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Previous Article | Next Article 
Clinical and Diagnostic Laboratory Immunology, November 2001, p. 1126-1130, Vol. 8, No. 6
1071-412X/01/$04.00+0 DOI: 10.1128/CDLI.8.6.1126-1130.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Mapping of Escherichia coli H27-Specific
Epitope from H-Specific Polypeptides
J. N.
Seah and
J.
Kwang*
Animal Health Biotechnology, Institute of
Molecular Agrobiology, The National University of Singapore,
Singapore 117604
Received 15 March 2001/Returned for modification 25 June
2001/Accepted 17 August 2001
 |
ABSTRACT |
A murine monoclonal antibody (MAb) reactive to H27 flagellin
antigen was produced and characterized. Forty-nine partially purified
native H-type flagellins were used to evaluate the specificity of the
MAb. The fliC gene of H27 is 1,464 bp in length (487 amino acids [aa]; 50.88 kDa). The central variable region (CVR) of the H27
flagellin gene was defined by comparison with flagellin sequences derived from H8, H34, and H49. To study the distribution of antigenic epitopes, the CVR covering amino acid residues 70 to 457 (388 aa) was
dissected into seven overlapping fragments. Fragments carrying the
H-type-specific antigenic determinants were identified by H27-specific
antiserum. Polyclonal antibodies raised against different H-type
flagellin proteins were used to determine the cross-reactive
determinants. Three fragments, spanning amino acid residues 240 to 380, which carried the potential H-specific determinants were used for MAb
production. A MAb specific to H27 was produced, and the specific
epitope was mapped to amino acid residues 330 to 340. In this study, we
produced MAbs from predetermined H27-specific polypeptides and used
whole flagellin in enzyme-linked immunosorbent assays to circumvent the
interference of anti-glutathione S-transferase antibodies.
These factors when combined could help to improve the identification of
the desired MAb.
| |
INTRODUCTION |
The bacterial flagellum is a complex
consisting of a basal body, a hook, and a filament (13).
The flagellar filament is a homopolymer composed of a repeated protein,
flagellin (7), which is Escherichia coli is
encoded by the fliC gene (10). Sequence
analysis of the fliC genes for different serological specificities reveals highly conserved N termini (150 amino acids) and
C termini (100 amino acids) and a central region with considerable variation (10, 16, 17).
The N-terminal and C-terminal conserved regions are essential for the
polymerization and secretion of flagellin molecules (4, 6, 8,
11). On the other hand, the central variable region (CVR)
encodes major determinants contributing to the different E. coli H types (2, 9, 12, 15). Therefore, flagellin carries H-type-specific epitope(s) that are useful for H serogrouping. The agglutination test is routinely used for E. coli H
serotyping. Nevertheless, serological cross-reactions are frequently
observed in agglutination tests due to the presence of cross-reactive
epitopes on the different H-type flagellins. Therefore, identification of H-type-specific epitopes could help to improve E. coli
serotyping. Studies of the characterization of H-specific epitopes by
using monoclonal antibodies (MAbs) (3, 12, 15, 18) and
polyclonal antibodies (17) have been reported. However,
the production and characterization of MAbs to different H-type
flagellins using whole-flagellin immunization are tedious and
time-consuming. Several rounds of screening and confirmation are
required to verify the antigenic specificity of each MAb. In this
study, we modified the protocol with the following advantages: (i) only
polypeptides displaying H specificity were introduced for immunization,
(ii) the complete flagellin sequence was obtained, and
(iii) cross-reactive-polypeptide information was available to
facilitate the production and characterization of the desired MAb. In
this study, we combined molecular cloning and gene expression to
identify the potential H27-specific polypeptides and used the MAb
technique to map the epitope.
| |
MATERIALS AND METHODS |
Bacterial culture, plasmid and PCR amplification, and cloning of
fliC.
H-type E. coli strains purchased from
ECRC (Escherichia coli Reference Center, Pennsylvania State
University, University Park) were grown in Luria-Bertani medium
(Becton Dickinson, Paramus, N.J.). Bacterial genomic DNA was
prepared as previously described (14). Plasmid pGEX-2T
(Amersham Pharmacia Biotech, Uppsala, Sweden) was used for glutathione
S-transferase (GST) fusion protein expression. MacVector
6.0.1 (Oxford Molecular Group, Oxford, United Kingdom) was used
to analyze the DNA and protein sequences. Oligonucleotide primers were
designed based on the published sequence of the E. coli K-12
fliC gene (10). The forward primer, comfla-1
(5'-CCGGATCCATGGCACAAGTCATTA-3'), contained the
first 16 nucleotides of the fliC 5' terminus with a
BamHI restriction site (underlined), and the reverse primer, comfla-2 (5'-CCGAATTCTTAACCCTGCAGTAGAGA-3'),
contained 18 3'-terminal complementary nucleotides of
fliC with an EcoRI restriction site (underlined).
Recombinant truncated CVR of flagellin.
The CVR of H27 was
defined by aligning it with the flagellin amino acid sequences derived
from H8, H34, and H49 using the Mac Vector program. The CVR of H27,
which comprised amino acid residues from 70 to 457 (388 amino acids
[aa]), was dissected into seven truncated fragments by PCR.
Oligonucleotide primers with a BamHI site at the 5' end and
an EcoRI site at the 3' end were designed based on the
sequence of the H27 fliC gene. The relative position of each
truncated fragment was determined (see Fig. 2a). Each fragment was
cloned and expressed as a GST fusion protein.
Preparation of H-specific polyclonal antibodies from guinea
pigs.
Native flagella were purified using semisolid medium and
ultracentrifugation as described previously (3). Partially
purified flagellin was emulsified with the adjuvant MONTANIDE ISA 70 (Seppic, Paris, France) according to the manufacturer's protocol.
Guinea pig anti-H antisera were prepared as described previously
(17). Thirty-six E. coli H-specific antisera
were generated in our laboratory: H1, H2, H3, H4, H5, H6, H7, H8, H9,
H10, H11, H12, H14, H16, H18, H19, H21, H24, H27, H28, H29, H31, H32,
H33, H34, H37, H38, H40, H42, H43, H44, H45, H46, H49, H52, and H54.
Generation of MAb, immunoblotting, and ELISA.
MAbs to the
truncated fragments 3, 6, and 7 of the H27 CVR were prepared as
described previously (1). Sodium dodecyl
sulfate-polyacrylamide gel electrophoresis and immunoblotting
procedures were performed as described previously (17).
Enzyme-linked immunosorbent assays (ELISAs) were performed as described
previously (5). The reading of optical densities (ODs) was
done at 490 nm (OD49).
MAb isotyping by antigen-dependent method.
An isotyping kit,
ImmunoPure monoclonal antibody isotyping kit I (horseradish
peroxidase-2-2'-azinobis [3-ethylbenzothiazoline-6-sulfonic acid]
diammonium salt) (Pierce, Rockford, Ill.) was used to type the
MAbs according to the manufacturer's protocol. Briefly, a microtiter
plate was coated with antigen for 2 h at 37°C, and culture
medium was then added to the wells. After the plate was incubated and
washed, subclass-specific rabbit anti-mouse immunoglobulins were added
to the wells. The reading of optical densities (ODs) was done at
405 nm (OD405).
Nucleotide sequence accession numbers.
All fliC
gene sequences were deposited in GenBank under accession numbers
AF345848 (H27), AF345847 (H8), AF345850 (H34), and AF345851 (H49).
| |
RESULTS |
H27 fliC gene analysis and determination of
CVR.
A single DNA fragment was amplified from H27 genomic DNA. The
PCR fragment was restricted with BamHI and EcoRI
and cloned into the pGEX-2T expression vector for sequence analysis.
The fliC gene of H27 was found to contain 1,464 bp, and the
deduced protein had a relative molecular mass of 50.88 kDa. The CVR of H27, which comprised amino acid residues 70 to 457, was defined by
aligning it with the amino acid sequences of fliC genes
derived from H8, H34, and H49 using the MacVector program (Fig.
1).
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FIG. 1.
Amino acid sequences of fliC genes from H
types H8, H27, H34, and H49. All sequences were aligned using MacVector
to define the CVR of H27. The CVR of H27 was designed to cover residues
70 to 457 (indicated by the arrows). Identical amino acid
residues are boxed and darkly shaded. Gaps inserted to facilitate
alignment are denoted by dashed lines.
|
|
Construction of overlapping fragments and distribution of antigenic
sites on the CVR of H27.
The CVR of H27 was dissected into seven
overlapping fragments by PCR, and each fragment was expressed as a GST
fusion protein. The relative size and position of each fragment is
illustrated in Fig. 2a. These fragments
were useful in understanding the distribution of antigenic sites in the
H27 CVR. When all the truncated fragments were incubated with anti-H27
flagellin antiserum in immunoblotting, the antigenic sites of H27 were
primarily found in fragments 1 (aa 70 to 150), 3 (aa 270 to 350), 4 (aa
370 to 457), 5 (aa 140 to 180), 6 (aa 240 to 280), and 7 (aa 340 to
380) (Fig. 2b).
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FIG. 2.
Truncation of H27 CVR. These fragments were used to
study the distribution of H27-specific and cross-reactive determinants.
See Results for details. (a) The 388-aa variable region (amino acid
residues 70 to 457) of fliC from H27 was dissected into
seven overlapping fragments (F1 to F7). (b) Recombinant peptides
reacted with anti-H27 antiserum, showing the distribution of
immunogenic sites. (c) Thirty-six antisera were pooled to identify the
cross-reactive determinants in the CVR of H27. An arrow denotes each
truncated flagellin.
|
|
Determination of the distribution of cross-reactive determinants by
using different H-type antisera.
The CVR of flagellin has been
shown to carry both H-type-specific and cross-reactive epitopes.
Cross-reactive epitopes can be identified by using different
H-type-specific antisera. Truncated H27 CVR fragments were resolved by
sodium dodecyl sulfate-polyacrylamide gel electrophoresis and
transferred nitrocellulose membranes for immunoblotting. Thirty-six
antisera raised against different H-type flagellins, excluding anti-H27
flagellin antiserum, were pooled and incubated with all of the
truncated H27 CVR fragments. As shown in Fig. 2c, fragment 1 (aa 70 to
150), fragment 4 (aa 370 to 457), and fragment 5 (aa 140 to 180) were
positive, suggesting that these fragments carried cross-reactive
determinants. Therefore fragments 3, 6, and 7, carrying H27-specific
epitopes, were used for MAb production.
Production of MAb.
Fragments 3, 6, and 7 from the H27 CVR,
comprising residues 240 to 380 and showing specificity for H27
flagellin, were used for MAb production. A hybridoma clone, H27S1,
showing a positive reaction to partially purified native H27 flagellin,
was recovered. This MAb was identified as the immunoglobulin G1 subtype.
Antigenic specificity of MAb.
The antigenic specificity of the
MAb H27S1 was confirmed by testing it against different H-type
flagellins in ELISA. A panel of 49 partially purified H-type flagellins
was used in this study. Each antigen was individually adsorbed onto
microtiter wells in triplicate to verify the specificity of the MAb.
MAb H27S1 showed a strong reaction to purified H27 flagellin but showed
no reaction to other H-type flagellin proteins and had weakly positive
reactions to H2, H4, H5, H6, and H38 (Table
1). These H-type flagellins later tested
negative to H27S1 in immunoblotting.
Mapping of H27S1 epitope.
Fragments 3, 6, and 7, comprising
residues 240 to 380 of the H27 CVR, were initially used for MAb
production. Therefore, the fragment containing the putative epitope
which the MAb derived from was not immediately clear. The preliminary
ELISA data showed that the MAb specifically reacted with fragment
F3, indicating the location of the epitope (data not shown).
With the specificity confirmed, fragment F3 (80 aa) was further
dissected into three overlapping fragments, F3-1 (aa 270 to 300), F3-2
(aa 320 to 350), and F3-3 (aa 295 to 325), respectively (Fig.
3a). When incubated with the MAb, only
fragment F3-2 (aa 320 to 350) was reactive, suggesting that fragment
F3-2 carried the putative epitope of H27S1 (Fig. 3a). The minimal
sequence of the H27-specific epitope was defined by serially truncating
fragment F3-2 (aa 320 to 350) from both termini (Fig. 3b). Three
overlapping constructs varying in length, sF3-1 (aa 325 to 340; 16 residues), sF3-2 (aa 330 to 345; 16 residues), and sF3-3 (aa 330 to 340; 11 residues), were constructed. Interestingly, the MAb reacted
indiscriminately with these fragments in an immunoblotting assay,
suggesting that all three fragments shared a common sequence which was
essential to form an immunogenic epitope. Therefore, the H-type epitope
of H27 was found in residues 330 to 340.
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FIG. 3.
Epitope mapping of MAb H27S1. (a) The 80-aa fragment F3
was dissected into three overlapping fragments, F3-1, F3-2, and F3-3;
only fragment F3-2 (residues 320 to 350) reacted with the MAb. (b)
Fragment F3-2 was dissected into three overlapping fragments, sF3-1
(residues 325 to 340), sF3-2 (residues 330 to 345), and sF3-3 (residues
330 to 340). All of the fragments were positive, and the core sequence
of the epitope comprised residues 330 to 340.
|
|
| |
DISCUSSION |
An agglutination test based on the somatic (O), capsule
(K), and flagellin (H) antigens is conventionally used to identify E. coli serotypes. However, the presence of common epitopes
in these antigens has resulted in some H-type E. coli
isolates not being readily discriminated. In this study, we report a
method to map the H27-specific epitope combining molecular cloning,
gene expression, MAbs, and polyclonal antibodies. The distribution of
both specific and cross-reactive determinants could be readily determined by antisera to different H-type flagellins. In the process
of MAb production, only those polypeptides displaying H27 specificity
with few antigenic determinants (compared to whole-flagellin or
whole-bacteria immunization) were used for MAb production. In the
subsequent screening stages, purified H27 flagellin was used in ELISA
to enhance the screening efficiency. In conventional H epitope mapping,
whole flagellin is used for both MAb production and ELISA screening.
Therefore, the lack of flagellin sequence information, the dominance of
cross-reactive epitopes, and the undefined potential H-specific
polypeptides hinder epitope identification.
We used the H type H27 as an example to illustrate the mapping strategy
to identify the H27-specific epitope. The CVR of H27 was first defined
by aligning it with three sequences (H8, H34, and H49) (unpublished
results). Sequence alignment revealed that two regions in the H27
flagellin near the N and C termini carried several nonidentical amino
acids: region 1, comprising residues 100 to 150 (equivalent to fragment
1 in Fig. 2a), and region 2, comprising residues 540 to 614 (equivalent
to fragment 4 in Fig. 2a) (Fig. 1). The functional roles of these
nonidentical amino acid residues in sequence conservation and
cross-reactive-epitope formation were not clear. Therefore, the H27 CVR
was designed to include regions 1 and 2 (comprising residues 70 to
457). There was a slight difference in the conservation of residues
according to the published result (16). However,
both region 1 (fragment 1) and region 2 (fragment 4) showed strong
reactions with non-H27 antisera in an immunoblotting assay (Fig. 2c),
suggesting that regions 1 and 2 could be either carrying cross-reactive
determinants or sharing conserved sequence with other H-type flagellins.
A hybridoma clone, H27S1, reactive to purified H27 flagellin in both
ELISA and immunoblotting, was produced by immunizing BALB/c mice with
H27-specific polypeptides. The specificity of the MAb was confirmed by
reacting it with a panel of 49 partially purified flagellins. Most of
the flagellins gave readings equivalent to that of the negative control
except H types H2, H4, H5, H6, and H38 (Table 1). Flagellin extracted
from H types H2, H4, H5, H6, and H38 were weakly reactive in an ELISA
screen, which was later proven to be nonspecific interaction in an
immunoblotting assay (data not shown). In order to determine the
smallest fragment sequence encoding the H27-specific epitope,
three overlapping polypeptides with the core sequence KAATASDLDLN,
comprising residues 330 to 340, were constructed. All of the
polypeptides, sF3-1, sF3-2, and sF3-3, reacted indiscriminately with
the MAb (Fig. 3b). Therefore, the H27-specific epitope was mapped to
amino acid residues 330 to 340. The epitope sequence was submitted to
GenBank for comparison. A candidate flagellin gene, STEC-O26:H11
(19), which has one amino acid different from the H27
epitope at residue 334, was identified from GenBank. An alanine (A) at
residue 334 of the H27 flagellin was replaced by a leucine (L) at the
same position in the H11 flagellin. However, ELISA and immunoblotting repeatedly showed that there was no cross-reaction between these two H
types and ruled out the possibility that the identified region could be
an immunodominant region in other serotypes, such as H type H11.
We also tried to predict the putative H-specific epitope by comparing
flagellin amino acid sequences derived from several H-type E. coli strains. However, no significant conclusion was made
based on the sequence alignment. In addition, no consensus sequence was
defined due to the highly variable CVR. Moreover, it has been shown
that a single-amino-acid change in the CVR is sufficient to determine a
single serotype in E. coli (12). The role of
the primary sequence of flagellin in determining the specificity and
cross-reaction of H-antigen is clear, but more flagellin sequences are
needed in order to identify the H-specific epitope through sequence analysis.
| |
ACKNOWLEDGMENTS |
This work was supported by the National Science and
Technology Board (NSTB), Singapore.
We acknowledge Y. K. Lee for his helpful suggestions. We thank Liu
Wei and Yap Lee Hua for their help with the production of guinea pig
antisera. The MONTANIDE ISA adjuvant was kindly provided by Seppic,
Paris, France.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Animal Health
Biotechnology, Institute of Molecular Agrobiology, 1 Research Link, The National University of Singapore, Singapore, 117604. Phone: 65-8727473. Fax: 65-8727007. E-mail: Kwang{at}ima.org.sg.
| |
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Clinical and Diagnostic Laboratory Immunology, November 2001, p. 1126-1130, Vol. 8, No. 6
1071-412X/01/$04.00+0 DOI: 10.1128/CDLI.8.6.1126-1130.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
