E. coli RS218 and subcloned into a
pBluescript KS vector (pKS7-7B). pKS7-7B was capable of completely
restoring the BMEC invasion of the noninvasive
TnphoA mutant 7A-33 and the ibeB deletion
mutant IB7D5 to the level of the parent strain. More importantly,
the ibeB deletion mutant IB7D5 was fully complemented by
pFN476 carrying the ibeB ORF (pFN7C), indicating that
ibeB is required for E. coli K1 invasion of
BMEC. Taken together, these findings indicate that several
E. coli determinants, including ibeA and
ibeB, contribute to crossing of the blood-brain barrier.
Bacterial meningitis has remained
associated with high mortality and morbidity despite advances in
antimicrobial chemotherapy and supportive care (16, 24). A
major contributing factor is the incomplete understanding of the
pathogenesis and pathophysiology of this disease. For example,
most cases of bacterial meningitis develop as a result of
hematogenous spread, but it is not completely understood how
circulating bacteria cross the blood-brain barrier.
Escherichia coli is the most common gram-negative
organism that causes meningitis during the neonatal period. Using
E. coli as a paradigm, we have examined how circulating
bacteria cross the blood-brain barrier. These studies have become
feasible because of the availability of both in vitro and in vivo
models of the blood-brain barrier (7, 22). For example, we
have successfully isolated and cultivated brain microvascular
endothelial cells (BMEC), which constitute the blood-brain barrier
(22, 23). The in vivo model of the blood-brain barrier has
been established by induction of hematogenous meningitis in infant rats
(7, 10). In this experimental meningitis model, bacteria are
injected via the subcutaneous or intracardiac route, resulting in
bacteremia and subsequent entry of bacteria into the central nervous
system (CNS). Since the blood-brain barrier separates the brain and
cerebrospinal fluid (CSF) from the intravascular compartment,
the entry of bacteria should occur at sites of the blood-brain barrier.
The development of techniques for atraumatic collection of blood and
CSF specimens has enabled us to use this in vivo model to examine the
pathogenic mechanisms involved in crossing of the blood-brain barrier
by circulating E. coli (10).
To facilitate the identification of the genes contributing to
E. coli invasion of BMEC, we have used transposon
TnphoA and generated a collection of noninvasive
E. coli mutants (7). TnphoA is
a modified transposon engineered by insertion of the phoA gene into one end of Tn5 (12).
The gene fusion can be randomly generated by TnphoA
insertion into the target gene in the chromosome or plasmid. The
TnphoA approach has led to the discovery of critical E. coli determinants involved in the invasion of BMEC
in vitro and in vivo. For example, we have previously identified the
ibeA (ibe10) locus via TnphoA
mutagenesis and screening for loss of invasiveness by use of the in
vitro and in vivo models of the blood-brain barrier (7). In
addition, we have shown that E. coli OmpA contributes
to the invasion of BMEC (15). In the present study, we
characterized the noninvasive mutant 7A-33, which was derived from a
CSF isolate of E. coli K1 strain RS218 by
TnphoA mutagenesis. This mutant was significantly less able
than the parent strain to invade BMEC in vitro and to enter the CNS in the newborn rat model of hematogenous meningitis in vivo. Similar findings were obtained with an ibeB deletion mutant. The DNA
fragments containing ibeB (invasion of brain endothelial
cells) were shown to restore the ability of the noninvasive mutant
7A-33 and the ibeB deletion mutant to invade BMEC.
Bacterial strains, plasmids, and media.
E. coli
RS218 (O18:K1:H7) is a clinical isolate from the CSF of a newborn
infant with meningitis (21), and E44 is a spontaneous rifampin-resistant mutant of RS218. DH5 Chemicals and enzymes.
Restriction endonucleases, T4 DNA
ligase, and other enzymes were purchased from New England Biolabs
(Beverly, Mass.) unless otherwise noted. Chemicals were purchased from
Sigma (St. Louis, Mo.). All isotopes were obtained from New England
Nuclear Corp. (Boston, Mass.). Reagents for preparation of DNA
sequencing gels were ultrapure quality and were obtained from National
Diagnostics (Atlanta, Ga.). Reagents for DNA sequencing reactions with
Sequenase and other chemicals were purchased from U.S. Biochemical
Corp. (Cleveland, Ohio). DNA sequencing kits with dye terminators were obtained from PE Applied Biosystems (Foster City, Calif.).
Isolation of the noninvasive TnphoA mutant 7A-33 of
E. coli K1.
The noninvasive TnphoA
mutant 7A-33 was generated as previously described (7).
Briefly, strain SM10 Tissue cultures and invasion assays.
BMEC were prepared from
bovine and human brains (22, 23), and invasion assays were
performed as previously described (7). Briefly, brain
specimens devoid of large blood vessels were homogenized in Dulbecco
minimal essential medium (DMEM) containing 2% bovine calf serum
(DMEM-S) and centrifuged in 25% bovine serum albumin for bovine BMEC
or in 15% dextran in DMEM-S for human BMEC. The pellets containing
crude microvessels were further digested in a solution containing
collagenase or dispase (1 mg/ml). Microvascular capillaries were
isolated by adsorption to a column of glass beads and were recovered in
growth medium (22). The resulting bovine and human BMEC were positive
for factor VIII, carbonic anhydrase IV, gamma-glutamyl transpeptidase,
and the ability to take up low-density lipoproteins, demonstrating
their brain endothelial cell characteristics (22, 23).
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Identification and Characterization of an Escherichia
coli Invasion Gene Locus, ibeB, Required for
Penetration of Brain Microvascular Endothelial Cells
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
is a host strain for subcloning and preparation of plasmids for DNA sequence determination. Strains containing plasmids were grown at 37°C in L broth (10 g of
tryptone, 5 g of NaCl, and 5 g of yeast extract per liter) with ampicillin (50 µg/ml), kanamycin (50 µg/ml), tetracycline (20 µg/ml), or chloramphenicol (100 µg/ml) for positive selection of
plasmids (Table 1). Bacteria were
cultured in L broth and stored in L broth plus 20% glycerol at
70°C.
TABLE 1.
E. coli strains and plasmids used in
this study
pir containing the suicide vector plasmid pRT733
was used as a TnphoA donor, while E. coli K1
strain E44 was used as a recipient. SM10pir carrying pRT733 was
mated with E44 on Luria-Bertani (LB) agar by cross-streaking and then
incubation at 37°C for 6 h. The conjugants were selected on LB
agar containing kanamycin and rifampin (7).
TnphoA mutants were screened for their ability to invade
BMEC as described previously (7). Probing of the DNA blots
with a 32P-labeled 0.6-kb Kanr gene fragment
derived from Tn5 identified noninvasive mutants with a
single TnphoA insertion (7).
Neonatal rat model of hematogenous E. coli K1 meningitis. The noninvasive mutant with a single TnphoA insertion (7A-33) was examined for its ability to enter the CNS in our neonatal rat model of hematogenous E. coli meningitis as described previously (7, 10). Briefly, at 5 days of age, all members of each litter were randomly divided into two groups to receive subcutaneously 1.4 × 104 CFU of the parent strain E44 or 4.4 × 104 CFU of the mutant strain 7A-33. Our pilot experiments revealed that these bacterial inocula for strains E44 and 7A-33 produced nonlethal bacteremia of 105 to 108 CFU/ml of blood in >90% of animals within 18 h of inoculation. At 18 h after bacterial inoculation, blood and CSF specimens were obtained for quantitative cultures as described previously (10). Blood and CSF specimens obtained from animals infected with mutant 7A-33 were cultured in brain heart infusion broth and agar containing kanamycin (40 µg/ml).
Cloning of TnphoA fragments.
MluI-digested
genomic DNA from the noninvasive mutant 7A-33 was cloned into the
MluI site of pCVD433, which was derived from pACYC184 by
insertion of MluI linkers into the EcoRV site
(3). Transformation was performed by electroporation of
E. coli DH5 in 10% glycerol with 0.1-cm cuvettes
and an E. coli gene pulser (Bio-Rad Laboratories,
Richmond, Calif.) set at 1.8 kV, 200 
, and 25 µF as previously
described (7). The kanamycin-resistant transformants were
identified as MluI fragments containing TnphoA. The construct carrying a 13-kb MluI fragment of the
noninvasive mutant 7A-33 in pCVD433 was designated pCD7A (Table 1).
PCR cloning and analysis of ibeB.
The PCR was
performed as described previously (8, 11). Briefly, 0.5 µg
of genomic DNA was added to a mixture containing 1× Taq
polymerase buffer (Cetus), 1.5 mM MgCl2, 0.5 mM
deoxynucleoside triphosphates (Cetus), 50 pmol of each primer, and
Taq DNA polymerase in a final volume of 50 µl.
Amplification was carried out with a PTC-100 programmed thermal
controller (M. J. Research) for 40 cycles: denaturation for 1 min
at 94°C, primer annealing for 1 min at 55°C, and primer extension
for 3 min at 70°C. The two pairs of primers (primers IB7-3a and
IB7-5a and primers IB-5HB and IB7-5a) (Table
2) used for the PCR were synthesized with
an Applied Biosystems (Foster City, Calif.) 380B DNA synthesizer. Two
DNA fragments, a 0.67-kb fragment carrying the partial ibeB
coding sequence and a 1.6-kb fragment containing the complete
ibeB open reading frame (ORF), were amplified from genomic
DNA of wild-type strain RS218 and subcloned into TA cloning vector
pCRII (Invitrogen). The resulting constructs were designated pCIB7B and
pCR7C, respectively (Table 1).
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DNA sequencing and analysis. The nucleotide sequence of ibeB was determined by the dideoxy chain termination method of Sanger et al. (19) with a Sequenase version 2.0 kit from U.S. Biochemical Corp. and [35S]dATP (1,000 to 1,500 Ci/mmol) from Du Pont, NEN Research Products (Boston, Mass.). To sequence the portion of ibeB proximal to the TnphoA insertion site, the initial DNA sequence was obtained from plasmid pCD7A with the 5' primer Tnp5 and the 3' primer Tnp3 (Table 2). The two primers are complementary to the two ends of TnphoA. The remaining DNA sequence of ibeB was determined with primers complementary to the ibeB sequence in pCD7A, pFN7C, and pKS7-7B (Table 1). Both strands of the DNA were resequenced by the automated approach with fluorescence-labeled nucleotides (Applied Biosystems 373A automated sequencer) to ensure accuracy, and the sequence data were analyzed with the DNA analysis program developed by the Genetics Computer Group of the University of Wisconsin. DNA and deduced protein sequences were used to search the DNA and protein databases at the National Center for Biotechnology Information (National Library of Medicine, Washington, D.C.) by use of the BLAST algorithm.
Construction and screening of a genomic library of E. coli RS218.
High-molecular-weight chromosomal DNA was
purified from E. coli K1 strain RS218 as previously
described (7). Genomic DNA was partially digested with
Sau3AI (New England Biolabs), which is compatible with
BamHI. Partially digested genomic DNA (15 to 23 kb) was
partially filled in with dGTP and dATP. This DNA was ligated into
LambdaGEM-12 arms with an XhoI half site. Ligation and
packaging of recombinant lambda phage were performed according to the
manufacturer's instructions (Promega). The E. coli
genomic library was screened by DNA hybridization (7) to
identify phage clones that contained ibeB. A 0.67-kb
ibeB DNA fragment in pCIB7B was released with
EcoRI, purified by preparative agarose electrophoresis and
by use of Geneclean (Bio 101), labeled with
[-32P]dCTP by use of an Oligolabeling kit
(Pharmacia), and used as a probe for screening (>1 × 108 cpm/µg). The phage plaques were replicated onto nylon
filters, UV linked, and hybridized as described previously (7,
9). Plaques hybridizing to the probe were identified by
autoradiography and then purified.
Complementation analysis.
A 7.0-kb
BamHI-EcoRI subclone of pKS7-13K containing the
ibeB ORF (7B) and a 5.7-kb BamHI-HpaI
subclone lacking this sequence (5H) were subcloned into the
pBluescriptII KS vector (see Fig. 2). The resulting constructs were
designated pKS7-7B and pKS7-5H, respectively. A 1.6-kb
XbaI-HindIII subclone of pCR7C carrying the
complete ibeB ORF was subcloned into pFN476. The resulting construct was designated pFN7C. The ligation mixture was used to
transform DH5, and selection was done on LB plates containing ampicillin, isopropyl-
-D-thiogalactopyranoside (IPTG),
and 5-bromo-4-chloro-3-indolyl--D-galactopyranoside (X-Gal). The white colonies were picked for identification of plasmids
containing the insert. Cells of the noninvasive E. coli K1 mutants 7A-33 and IB7D5 were made competent in 10% glycerol as
described previously (7). 7A-33 was transformed with the pBluescriptII KS vector and the recombinant plasmids pKS7-7B and pKS7-5H (Table 1). IB7D5 was transformed with pFN7C and pGP1-2. The
expression of ibeB in pFN476 is driven by the T7 promoter, and pGP1-2 is a vector carrying the T7 RNA polymerase gene
(20). The transformants were tested for their ability to
invade BMEC.
Nucleotide sequence accession number. The nucleotide sequence of ibeB has been deposited in the GenBank nucleotide sequence data library under accession no. AF94824.
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RESULTS |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Noninvasive phenotype of the TnphoA insertion mutant 7A-33. We previously showed that the mutant 7A-33, with a single TnphoA insertion, retained the same phenotypic and genotypic characteristics as the parent strain RS218 or E44 (7). When mutant 7A-33 was examined for its ability to invade bovine and human BMEC, compared to that of the parent strain, its invasion capacity was <0.001%, while the parent strain exhibited an invasion frequency of 0.1%.
Prevalence of meningitis in infant rats.
We next examined
whether the differences in BMEC invasiveness would be biologically
relevant in our well-established infant rat model of experimental
hematogenous meningitis. Table 3
summarizes the prevalence of meningitis (defined as positive CSF
cultures) in 5-day-old rats infected with the parent strain E44 or its
noninvasive mutant with a single TnphoA insertion, 7A-33. As
expected, subcutaneous injections of 1.4 × 104 CFU of
strain E44 or 4.4 × 104 CFU of mutant 7A-33 resulted
in bacteremia of 105 to 108 CFU/ml of blood in
100% of the animals. This level of bacteremia has been shown to be
sufficient to allow circulating E. coli to enter the
CNS (10). As shown in Table 3, the magnitudes of bacteremia
were similar between the two groups. However, the occurrence of
meningitis was significantly lower (P, 0.003) in animals
receiving mutant strain 7A-33 (4 of 25, or 16%) than in those
receiving parent strain E44 (15 of 27, or 56%). These findings support
the concept that the TnphoA insertion mutant 7A-33 is truly
less invasive both in vitro and in vivo, suggesting that the DNA
flanking the transposon insertion in mutant 7A-33 may contain a gene(s)
necessary if not sufficient for invasion of BMEC. It is also
important to recognize that the BMEC invasion frequency of 0.1% is
related to enhanced invasion of the CNS in vivo.
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Sequence analysis of ibeB.
In order to identify the
ibeB gene, we sequenced the corresponding region of
DNA flanking TnphoA. As shown in Fig.
1, a 1,383-nucleotide open reading frame
(ORF) assigned to the ibeB gene coded for a protein
with 460 amino acids and a calculated molecular mass of 50 kDa (Fig. 1). This ORF was found to be 97% identical to a gene encoding a 50-kDa hypothetical protein (p77211) and located in the
13-min region of the E. coli K-12 genome
(1). However, no homology was observed between
ibeB and other known invasion genes when DNA and protein
databases in GenBank were searched. Potential 10 (TATGAG)
and 35 (TTGTCA) promoter regions were found at the
5' noncoding region of ibeB. The TnphoA insertion site was identified by sequencing the fusion joint with the 5' primer
Tnp5 and the 3' primer Tnp3, which are complementary to the two ends of
TnphoA. The insertion occurred in the codon corresponding to
residue 419.
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Construction of an E. coli RS218 LambdaGEM-12 library and isolation and subcloning of invasion determinants. E. coli K1 strain RS218 was used as the source of DNA for cloning experiments. This virulent strain is capable of invading human and bovine BMEC and inducing meningitis in newborn rats (7). To clone the invasion determinants from RS218, a genomic library was constructed in LambdaGEM-12. By use of XhoI half sites in the vector and Sau3AI in the genomic inserts for library construction, self-ligation of vector and genomic sequences was eliminated, since only recombinant phages containing a single insert of the appropriate size (9 to 23 kb) were capable of being packaged. Using ibeB (0.67 kb) as a probe, approximately 5 × 105 recombinant phages were screened and seven phage clones for ibeB were identified. The recombinant phage DNAs were purified and digested with NotI. The sizes of the inserts were between 12 and 16 kb. A 13-kb insert containing ibeB was subcloned into the NotI site of pBluescriptII KS (pKS7-13K).
Construction of an isogenic in-frame deletion mutant. In order to determine whether or not the noninvasive phenotype of the mutant 7A-33 was due to a polar effect of the TnphoA insertion, an ibeB in-frame deletion mutant was generated by integration of the suicide plasmid pCD7D (Table 1). pKS7-6N was constructed by removing the 0.87-kb SmaI-NsiI N-terminal fragment of ibeB from pKS7-7B and religating the plasmid containing part of ibeB with a 30-bp EcoRV-NsiI fragment from plasmid pZerO-2.1 (Invitrogen). A 2.3-kb BglII-EcoRI fragment carrying mutated ibeB from pKS7-6N was converted into blunt ends through a filling-in reaction (18) and subcloned into pCVD442 (4) with SmaI. The resulting construct (pCD7D) was confirmed by PCR and DNA sequencing as having the ibeB in-frame deletion.
The mutants were obtained by mating E44 with SM10pir carrying pCD7D
and selection on LB agar containing ampicillin and rifampin. A single
such colony was picked and grown to the late logarithmic phase in LB
broth without selection. Dilutions were plated on LB agar plates
containing no NaCl and 5% sucrose. Sucrose-resistant colonies were
tested for the loss of ampicillin resistance, indicative of the
loss of vector sequences.
PCR was used to confirm the deletion in the desired chromosomal
ibeB gene in the deletion mutant IB7D5 with a 5' primer
(5'-ATTTCCTCCGCATGTTGC-3') and a 3' primer (IB7-31).
Amplification was carried out with the following cycle profile: 40 cycles at 94°C for 1 min, 55°C for 1 min, and 70°C for 3 min. The
PCR DNA samples were sequenced with primers IB7-31 and IB7-32 to
confirm the ibeB in-frame deletion (Table 2).
Complementation of noninvasive mutants. The mutagenesis experiments (TnphoA insertion and isogenic deletion of ibeB) indicated that ibeB was required for invasion of BMEC by strain E44. As shown in Fig. 3, The TnphoA insertion mutant (7A-33) and the ibeB deletion mutant (IB7D5) were significantly less invasive than E44 in BMEC. To demonstrate that the TnphoA insertion and the ibeB deletion were truly responsible for the noninvasive phenotype, we attempted to complement the noninvasive mutants with pKS7-13K, which contained a 13-kb DNA fragment with ibeB in the pBluescriptII KS vector; pKS7-7B, carrying a 7-kb BamHI-EcoRI DNA fragment with ibeB derived from pKS7-13K; and pFN7C, carrying the ibeB gene (1.6 kb). pKS7-7B was capable of completely restoring the invasive phenotype of the TnphoA noninvasive mutant 7A-33 (Fig. 4A) and the ibeB deletion mutant IB7D5 (Fig. 4B). More importantly, pFN7C was able to fully confer invasive capability to IB7D5 (Fig. 4C). However, pKS7-13K was able to partially complement the mutants (Fig. 4A), suggesting that the expression of ibeB may be reduced because of a larger plasmid with a decreased copy number or some unknown repressor elements present in the larger DNA fragment (18). On the contrary, pKS7-5H, carrying a 5.7-kb BamHI-HpaI DNA fragment with an ibeB deletion derived from pKS7-7B, was unable to complement the TnphoA mutant 7A-33 or the ibeB deletion mutant IB7D5 (Fig. 4A and B).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Although most cases of bacterial meningitis develop as a result of hematogenous spread, how circulating bacteria cross the blood-brain barrier is not completely understood. We have previously shown that several E. coli-BMEC interactions contribute to successful crossing of the blood-brain barrier by E. coli; these include E. coli binding to BMEC via S fimbriae (7, 15, 22). However, S fimbria-mediated binding to BMEC glycoproteins and glycolipids was not accompanied by invasion of BMEC (22), suggesting that binding and invasion are separate phenomena for E. coli translocation from blood to the CNS. We have shown that invasion of BMEC is needed for E. coli to cross the blood-brain barrier in vivo. We have recently described the invasion gene locus ibeA (ibe10) from E. coli K1 strain RS218; this locus has been shown to contribute to invasion of BMEC both in vitro and in vivo (7).
In the process of characterizing the noninvasive mutant 7A-33 derived from E. coli K1 strain RS218, we showed that mutant 7A-33 had a single TnphoA insertion and was considerably less invasive for BMEC (the invasion frequency was 0.001%; that for the parent strain was 0.1%) and significantly less invasive for the CNS in the newborn rat model of experimental hematogenous meningitis (4 of 25, or 16%, for the mutant strain versus 15 of 27, or 56%, for the parent strain; P, 0.003). We have previously shown that a high degree of bacteremia is a primary determinant for meningeal invasion by E. coli K1 (10). The magnitudes of bacteremia between the two groups of animals receiving the parent strain and the mutant strain were similar, indicating that a decreased ability of the mutant to enter the CSF was not an artifact of the lack of a sufficient number of circulating bacteria in the bloodstream. Taken together, these findings suggest that the DNA flanking the transposon insertion in the mutant 7A-33 includes a gene(s) necessary if not sufficient for the invasion of BMEC. This gene, derived from mutant 7A-33, was termed ibeB (invasion of brain endothelial cells).
We have previously shown, using the hematogenous E. coli meningitis model, that the K1 capsule is a critical determinant needed for E. coli to cross the blood-brain barrier as live bacteria (10). We have also shown that OmpA contributes to the invasion of BMEC by E. coli K1 (15). Both the parent strain RS218 and the mutant strain 7A-33 were found to possess the K1 capsule and OmpA. In addition, the EcoRV-MluI TnphoA fragment of the mutant 7A-33 did not hybridize to the probes for the K1 capsule and OmpA. These findings suggest that the noninvasive property of 7A-33 is not likely to be the result of a polar effect of TnphoA on the other known genes involved in invasion (e.g., those for the K1 capsule and OmpA). This concept was also supported by our demonstration that the isogenic ibeB deletion mutant IB7D5 was unable to invade BMEC, and its inability to invade BMEC was fully complemented by the ibeB ORF.
Nucleotide sequence analysis of the ibeB gene showed a single ORF encoding a protein of 460 amino acids and having a predicted molecular mass of 50 kDa (Fig. 1). The deduced protein displayed the characteristics of an outer membrane protein with two transmembrane domains (Fig. 1). This ORF was found to be 97% identical to a gene encoding a 50-kDa hypothetical protein (p77211) and located in the 13-min region of the E. coli K-12 genome. However, no homology was found with genes for any other recognized invasion proteins, suggesting that E. coli K1 ibeB results in a novel phenotype, i.e., E. coli invasion of BMEC. It is not clear whether the ibeB homologue from E. coli K-12 will result in the same phenotype in E. coli K1 strains.
The invasion of BMEC by E. coli represents a unique
mechanism used by bacteria to gain entry into the CNS. We have
previously shown that the characteristics of invasion of endothelial
cells by E. coli K1 are specific to BMEC and that no
such invasion characteristics are observed for endothelial cells of
nonbrain origin, e.g., human umbilical vein endothelial cells
(15). It is of interest that human BMEC have been shown to
form a continuous lining of endothelial cells and to exhibit a
transendothelial electrical resistance of 100 to 600 · cm
(14, 17), a unique property of the BMEC monolayer (compared
to the systemic vascular endothelium). It is important to recognize
that the frequency of invasion of BMEC by the parent strain RS218
(approximately 0.1%) is considerably lower than the reported frequency
of invasion of epithelial cells by other gram-negative bacteria, such
as Shigella and Salmonella species (usually 1 to
10%). However, as shown here and in our previous publication
(7), the BMEC invasion frequency of approximately 0.1%
contributes to enhanced bacterial penetration through the blood-brain
barrier in vivo and thus is biologically relevant.
We have recently shown that the invasion gene locus ibeA contributes to E. coli invasion of human BMEC (7). Here we report another chromosomal invasion locus, ibeB, contributing to E. coli invasion of BMEC. The genetic locus ibeB was capable of completely restoring the ability of the ibeB deletion and TnphoA insertion mutants to invade BMEC. However, E. coli K-12 strain HB101 was not complemented by the ibeB locus (data not shown), suggesting that multiple determinants contribute to E. coli invasion of BMEC. Our demonstration that multiple chromosomal genes are required for E. coli invasion of BMEC is conceptually similar to the reported requirements for different determinants in the attachment and entry of epithelial cells by other meningitis-causing bacteria (2, 13, 25). It remains to be determined how different invasive loci of E. coli contribute to crossing of the blood-brain barrier.
In conclusion, we cloned and characterized the chromosomal gene locus that allows E. coli K1 strain RS218 to invade BMEC both in vitro and in vivo. This gene, termed ibeB, encoded a 50-kDa potential membrane protein. A 7-kb DNA fragment (7B) containing ibeB as well as the ibeB ORF was able to restore the ability of the in-frame ibeB deletion mutant to invade BMEC. Studies are in progress to define the mechanisms by which the ibeB locus exerts its invasive phenotype.
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ACKNOWLEDGMENTS |
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We thank Jin Liu for restriction enzyme mapping of ibeB clones.
This study was supported by a research career development award from Childrens Hospital Los Angeles Research Institute (to S.-H.H.), a grant-in-aid from the American Heart Association Great Los Angeles Affiliate (to S.-H.H.), and USPHS grants R29AI40635 (to S.-H.H.) and R01NS26310 (to K.S.K.).
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FOOTNOTES |
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* Corresponding author. Mailing address: Division of Infectious Diseases, Childrens Hospital Los Angeles, 4650 Sunset Blvd., Mailstop 51, Los Angeles, CA 90027. Phone: (323) 660-2450, ext. 4470. Fax: (323) 660-2661. E-mail: shhuang{at}hsc.usc.edu.
Editor: P. E. Orndorff
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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