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Infection and Immunity, September 2001, p. 5921-5924, Vol. 69, No. 9
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.9.5921-5924.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Demonstration of Polysaccharide Capsule in Campylobacter
jejuni Using Electron Microscopy
Andrey V.
Karlyshev,
Maria V.
McCrossan, and
Brendan
W.
Wren*
Department of Infectious and Tropical Diseases, London
School of Hygiene and Tropical Medicine, University of London,
London WC1E 7HT, United Kingdom
Received 8 February 2001/Returned for modification 10 April
2001/Accepted 30 May 2001
 |
ABSTRACT |
Recently, we reported that Campylobacter jejuni, an
important gastrointestinal pathogen, has the genetic determinants
to produce a capsular polysaccharide (Karlyshev et al., Mol. Microbiol.
35:529-541, 2000). Despite these data, the presence of a
capsule in these bacteria has remained controversial. In this study we
stain C. jejuni cells with the cationic dye Alcian
blue and demonstrate for the first time by electron microscopy that
C. jejuni cells produce a polysaccharide capsule that is
retained in the coccoid form but is absent in a kpsM mutant.
| |
TEXT |
Campylobacter jejuni is
currently a major cause of bacterial gastrointestinal disease in humans
in many countries (13). Despite deciphering the genomic
sequence of one isolate, NCTC 11168 (12), many questions
relating to the biochemistry, physiology, and pathogenicity of the
microorganism remain unanswered (20). Capsules frequently
play key roles in the survival of bacteria and in immune evasion of
several bacterial pathogens (16). Recently, it has been
suggested that the high-molecular-weight fractions of C. jejuni lipopolysaccharide may be capsular polysaccharide (CPS)
(3). Using the NCTC 11168 genome sequence data, we
reported the genetic and biochemical characterization of these
molecules and found that they are related to group II and III CPS found in other pathogenic bacteria (8). Despite detection of CPS in C. jejuni, to date there have been no reports on the
direct visualization of capsules in this species. In this study, using electron microscopy (EM), we demonstrate for the first time that this
important pathogen does produce a polysaccharide capsule surrounding
the surface of the cell. Capsule detection was facilitated by our
recent discovery that CPS of C. jejuni has a strong affinity to Alcian blue dye (9).
Bacterial polysaccharide capsules are usually heavily hydrated polymers
loosely attached to the bacterial cell surface (16). Because of their fragile nature, they may be lost during sample preparation for EM. A number of different approaches to stabilize capsules for EM visualization have been used, including treatment with
antibodies, different dyes, and chemical cross-linking
(2). Alcian blue has been used for staining capsules in
several bacterial species, including Klebsiella pneumoniae
(2), Neisseria gonorrhoeae (6,
14), Bordetella bronchiseptica (10),
Pasteurella multocida (5), and
Haemophilus pleuropneumoniae (7). Both
whole bacteria (10) and thin sections (2, 5, 6, 7,
14) were used successfully. To avoid disturbing fragile
capsular material, bacteria are often fixed and stained directly on
agar plates, followed by thin-section analyses (7, 14).
Ruthenium red dye has also been used for staining bacterial CPS, for
example, in Vibrio parahaemolyticus (4, 5).
Alcian blue may stabilize the capsule, since treatment of cells only
during the initial fixation step but not at subsequent stages
facilitated capsule detection (10). Although Alcian blue is known to have a high affinity for acidic polysaccharides
(1), the mechanism by which the dye binds is unclear.
Bacterial strains G1 (isolate from a patient with Guillain-Barré
syndrome), X (gastrointestinal isolate) (8), and
NCTC 11168 were grown at 37°C on agar plates (Columbia agar; Oxoid, Basingstoke, United Kingdom) containing growth and selective
supplements (Oxoid) in a microaerobic atmosphere for 2 days. Agar
pieces containing bacteria were cut, fixed, and treated with Alcian
blue (17) or ruthenium red (11).
Fixation and processing steps were performed within a fume cupboard at
room temperature in vials on a rotary mixer. Agar pieces with bacteria
were put into fixative containing 1% Alcian blue 8GX (or 0.1%
ruthenium red) and 3% glutaraldehyde prepared in 0.075 M sodium
cacodylate buffer (pH 7.4) and incubated for 2.5 h. The samples
were then washed with four changes of 0.2 M sucrose in 0.075 M sodium
cacodylate buffer for 1.5 h and left for a further 1.5 h in
1% osmium tetroxide. The samples were incubated in buffered 0.2 M
sucrose solution overnight in a refrigerator at 4°C, washed in
ultrapure MilliQ water, and dehydrated through a graded series of 30 to
100% ethanol for 10 min per step, transferred sequentially into 3:1,
1:1, and 1:3 ethanol-TAAB resin (TAAB Laboratories, Reading,
United Kingdom) mixtures for 1 h per step, and finally into 100%
TAAB resin overnight. The samples were incubated in fresh 100% TAAB
resin for 3 h, embedded in silicone flat molds, and placed into a
60°C oven to polymerize for 2 days. The blocks were removed from the
molds and trimmed and 100-nm ultrathin sections were cut using a glass
knife and a Leica Ultracut R ultramicrotome, (Leica Microsystems,
Milton Keynes, England). The sections were floated onto MilliQ water
and then placed onto copper grids coated with a thin Pioloform support
film. The grid-mounted sections were then stained with 2% alcoholic
uranyl acetate for 10 min in the dark, thoroughly washed in MilliQ
water, then stained for a further 10 min on a drop of Reynolds' lead
citrate (15) in a CO2-free
atmosphere, washed in MilliQ water, and allowed to air dry before
examination and photography on a Jeol 1200EX transmission electron
microscope at 80 kV (Jeol Ltd, Welwyn Garden City, England). Micrographs were taken on Agfa Scienta EM film, and the resulting images were printed on Agfa multicontrast resin-coated paper using an
Agfa Rapidoprint processor and Agfa chemistry.
Ruthenium red dye was unable to stain C. jejuni cells (Fig.
1). By contrast, clearly defined capsules
were detected after cells on agar blocks were fixed in the presence of
Alcian blue (Fig. 2A and 2B). The capsule
was presented as a thick amorphous structure covering bacterial cells.
The thickness of the capsule usually varied between 70 and 100 nm,
whereas the diameter of cross-cut cells was in the range of 200 to 250 nm. Some capsules were extended by a distinct massive fibrous layer (F)
containing a characteristic bright internal area (Fig. 2C). As F
structures have been reported during Alcian blue EM visualization of
capsules in other microorganisms (2, 5), we investigated
their nature. Surprisingly, such F structures could also be observed
after treatment of blank agar blocks with Alcian blue. We suggest that
F structures visible in EM are aggregates of Alcian blue dye. Such
aggregates, which can often be observed on EM photographs between the
cells, stick to encapsulated cells (Fig. 2C) and can easily be
differentiated from amorphous capsule layer with irregular structure
(Fig. 2A and B).
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FIG. 2.
EM at different magnifications (A and B) of cells of
strain G1 treated with Alcian blue. Capsulated cells with fibrilla-like
structures are also shown (C). CA, capsule; F, fibrillae.
|
|
To investigate whether the capsule in the G1 strain consists of CPS,
Alcian blue staining and EM were performed on defined insertional G1
mutants. One of the mutations, pldA, does not affect CPS
production (9), and this mutant was used as a positive control. By contrast, the kpsM mutation was found to abolish
production of CPS molecules (8). A capsule was seen in the
pldA mutant, but it was somewhat thinner than the capsule
observed in the wild-type strain (Fig.
3A). The reason for this difference
remains unclear, although one cannot exclude that capsule formation can
be modulated by the outer membrane phospholipase product of the
pldA gene. As expected, no capsule was detected in the
kpsM mutant by Alcian blue staining (Fig. 3B), confirming
that the structure detectable in wild-type G1 cells is CPS.
The results presented in Fig. 1 to 3 were from a 2-day-old culture. It
is known that C. jejuni cells are prone to undergo transformation from a spiral to a coccoid morphology after prolonged incubation on a growth medium (19). We investigated
whether this transformation has any effect on capsule staining.
Four-day agar cultures of strain G1 were analyzed in EM after staining with either ruthenium red or Alcian blue dye. Most cells after 4 days
of growth had become oval, with an average size of about 900 nm, i.e.,
about three times the cross-section of the spiral forms (Fig.
4A and B). As with 2-day-old cultures, no
capsule could be detected with ruthenium red (Fig. 4A). A dark internal area presumably consisting of a nucleoid could be observed in the older
culture. Interestingly, in contrast to 2-day-old cultures, the space
between the nucleoid and cell wall is nonstainable. This probably
indicates dramatic reduction in biochemical (transcriptional) activity
in the coccoid cells. Similar observations were noticed when the same
culture was treated with Alcian blue. A difference in this case,
however, was the presence of a capsule (Fig. 4B).
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FIG. 4.
Cells of 4-day agar culture of strain G1 after treatment
with ruthenium red (A) and Alcian blue (B).
|
|
As in strain G1, a capsule was detected in wild-type strain X but not
in the X kpsM::kan mutant (data
not shown). The use of kpsM mutants in both cases was
essential in eliminating the possibility of false-positive results due
to a potential of Alcian blue to form aggregates and interact with
other molecules on the cell surface (14).
We also attempted to detect a capsule in the sequenced strain NCTC
11168 (12). A gene cluster related to CPS production is
present in this strain (8). However, attempts to detect capsule in this strain have not been successful despite the observation that CPS of this strain is stainable with Alcian blue (9). One possibility is that the CPS of NCTC 11168 has lower affinity for
Alcian blue and staining conditions on a gel (acid pH) are different
from those used for staining-fixation for EM. This correlated with the
lower intensity of CPS in the NCTC 11168 strain compared to that of
strain G1 (Fig. 5). It is possible that
despite CPS production in NCTC 11168, the mechanism of capsule
formation in this strain is impaired or specific environmental signals
are required for capsule formation. Reversible loss of capsule has been
reported in some bacteria (4). As the kpsM gene
is present in all nine C. jejuni strains tested (data not
shown) and this gene is involved in both CPS biosynthesis and capsule
formation in strain G1, we suggest that the majority of C. jejuni strains make or have the potential to make a polysaccharide
capsule.
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FIG. 5.
Alcian blue staining of heat extracts of different
C. jejuni strains and their mutants after
electrophoresis in an acrylamide gel as described (9).
Lanes: 1, G1; 2, NCTC 11168; 3, 11168H (hypermotile clonal isolate of
NCTC 11168); 4, G1 pldA::kan;
5, G1 kpsM::kan; 6, X
kpsM::kan; 7, NCTC 11168 kpsM::kan; 8, prestained
protein markers (New England BioLabs). The arrows indicate locations of
CPSs of G1 and NCTC 11168 strains.
|
|
Through a combination of Alcian blue staining and EM, we have shown for
the first time visualization of a C. jejuni capsule. This
finding has confirmed the prediction from sequence analysis that
C. jejuni cells may produce CPS and paves the way for the full genetic, biochemical, and structural analysis of this subcellular organelle. We have also demonstrated that despite apparent significant structural and biochemical changes, the coccoid form of C. jejuni retains the capsule. By similarity to the polysaccharide
capsules of other microorganisms, C. jejuni capsules may be
involved in enhancing survival of the microorganism in the environment
by affording resistance to desiccation and increased adherence to various surfaces via biofilm formation, as well as in colonization and
resistance to nonspecific and specific host immunity (reviewed in
reference 16).
C. jejuni remains a major conundrum in microbiology. One
paradox is how a microorganism that is difficult to culture and that has reduced viability when cultivated in vitro is able to survive in
the environment to be the most frequently isolated bacterial food-borne
pathogen (13, 18). The polysaccharide capsule described in
this study might be an important new factor essential for the survival
and pathogenicity of C. jejuni. Its discovery should facilitate future investigations on the survival, transmission, and
pathogenesis of this problematic food-borne pathogen and may assist in
the development of improved intervention strategies to reduce the
burden of C. jejuni infection.
| |
ACKNOWLEDGMENTS |
This work was supported by the BBSRC and the Wellcome
Trust, United Kingdom.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Infectious and Tropical Diseases, London School of Hygiene and Tropical Medicine, University of London, Keppel Street, London WC1E 7HT, United
Kingdom. Phone:: 44 (0) 207 927 2288. E-mail:
brendan.wren{at}lshtm.ac.uk.
Editor:
V. J. DiRita
| |
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Infection and Immunity, September 2001, p. 5921-5924, Vol. 69, No. 9
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.9.5921-5924.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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