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Infection and Immunity, July 2000, p. 4092-4101, Vol. 68, No. 7
Department of Microbiology, University of
Texas Southwestern Medical Center, Dallas, Texas
75390-9048,1 and Department of Cellular
Biochemistry, Institute of Haemotology and Blood Transfusion,
Prague, Czech Republic2
Received 14 January 2000/Returned for modification 14 February
2000/Accepted 23 March 2000
Haemophilus influenzae can utilize different
protein-bound forms of heme for growth in vitro. A previous study (I. Maciver, J. L. Latimer, H. H. Liem, U. Muller-Eberhard, Z. Hrkal, and E. J. Hansen. Infect. Immun. 64:3703-3712, 1996)
indicated that nontypeable H. influenzae (NTHI) strain
TN106 expressed a protein that bound hemoglobin-haptoglobin and was
encoded by an open reading frame (ORF) that contained a CCAA nucleotide
repeat. Southern blot analysis revealed that several NTHI strains
contained between three and five chromosomal DNA fragments that bound
an oligonucleotide probe for CCAA repeats. Three ORFs containing CCAA
repeats were identified in NTHI strain N182; two of these ORFs were
arranged in tandem. The use of translational fusions involving these
three ORFs and the All Haemophilus
influenzae strains have an absolute requirement for heme for
aerobic growth because they are unable to convert When H. influenzae is grown in vitro, free heme satisfies
the porphyrin requirements (13) and, in part, the iron
requirements (8) of this organism. For growth in vivo,
however, H. influenzae faces a major impediment to heme
acquisition. Free heme is toxic, and the human body possesses highly
specific mechanisms for the complexing of this tetrapyrrole molecule
(18). The abundant serum proteins albumin and hemopexin bind
heme avidly, with Kd values of 10 A previous study from our laboratory identified a 115-kDa outer
membrane protein (HhuA), expressed by nontypeable H. influenzae (NTHI) strain TN106, that was involved in the binding
and utilization of hemoglobin-haptoglobin (23). The HhuA
protein exhibited features typical of a TonB-dependent outer membrane
receptor, having significant homology with other TonB-dependent
proteins over the regions characteristic of these proteins
(22). Elimination of expression of the hhuA gene
product decreased but did not eliminate the ability of this NTHI strain
to utilize hemoglobin-haptoglobin for aerobic growth, a finding which
suggested the existence of an alternative mechanism or pathway for
utilization of this heme-protein complex.
A striking feature of the hhuA gene is the presence of a
four-nucleotide (CCAA) repeat motif near the start of this open reading frame (ORF). Inspection of the H. influenzae Rd genome
(11) revealed that several other predicted ORFs shared this
feature and encoded predicted proteins that were likely to be TonB
dependent. The presence of these additional ORFs containing the CCAA
repeat raised the possibility that there might exist a family of
hemoglobin- or hemoglobin-haptoglobin-binding outer membrane proteins
in H. influenzae. Moreover, expression of the encoded
proteins might be affected by the recombination-independent slippage
mechanism (i.e., slipped-strand mispairing) known to mediate the phase
variation of surface antigens encoded by genes with homopolymeric or
heteropolymeric nucleotide repeats. The latter include the PII protein
of Neisseria gonorrhoeae (27), the enzymes that
synthesize the lipooligosaccharide of H. influenzae
(43), and hemoglobin-binding outer membrane proteins of both
N. gonorrhoeae (3) and N. meningitidis
(19, 34).
In the present study, we identified three genes in NTHI strain N182
that contain CCAA repeats and encode proteins very similar to HhuA. We
used translational fusions to prove that these proteins can bind
hemoglobin or hemoglobin-haptoglobin. Monoclonal antibodies (MAbs) were
used to detect phase variation in the expression of these NTHI proteins.
Bacterial strains and growth conditions.
Wild-type NTHI
strain N182 and nine additional NTHI strains have been described
previously (5). All NTHI isolates were cultured routinely in
brain heart infusion broth (Difco Laboratories, Detroit, Mich.) with
NAD (10 µg/ml; Sigma Chemical Co., St. Louis, Mo.) (BHI) and
hemin chloride (50 µg/ml; Sigma) (BHI-Hm). Isolates were also grown
in BHI containing NAD and human hemoglobin (100 µg/ml; Sigma)
(BHI-Hg). Addition of
ethylenediamine-di(o-hydroxyphenylacetic acid) (EDDA; Sigma)
to a final concentration of 100 µM in broth media was used for iron
chelation. All broth cultures were grown at 37°C with aeration;
agar-solidified media were incubated at 37°C in an atmosphere of
95% air-5% CO2. Escherichia coli strain DH5 Recombinant DNA methods.
Standard recombinant DNA methods,
including restriction enzyme digestions, alkaline phosphatase
reactions, ligation reactions, agarose gel electrophoresis, and plasmid
purification, were performed as previously described (36) or
in accordance with the manufacturer's instructions. Restriction
enzymes were purchased from New England Biolabs (Beverly, Mass.).
Shrimp alkaline phosphatase was purchased from USB (Cleveland, Ohio).
T4 DNA ligase was purchased from GIBCO-BRL (Bethesda, Md.). Plasmid DNA
was prepared with the Wizard Plus Miniprep DNA Purification
System (Promega, Madison, Wis.) and the Qiagen Plasmid Midi Kit (Qiagen
Inc., Valencia, Calif.). Chromosomal DNA was isolated by the method of
Marmur (24).
Southern blot analysis.
NTHI chromosomal DNA was digested to
completion with a variety of restriction enzymes and probed by Southern
blot analysis with an oligonucleotide probe that consisted of five
consecutive repeats of the tetranucleotide CCAA. This 20-mer was
labeled by using the chemiluminescence-based Renaissance
Oligonucleotide 3' End-Labeling Kit (NEN, Boston, Mass.) as described
by the manufacturer.
PCR.
PCR was performed with either the GeneAmp XL PCR Kit
(Perkin-Elmer Corp., Foster City, Calif.) or the Taq DNA
Polymerase Kit (Promega). To amplify products from N182 genomic DNA, 1 µg of chromosomal DNA and 100 ng of each primer were used in a
100-µl reaction mixture. PCR products used for nucleotide sequence
analysis were purified by agarose gel electrophoresis, followed by the use of the Wizard PCR DNA Purification System (Promega) in accordance with the manufacturer's directions. PCR products used for the construction of translational fusions were first digested with PstI and then subjected to gel purification as described
above. The compositions of the oligonucleotide primers used to generate various PCR products are listed in Table
1.
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Detection of Phase Variation in Expression of
Proteins Involved in Hemoglobin and Hemoglobin-Haptoglobin Binding
by Nontypeable Haemophilus influenzae
ABSTRACT
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
-lactamase gene from pBR322 revealed that these
three ORFs, designated hgbA, hgbB, and
hgbC, encoded proteins that could bind hemoglobin,
hemoglobin-haptoglobin, or both compounds. Monoclonal antibodies (MAbs)
specific for the HgbA, HgbB, and HgbC proteins were produced by
immunizing mice with synthetic peptides unique to each protein. Both
HgbA and HgbB were readily detected by Western blot analysis in N182
cells grown in the presence of hemoglobin as the sole source of heme,
whereas expression of HgbC was found to be much less abundant than that
of HgbA and HgbB. The use of these MAbs in a colony blot
radioimmunoassay analysis revealed that expression of both HgbA and
HgbB was subject to phase variation. PCR and nucleotide sequence
analysis were used in conjunction with Western blot analyses to
demonstrate that this phase variation involved the CCAA repeats in the
hgbA and hgbB ORFs.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-aminolevulinic
acid to protoporphyrin IX, the immediate biosynthetic precursor of heme
(13, 45). Analysis of the H. influenzae Rd genome
(11) revealed the genetic basis for this growth requirement in that many of the genes encoding the relevant enzymes are missing in
H. influenzae (42). Therefore, H. influenzae has evolved or acquired mechanisms for the binding and
transport of exogenously supplied heme because aerobic growth and
acquisition of heme by H. influenzae are absolutely
codependent (10).
8
and 1013 M, respectively (17, 38). Under
normal physiologic conditions, all circulating heme will be complexed
to hemopexin because this glycoprotein has a much greater affinity for
heme than does albumin (17). In addition, much of the
body's heme is present in the form of hemoglobin. While free
hemoglobin can be utilized readily by H. influenzae growing
in vitro (40), the small amount of circulating free
hemoglobin (i.e., that not present in erythrocytes) is tightly
complexed (Kd, ~1023 M) by the
serum protein haptoglobin (2).
MATERIALS AND METHODS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
and recombinants derived from it were grown at 37 or 30°C on
Luria-Bertani medium (36) supplemented with ampicillin (100 µg/ml) or tetracycline (15 µg/ml), as required.
TABLE 1.
Primers used to generate PCR products with N182
chromosomal DNA
Recombinant plasmid construction.
Plasmids p712-2, p661-1,
and p661-8 were constructed by ligating DNA fragments, derived from the
use of the GeneAmp XL PCR kit, into the TA Cloning Kit vector pCRII
(Invitrogen, San Diego, Calif.). The 1.4-kb insert in p712-2 was
generated from N182 chromosomal DNA by using the oligonucleotide
primers P1 and P2. The two different 1.4-kb inserts in p661-1 and
p661-8 were generated with primers P3 and P4. Translational fusions
involving -lactamase were generated by inserting PCR-derived partial
ORFs of the hgbA, hgbB, and hgbC genes
into the PstI site within the bla gene in pBR322.
The 3,225-nucleotide (nt) insert in pHgbA-FP was obtained by PCR with
the primers P5 and P6. Similarly, the 3,147-nt insert in pHgbB-FP and
the 3,058-nt insert in pHgbC-FP were obtained by using primers P7-P8
and P9-P10, respectively.
Colony blot hybridization.
N182 chromosomal DNA that had
been partially digested with Sau3AI was ligated into
pBluescript II SK+ (Stratagene, La Jolla, Calif.) and used to transform
E. coli DH5. Total DNA from each transformant colony was
hybridized with either the 1.4-kb insert from either p712-2 or p661-1
as previously described (36). The DNA probes were labeled by
using [-32P]dCTP and the Random Primed DNA
Labeling Kit (Boehringer Mannheim, Indianapolis, Ind.) in accordance
with the manufacturer's instructions. Two transformants were found to
react with the p712-2-derived DNA probe, and 10 transformants were
identified that bound with the p661-1-derived DNA probe.
Nucleotide sequence analysis. Both strands of three overlapping PCR products generated from N182 chromosomal DNA with primers P11 and P12 (3.9 kb), primers P13 and P14 (3.4 kb), and primers P15 and P16 (4.1 kb) were sequenced in their entirety using a model 373A Automated DNA Sequencer (Applied Biosystems, Foster City, Calif.). These overlapping PCR products encompassed the complete sequence of the tandem hgbA and hgbB genes. The nucleotide sequence of the hgbC gene was derived from the 3.9-kb PCR product generated with primers P17 and P18. In each instance, at least three independent PCRs were performed to obtain the DNA segments which were then pooled for sequence analysis. PCR products used to determine the numbers of CCAA repeats in the various hgb genes were generated by using the oligonucleotide primers P19 and P20 for the hgbA gene, P15 and P21 for the hgbB gene, and P17 and P22 for the hgbC gene. Nucleotide sequence data were analyzed by using the MacVector analysis package (version 6.5; Oxford Molecular Group, Campbell, Calif.).
MAbs. Spleens from mice individually immunized with three different keyhole limpet hemocyanin-conjugated synthetic peptides, derived from the HgbA, HgbB, and HgbC proteins, were fused with SP2/0-Ag14 plasmacytoma cells as previously described (35). These peptides included KEINNTTTPNSNSNKDKTYDFSKL from HgbA, KDSFNSQWTSMVERKEKQYTDITDIK from HgbB, and KFARIKDRKDKNNRDNRKIK from HgbC. The resultant lymphocyte hybridomas were screened in an enzyme-linked immunosorbent assay using an ovalbumin-conjugated form of the immunizing peptide as the antigen. Antibodies reactive in the enzyme-linked immunosorbent assay were then screened by Western blotting using a lysate of heme- and iron-starved NTHI N182 cells as the antigen. This approach resulted in the production of HgbA-specific MAb 17H3, HgbB-specific MAb 4B3, and HgbC-reactive MAb 12A2. All three of these MAbs were shown to readily bind their respective antigens (expressed as fusion proteins) by Western blot analysis. It should be noted that HgbC-reactive MAb 12A2 bound a doublet in a Western blot analysis of NTHI whole-cell lysates. The upper band of this doublet was HgbC; the identity of the lower band is not known. MAb 6B8 was used to detect the iron-regulated H. influenzae HitA protein (37).
SDS-PAGE, Western blotting, and colony blot RIA. Whole-cell lysates of NTHI (29) were subjected to SDS-PAGE, followed by Coomassie blue staining or Western blot analysis as previously described (6). NTHI N182 colonies were examined for reactivity with HgbA-specific MAb 17H3 and HgbB-specific MAb 4B3 in the colony blot radioimmunoassay (RIA) (14). With MAb 17H3, this assay was performed as previously described (14). With MAb 4B3, the colonies were first lifted onto a nitrocellulose membrane filter (Schleicher & Schuell, Keene, N.H.), which was then laid atop a filter pad (Gel Blot Paper; Schleicher & Schuell), presoaked with 62.5 mM Tris-HCl (pH 6.8) containing 10% (wt/vol) SDS. The nitrocellulose was left on this filter pad for 10 min at room temperature prior to incubation with the blocking agent. HgbC-reactive MAb 12A2 did not function in colony blot RIA analysis.
Detection of hemoglobin- and hemoglobin-haptoglobin-binding activities. NTHI strain N182 was screened for the ability to bind radioiodinated hemoglobin and hemoglobin-haptoglobin as previously described (23). (It must be noted that both the hemoglobin and haptoglobin in the hemoglobin-haptoglobin were radioiodinated.) To detect binding activity in the HgbA-FP, HgbB-FP, and HgbC-FP fusion proteins, total cell membranes were prepared from each recombinant E. coli strain using the Peripreps Periplasting Kit (Epicentre Technologies Corp., Madison, Wis.) and equal amounts of each fusion protein in membranes (as determined by SDS-PAGE and Coomassie blue staining) were loaded onto nitrocellulose membranes using a dot blot apparatus (Schleicher & Schuell) and tested for hemoglobin- and hemoglobin-haptoglobin-binding activities.
Detection of expression of Hgb proteins. NTHI N182 cells were grown in BHI-Hm broth to mid-exponential phase, at which point the cells were serially diluted and plated onto both BHI-Hm and BHI-Hg agar plates. Approximately 900 of the resultant heme-grown colonies were tested for reactivity with HgbA-specific MAb 17H3 using the colony blot RIA; another 900 heme-grown colonies were tested for the ability to bind HgbB-specific MAb 4B3. Two sets of approximately 300 colonies each grown on BHI-Hg agar were tested for reactivity with these two MAbs. In a second experiment, N182 cells were grown to mid-exponential phase in both BHI-Hm and BHI-Hg broth and the resultant cells were serially diluted and plated onto agar plates of the homologous medium. Approximately 300 colonies from each set of plates were tested for reactivity with the two MAbs described above. From these plates, five MAb-reactive colonies and five non-MAb-reactive colonies were selected and streaked for the isolation of single colonies on the same medium. Each of the 40 isolates was then passaged two more times on the same medium. The final isolates were grown in the homologous broth medium for Western blot analysis.
Nucleotide sequence accession numbers. The nucleotide sequences of the NTHI N182 hgbA, hgbB and hgbC genes were deposited in the GenBank database and assigned accession numbers AF221059 (for hgbA and hgbB) and AF221060 (for hgbC).
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Determination of the number of NTHI genes bearing CCAA repeats. We previously identified a gene (hhuA) in NTHI strain TN106 that contained a CCAA tetranucleotide repeat motif and encoded an outer membrane protein involved in the binding of hemoglobin-haptoglobin (23). However, an isogenic hhuA mutant was shown to still utilize both hemoglobin-haptoglobin and hemoglobin (23). Examination of the genome of H. influenzae strain Rd (11) revealed that it possessed four possible ORFs which encoded proteins homologous to HhuA and which also contained CCAA repeat motifs. We decided to investigate whether NTHI strains also possessed multiple genes with CCAA tetranucleotide repeats in their genomes.
Chromosomal DNAs from 10 NTHI strains were digested with EcoRI and probed by Southern blot analysis with an oligonucleotide comprised of five consecutive repeats of CCAA. Each strain had at least three EcoRI fragments that bound this probe (Fig. 1A). Strain N182 (Fig. 1A, lane 1), which appeared to possess only three hybridizing bands, was chosen for further study. When N182 chromosomal DNA was digested to completion with 10 different restriction enzymes and probed with this same oligonucleotide, at most three different fragments in any single digest bound the CCAA probe (Fig. 1B).
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Identification of CCAA repeat-containing genes. Oligonucleotide primers that flanked each of the four CCAA repeat-containing ORFs (HI661, HI635, HI712, and HI1566) found in the H. influenzae Rd genome (11) were used in a PCR with NTHI N182 chromosomal DNA, but no products were obtained. Four additional pairs of primers internal to these ORFs were designed, and two of these (P1 and P2 from the HI712 ORF and P3 and P4 from the HI661 ORF; Table 1) yielded 1.4-kb PCR products when used with N182 chromosomal DNA. These PCR products were cloned into the pCRII vector for nucleotide sequence analysis. The 1.4-kb fragment derived from the HI712-based primers contained a partial ORF that encoded a protein that was 82% identical to the predicted protein product of the H. influenzae Rd HI712 ORF. A single recombinant clone (p712-2) was chosen for further analysis. Sequence analysis of two recombinant clones (p661-1 and p661-8) generated from the HI661 internal primers showed two different incomplete ORFs that encoded protein products that were 84 and 40% identical, respectively, to the predicted protein product of the HI661 ORF in H. influenzae Rd and 39% identical to each other.
The remaining nucleotide sequences flanking these three partial ORFs were obtained by screening an N182 genomic library, constructed in E. coli as described in Materials and Methods, with the cloned partial ORFs described above. Compilation of nucleotide sequences derived from the various hybridization-positive recombinant clones revealed that the two complete ORFs containing the nucleotide sequences from the p661-8 and p712-2 DNA inserts were located in tandem in the N182 chromosome; these were designated (based on the fusion protein-based experiments discussed below) hemoglobin-binding proteins A (hgbA) and B (hgbB), respectively (Fig. 2). The complete ORF containing the nucleotide sequence from the p661-1 insert was not linked to these other two ORFs and was designated hgbC (Fig. 2). Immediately upstream from the hgbB ORF were tandem copies of 23-nt elements arranged as inverted repeats; these 23-nt elements were previously described as being associated with DNA duplications in the chromosome of H. influenzae (30). Immediately upstream from the hgbC ORF, there were at least four copies of this same 23-nt element (Fig. 2).
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Characteristics of the hgbA, hgbB, and
hgbC genes and their encoded products.
The
hgbA ORF contained 3,039 nt, and the encoded protein
consisted of 1,009 amino acids (aa) with a calculated molecular weight of 115,811. The end of the hgbA ORF was separated from the
beginning of the hgbB ORF by 855 nt. The 3,201-nt
hgbB ORF encoded a predicted protein of 1,067 aa with a
calculated molecular weight of 122,462. The hgbC ORF
contained 2,979 nt, and its predicted protein had 993 aa and a
calculated molecular weight of 113,608. All three ORFs possessed
apparent transcriptional terminators located 14 to 27 nt 3' from the
translational stop codons and also putative consensus 
35 and 10
promoter sequences located 34 to 41 nt upstream from the translation
initiation codons. A dyad repeat sequence with weak homology to the
Fur-binding consensus sequence (21) was located upstream
from the translation initiation codons in both hgbA and
hgbB; a similar dyad repeat sequence was not apparent upstream from the hgbC ORF (data not shown). Consecutive
CCAA tetranucleotide repeats were found near the beginnings of all three ORFs, with the hgbA ORF containing 25 repeats, the
hgbB ORF containing 19 repeats, and the hgbC ORF
containing 9 repeats. (The possible number of CCAA repeats in each ORF
varied [e.g., 23, 24, and 25 repeats in hgbA], as
determined by nucleotide sequence analyses of PCR products derived
independently from N182 chromosomal DNA
the selected numbers listed
above for the hgbA, hgbB, and hgbC
ORFs would allow full-length expression of each encoded protein as
discussed below.)
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Binding of hemoglobin and hemoglobin-haptoglobin by fusion
proteins.
The ability of the HgbA, HgbB, and HgbC proteins to bind
hemoglobin or hemoglobin-haptoglobin was examined in an E. coli background. Attempts to clone the intact NTHI N182
hgbA, hgbB, and hgbC genes into
E. coli were unsuccessful, so slightly truncated versions of
these three ORFs were fused to the -lactamase gene in pBR322 to
produce translational fusions (Fig. 4).
Each ORF was truncated at the 5' end to a point just beyond the end of
the CCAA repeat region. Each of the resultant fusion proteins (HgbA-FP,
HgbB-FP, or HgbC-FP) was shown to bind its homologous MAb by Western
blot analysis (Fig. 5A to C, lane 1).
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(pBR322) was used as a negative control
and did not bind either of the radiolabeled compounds (Fig. 6A and B,
row 1). HgbA-FP bound the labeled hemoglobin (Fig. 6A, row 2) but did
not appear to bind the labeled hemoglobin-haptoglobin (Fig. 6B, row 2).
HgbB-FP bound hemoglobin (Fig. 6A, row 3), but to a lesser degree
than did HgbA-FP. However, HgbB-FP was capable of
binding hemoglobin-haptoglobin (Fig. 6B, row 3), albeit
weakly. HgbC-FP bound hemoglobin (Fig. 6A, row 4) but did not
detectably bind hemoglobin-haptoglobin (Fig. 6B, row 4).
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Effects of heme and iron limitation on expression of the HgbA,
HgbB, and HgbC proteins.
NTHI N182 was grown in a basal medium
(BHI containing NAD) with high levels of heme (50 µg/ml), moderate
levels of hemoglobin (100 µg/ml), or no added heme source. (H. influenzae can grow aerobically for four to five generations in
the absence of exogenous hemethese latter conditions were used to
induce heme starvation). N182 was also grown under these same
conditions in the presence of the iron chelator EDDA. Western blot
analysis revealed that when N182 was starved for both heme and iron,
both HgbA (Fig. 5A, lane 9) and HgbB (Fig. 5B, lane 9) were readily
detectable whereas HgbC was not apparent (Fig. 5C, lane 9). Long-term
exposure of the autoradiogram revealed that HgbC was expressed (Fig.
5C, lane 8), albeit at relatively low levels.
Expression of HgbA, HgbB, and HgbC by NTHI N182 cells grown with heme or hemoglobin. The presence of the CCAA repeats in the hgbA, hgbB, and hgbC genes raised the possibilities that expression of these ORFs was regulated by the number of repeats and that phase variation of the encoded proteins could occur (27, 43). In a preliminary effort to ascertain whether HgbA and HgbB were consistently expressed by NTHI N182 cells, we first grew this strain in BHI-Hm broth and then plated these cells onto both BHI-Hm and BHI-Hg agar plates. The resultant individual colonies were evaluated for the ability to bind MAbs specific for the HgbA or HgbB protein in a colony blot RIA. (HgbC-reactive MAb 12A2 was not used in these experiments because it did not function in the colony blot RIA.) It was found that 96% of the colonies from the BHI-Hm agar plates bound the HgbA-specific MAb, while only 11% of the colonies reacted with the HgbB-specific MAb. Among the colonies that developed on the BHI-Hg plates, 98 and 8% bound the HgbA- and HgbB-specific MAbs, respectively. These results indicated that N182 cells, whether grown with heme or with hemoglobin, did not uniformly express HgbA and HgbB. (It should be noted that this experiment did not address the frequency of potential phase variation.)
To determine whether individual N182 isolates expressed all three proteins simultaneously, this NTHI strain was grown in BHI-Hm and in BHI-Hg broth, plated onto the homologous medium solidified with agar, and probed with the HgbA- and HgbB-specific MAbs. Five colonies that bound each MAb and five colonies that failed to bind each MAb were passaged by the single-colony isolation method three times on the homologous medium. The resultant 20 heme-grown and 20 hemoglobin-grown isolates were subjected to Western blot analysis to determine whether each isolate expressed the other two Hgb proteins. Heme-grown isolates originally identified in the colony blot RIA as reactive or unreactive with the HgbA MAb remained the same after serial passage on BHI-Hm agar (Fig. 7A, lanes 1 to 5 and 6 to 10, respectively). Similarly, isolates that bound the HgbB MAb or failed to bind this MAb in the colony blot RIA maintained these antigenic characteristics after in vitro passage (Fig. 7B, lanes 11 to 15 and 16 to 20, respectively). The 10 heme-grown isolates selected for their MAb reactivity (Fig. 7A, lanes 1 to 5, and B, lanes 11 to 15) expressed only the homologous Hgb protein (i.e., HgbA or HgbB); the other 10 MAb-unreactive isolates (Fig. 7, lanes 6 to 10 and 16 to 20) did not express detectable levels of any Hgb protein. No detectable HgbC protein was expressed by any of the 20 heme-grown isolates (Fig. 7C, lanes 1 to 10 and lanes 11 to 20).
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Effect of CCAA repeats on protein expression. To determine whether the number of CCAA repeats in the hgbA, hgbB, and hgbC ORFs was involved in control of expression of the Hgb proteins, the region containing these repeats was amplified by PCR from several of the isolates included in Fig. 7 and 8. Two isolates from each group of five (e.g., 1 to 5, 6 to 10, 11 to 15, and 16 to 20 in Fig. 7) were randomly chosen for this analysis. Each heme-grown isolate positive for HgbA expression (4 and 5 in Fig. 7) contained 25 CCAA repeats in its hgbA ORF; this number of repeats would theoretically allow full-length expression of the encoded protein. The HgbA MAb-unreactive isolates grown on heme (9 to 12, 16, and 17 in Fig. 7) had 23, 26, or 27 repeats in their hgbA ORFs; all of these would result in premature translational termination codons in the ORF. The heme-grown HgbB-positive isolates (11 and 12 in Fig. 7) contained 19 repeats in their hgbB ORFs, consistent with the predicted expression of the entire encoded protein. The companion HgbB-negative isolates (4, 5, 9, 10, 16, and 17 in Fig. 7) possessed 20 or 21 CCAA repeats in their hgbB ORFs; these would cause premature translational termination.
All of the hemoglobin-grown isolates (21, 22, 26, 27, 31, 32, 36, and 37 in Fig. 8) contained 22 or 25 CCAA repeats in their hgbA ORFs; both of these numbers of repeats would allow full-length protein expression. The two hemoglobin-grown isolates that expressed the HgbB protein (31 and 32 in Fig. 7) possessed 19 and 22 repeats in their hgbB ORFs, consistent with the potential for full-length protein expression. The hemoglobin-grown HgbB-negative isolates (21, 22, 26, 27, 36, and 37 in Fig. 8) had either 20 or 21 repeats in their hgbB ORFs; either of these would cause premature translational termination. The HgbC protein was not expressed by any of the eight heme-grown or eight hemoglobin-grown isolates subjected to PCR and nucleotide sequence analysis; the presence of either 10 or 11 CCAA repeats in all of the hgbC ORFs examined in these 16 isolates would result in premature termination of translation. These results indicated that protein expression, as detected by MAb reactivity, could be correlated with predicted protein expression as determined by the number of CCAA repeats present in the different ORFs.| |
DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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It is now apparent that H. influenzae strains have numerous mechanisms for the binding and uptake of heme, whether the heme is free or bound to a protein carrier (12, 15, 23, 31, 40). Considering the absolute dependence of H. influenzae on heme for aerobic growth, such redundancy in heme uptake systems is perhaps not surprising. Moreover, there are now data which indicate that some of the genes encoding these heme uptake systems are transcribed in the human body during the infectious process, at least in otitis media (44).
The present study extends our earlier finding that an NTHI outer membrane protein encoded by an ORF containing a CCAA repeat motif was involved in the binding and utilization of hemoglobin-haptoglobin (23). In NTHI strain N182, there appears to be a family of related proteins which can bind hemoglobin or hemoglobin-haptoglobin and which have in common the presence of a CCAA repeat in their respective ORFs. Work by Stull and colleagues (26) that was reported while the present study was in progress indicates that H. influenzae type b strain HI689 possesses three ORFs (i.e., hgpA, hgpB, and hgpC) that contain CCAA repeats and encode hemoglobin- or hemoglobin-haptoglobin-binding proteins, a finding which raises the possibility that this type of protein family is common to both NTHI and H. influenzae type b strains. The presence of CCAA repeats in the other NTHI strains described in the present study, as well as in other H. influenzae strains described independently by Morton and Stull (25), indicates that these genes are ubiquitous among H. influenzae strains.
Using the HgbA- and HgbB-specific MAbs in the colony blot RIA, we were able to detect the expression of these proteins individually and then use PCR to determine the number of CCAA repeats present in the relevant ORF. These data indicate that expression of HgbA or HgbB by a given isolate could be directly correlated with the presence of an appropriate number of CCAA repeats in the selected ORF (i.e., that which would be predicted to allow full-length protein expression). We were also able to use PCR to amplify the CCAA repeat-containing regions from the other two, unselected hgb ORFs in each isolate. In every case, when an isolate did not express a protein reactive with a given MAb, the number of CCAA repeats in that particular ORF was consistent with premature translational termination. These data, based on detection of protein expression with MAbs, are complemented by those of Ren et al. (33), who used a CCAA-containing gene from H. influenzae type b in a lacZ-based translational gene fusion to correlate phase-variable expression of LacZ with alterations in the number of CCAA repeats.
We were able to readily detect individual N182 isolates that expressed either HgbA or HgbB or both simultaneously (Fig. 7 and 8). In contrast, we did not detect any individual N182 isolates (Fig. 7 and 8) that readily expressed HgbC even though we could detect some HgbC expression in a population of N182 cells that had been starved for both heme and iron (Fig. 5C, lane 8). Again, nucleotide sequence analysis of the 5' end of the hgbC ORF in the 16 individual isolates that did not express HgbC indicated that, in every case, the number of CCAA repeats in the hgbC ORF would have resulted in premature termination of translation. The fact that HgbC-reactive MAb 12A2 did not function in a colony blot RIA analysis precluded direct identification of individual N182 isolates that expressed HgbC.
Slipped-strand mispairing resulting in phase-variable expression of an outer membrane protein was first reported by Cannon and colleagues with the PII (Opa) protein of N. gonorrhoeae, where a pentanucleotide repeat was present near the beginning of the ORF encoding this protein (27). Subsequently, the occurrence of slipped-strand mispairing has been described for several ORFs that encode proteins involved in the uptake of hemoglobin in both N. gonorrhoeae (3) and N. meningitidis (19, 34). Polyguanine tracts within the ORFs encoding the HpuA protein of N. gonorrhoeae (3) and the HpuA and HmbR proteins of N. meningitidis (19, 34) have been shown to be involved in phase variation that is controlled by slipped-strand mispairing.
The frequency of phase variation in the gonococcal hemoglobin
utilization system described above has been reported to be
approximately 103 (4), whereas different
serotypes of meningococci exhibited phase variation in hemoglobin
utilization at frequencies as high as 102 and as low as
106 (19, 34). We observed that when a
heme-grown isolate of N182 (Fig. 7, lane 7) that did not express HgbA,
HgbB, or HgbC was grown in BHI-Hm medium and then plated on BHI-Hm
plates, colonies that bound either the HgbA-specific MAb or the
HgbB-specific MAb arose at a frequency of 102 to
103 (data not shown).
While a number of different genes encoding proteins involved in heme acquisition have now been described in H. influenzae, the hgbA, hgbB, and hgbC genes in NTHI N182 and the very similar hgpA, hgpB, and hgpC genes in H. influenzae type b strain HI689 represent the first descriptions of genes that may have been derived from duplication events. The likelihood of this possibility is reinforced by our detection of large inverted repeats, proposed to be associated with gene duplications (30), immediately upstream from both the hgbB and hgbC ORFs in NTHI N182. Why other H. influenzae genes involved in heme acquisition (e.g., hxuCBA) (6) have not been duplicated in the H. influenzae chromosome is not known. It is possible that this redundancy in genes that express hemoglobin- or hemoglobin-haptoglobin-binding proteins reflects a greater functional significance of these particular protein-bound sources of heme to H. influenzae. We also cannot formally exclude the possibility that the presence of these related genes in NTHI strain N182 is the result of horizontal genetic exchange, especially in view of the fact that multiple strains of NTHI can coexist simultaneously in the human respiratory tract (28).
Our data on the expression of HgbA, HgbB, and HgbC by individual N182 isolates (Fig. 8, lanes 21 to 40) indicate that repeated passage of these cells with hemoglobin as the sole source of heme resulted in expression of HgbA by all of the individual isolates regardless of whether the original isolate (as identified by colony blot RIA) expressed this protein. This finding is likely the result of the selection of a population of HgbA-expressing cells. Whether HgbA functions more or less effectively than HgbB and HgbC in the binding and utilization of hemoglobin by strain N182 remains to be determined. A recent report by Stull and colleagues (26) indicates that a hgpA hgpB hgpC mutant of H. influenzae type b HI689 is still able to utilize hemoglobin as its sole source of heme for growth. This finding indicates that, at least in H. influenzae type b HI689, a protein encoded by a gene that does not contain CCAA repeats will function to allow this H. influenzae strain to acquire heme from hemoglobin. The identity of this gene product and its possible existence in NTHI strains remain to be determined.
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ACKNOWLEDGMENTS |
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This study was supported by U.S. Public Health Service grant AI17621 to E.J.H.
We thank Jo Latimer, Sheryl Lumbley, Sharon Thomas, and Yufan Zhu for technical assistance. We also thank Kathryn Edwards, Janet Gilsdorf, Timothy Murphy, and Peter Rice for providing many of the NTHI isolates used in this study.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Microbiology, Hamon Biomedical Research Building, NA6.200, University of Texas Southwestern Medical Center, 6000 Harry Hines Blvd., Dallas, TX 75390-9048. Phone: (214) 648-5974. Fax: (214) 648-5905. E-mail: hansen01{at}utsw.swmed.edu.
Editor: E. I. Tuomanen
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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