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Journal of Bacteriology, December 2001, p. 7224-7230, Vol. 183, No. 24
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.24.7224-7230.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Department of Microbiology, University of Illinois, Urbana, Illinois 61801
Received 1 May 2001/Accepted 4 September 2001
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ABSTRACT |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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An early step in the utilization of starch by Bacteroides thetaiotaomicron is the binding of starch to the bacterial surface. Four starch-associated outer membrane proteins of B. thetaiotaomicron that have no starch-degrading activity have been identified. Two of these, SusC and SusD, have been shown by genetic analysis to be required for starch binding. In this study, we provide the first biochemical evidence that these two proteins interact physically with each other. Both formaldehyde cross-linking and nondenaturing gel electrophoresis experiments showed that SusC and SusD interact to form a complex. Two other proteins encoded by genes in the same operon, SusE and SusF, proved not to be essential for starch utilization and actually decreased starch binding when they were present along with SusC and SusD. Consistent with this, nondenaturing gel analysis revealed that in a strain producing SusC, SusD, and SusE, the SusCD complex was partially destabilized. The strain producing SusC, SusD, and SusE also grew more slowly on starch than a strain producing SusC, SusD, SusE, and SusF (µmax, 0.29 and 0.37/h, respectively). Thus, SusE appears to interact with the SusCD complex. SusE also interacts with SusF, because SusE was less susceptible to proteinase K digestion when SusF was present, and nondenaturing gel analysis detected a complex formed by these two proteins. Our results indicate that SusC, SusD, SusE, and SusF form a protein complex in the outer membrane but that SusE and SusF are dispensable members of this complex.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Undigested polysaccharides are thought to be a major source of carbon and energy for members of the human colonic microflora. In an earlier survey, it was found that the most of the intestinal isolates that could degrade polysaccharides were members of the genus Bacteroides (12). The ability to utilize polysaccharides may explain why Bacteroides is one of the numerically predominant genera in the intestine. We have used the starch utilization system (Sus) of Bacteroides thetaiotaomicron as a model for investigating how Bacteroides species utilize polysaccharides.
Previously, we found that the starch-degrading enzymes of B. thetaiotaomicron are cell associated and that there are outer membrane proteins distinct from the enzymes that bind starch to the bacterial surface (11). Starch binding appears to be the first step in starch utilization. Bound starch is then digested by the degradative enzymes, and products of starch breakdown are internalized (14). This strategy for polymer breakdown helps the bacteria to degrade a large polymer into segments small enough to pass through outer membrane porins without losing the products of digestion to competitors located nearby. Eight genes that contribute to starch utilization have been identified; a regulatory gene, susR, and seven structural genes, susA through susG. Expression of the susA-through-susG genes is regulated by SusR, an activator that responds to the presence of maltose or larger oligosaccharides by increasing expression of the sus structural genes (5). The fact that maltose is an inducer of starch utilization gene expression makes it possible to study sus gene expression even in mutants that are unable to grow on starch.
The biochemical properties of some of the Sus structural proteins have
been determined. SusA is a neopullulanase, a type of starch-degrading
enzyme that can digest all three forms of starch: amylose (linear
chains of 
-1,4-linked glucose residues), amylopectin (amylose chains
linked by -1,6 linkages), and pullulan (maltotriose units linked in
a linear chain by -1,6 linkages). SusA is a soluble enzyme which
appears to be located in the periplasmic space (4). When
susA is disrupted, B. thetaiotaomicron
can still grow on starch, but the growth rate is only 30% that of the
wild type (4). Another starch-degrading enzyme is SusG,
which is also a neopullulanase. SusG is an outer membrane protein and
is essential for growth on starch (14). Disruption of
susG abolishes growth on any form of starch. SusB breaks
down the oligosaccharides released by SusA and SusG into glucose residues.
Much less is known about the biochemical characteristics and functions
of SusC, SusD, SusE, and SusF. Previous work has shown that they are
all outer membrane proteins with no detectable enzyme activity. Genetic
analyses have suggested that they have a role in binding starch to the
bacterial surface (11). Disruption of susC and
susD abolished starch binding completely, and a disruption in susE was associated with reduced starch binding compared
to that for the wild type. A mutant with a disruption in
susF bound starch almost as well as the wild type. These
results suggested that SusC and SusD are responsible for most of the
starch-binding activity detected using intact wild-type cells but that
SusE might make some additional contribution to binding. One hypothesis
to explain these results is that SusC, SusD, SusE, and possibly SusF form a starch-binding complex in the outer membrane. Two findings indirectly supported the hypothesis that SusC and SusD interact. First,
when SusC and SusD were provided individually, their susceptibilities to protease digestion increased. Second, neither SusC nor SusD alone bound to a starch column, but when present together they were
retained on the column (13). This finding could also be explained, however by a different hypothesis
that one of the proteins modified the other to a form that bound starch. In this paper, we provide direct
biochemical evidence for direct physical interactions between SusC and
SusD and for an interaction between SusE and SusF.
The susA gene is in its own transcriptional unit, but susB through susG are arranged in an operon. This operon structure has made it difficult to assess whether the genes in the susB operon are essential for growth on starch, because disruptions in any of the genes upstream of susG have a polar effect on susG, a gene which is essential for starch utilization. In this study, we have determined which of the outer membrane proteins encoded in this region are essential for starch utilization.
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Bacterial strains and growth conditions.
The bacterial
strains and plasmids used in this study are listed in Table
1. All Escherichia coli
strains used in this study were grown in Luria-Bertani (LB) broth or on
LB agar at 37°C. B. thetaiotaomicron 5482, transposon-generated derivatives, and single disrupted mutants used in
this study have been described previously (2, 4, 11).
Cells were grown initially in a prereduced Trypticase-yeast
extract-glucose (TYG) medium. For optimal induction of starch
utilization genes, cells were transferred to a defined medium
(7) containing maltose (0.3%) as the sole carbohydrate
source. To test for growth on malto-oligosaccharides or starch, cells
were inoculated into a defined medium with maltopentaose (G5),
maltoheptaose (G7), amylopectin, or pullulan (0.3%) as a sole
carbohydrate source. Antibiotic concentrations used in this study were
as follows: for ampicillin, 50 µg/ml; for chloramphenicol, 20 µg/ml
(E. coli) or 15 µg/ml (B. thetaiotaomicron);
for erythromycin, 10 µg/ml; for gentamicin, 200 µg/ml; and for
tetracycline, 1 µg/ml.
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DNA methods.
Plasmids were isolated using a Wizard Plus DNA
purification system (Promega Corp). Dephosphorylation reactions and
restriction digestions were performed in accordance with the
manufacturer's instructions (Bethesda Research Laboratories, Bethesda,
Md., or New England Biolabs, Beverly, Mass.). E. coli
DH5MCR was transformed by the method of Lederberg and Cohen
(9). Conjugations, where constructs generated in E. coli were transferred to Bacteroides recipients, were
performed as described by Shoemaker et al. (15). Insertional and replicative shuttle vectors were mobilized from E. coli donors to Bacteroides recipients by the
transfer function of RP4 integrated into the chromosome of S17-1
(17).
Chemicals. 14C-labeled starch (Nicotinia tabacum 1) was purchased from DuPont, NEN. Glucose, maltose, maltopentaose, maltoheptaose, amylopectin, pullulan, proteinase K, and phenylmethylsulfonyl fluoride (PMSF) were purchased from Sigma Corp. Formaldehyde was purchased from J. T. Baker Chemical Co.
Expression of susG in trans.
pSGC23A
(14), a plasmid that carries susG cloned
downstream of the susA promoter, had been used previously to
characterize the activities of SusG independently of the other Sus
proteins. pSGC23A was used to provide SusG in strains with disruptions
in upstream sus genes. The E. coli strain that
contained pSGC23A was mated to BT
susC,
BTsusD, BTsusE, BTsusF,
and BTsusG. The transconjugants were named
BTsusC(pSGC23A), BTsusD(pSGC23A), BTsusE(pSGC23A), BTsusF(pSGC23A), and
BTsusG(pSGC23A), respectively. These strains
were tested for SusG production by Western blotting. The production
of SusC, SusD, SusE, and SusF was also monitored by Western blot
analysis. This was important because a previous study had shown that
providing either the susA promoter or the susB
promoter in trans on a multicopy plasmid (about 5 copies per cell)
caused a decrease in expression of the chromosomal genes, presumably
due to titration of SusR by the cloned promoter regions. The
susA promoter is weaker than the susB promoter
and exerts less of a titration effect when provided on the plasmid.
This is the reason that the susA promoter was used instead
of the susB promoter in the plasmid that provided
susG in trans. These strains were tested for
growth on starch and for starch-binding activity. Western blotting was
done as described previously (10). Approximately 50 µg
of protein in a membrane fraction was loaded in each lane of the gel.
Antibodies bound to the protein were detected with biotinylated
secondary antibodies, followed by treatment with streptavidin
-galactosidase reagent (Bethesda Research Laboratories). Membrane
protein concentrations were determined using the DC protein assay kit
in accordance with the manufacturer's instructions (Bio-Rad Laboratories, Hercules, Calif.).
Starch binding activity. Binding of 14C-labeled starch to intact cells of B. thetaiotaomicron was carried out as described by Shipman et al. (13). Briefly, labeled starch was added to washed intact cells and incubated for 5 min at room temperature. Cells were then harvested by centrifugation and washed twice. Previous work has shown that the starch is bound irreversibly to the cells so that cells can be washed to reduce the nonspecific background. Under aerobic conditions, the cells do not internalize or accumulate starch except for that initially bound (1). Thus, in this assay, binding is uncoupled from uptake into the cytoplasm. B. thetaiotaomicron 4007 was used as the wild-type control because it contains the tetQ gene, which was used as a selectable marker in construction of the insertional disruption mutants. Thus, tetracycline could be added to the media used to grow all strains, including the wild-type control.
Binding values are reported in as micrograms of starch bound per milligram of cell protein. These values were obtained by multiplying the total counts per minute by a dilution factor, which was the ratio of labeled starch to total starch in each assay. That number was converted by an empirical constant based on observed counts per minute per a given amount of starch to disintegrations per minute (dpm), which allowed the total micrograms of starch bound to be calculated by using the reported values of 2.2 × 106 dpm per µg of starch. Experimental values were standardized by assaying the cell protein concentration after sonication.Proteinase K treatment of cells to assess surface exposure of Sus proteins. The surface exposure of Sus proteins was assessed as described by Shipman et al. (14). Briefly, proteinase K was added to washed and resuspended intact cells and incubated with the cells at 37°C for various times. PMSF (final concentration, 1 mM) was added to stop the reaction. Cells were sonicated, and proteins were detected on Western blots with antisera obtained as described previously (14). Antibodies bound to proteins were detected with secondary antibodies conjugated with horseradish peroxidase. To confirm that the cells survived the incubation with proteinase K intact, a protease-sensitive periplasmic marker, SusA, was also detected on Western blots at the initial and final time points. For all the experiments reported here, the concentration of SusA at the end of the incubation period was the same as that at the beginning, indicating that the outer membrane had not been breached.
Formaldehyde cross-linking experiments. Cells were grown on 100 ml of defined medium plus maltose (0.3%) to an optical density at 650 nm of 0.5 and were pelleted by centrifugation at room temperature (22°C). The cell pellet was washed twice with 0.1 M potassium phosphate (KPi) buffer (pH 7.2) and suspended in 1/2 volume of KPi buffer. PMSF (14 µg/ml) was added to protect cells from protease. Formaldehyde was added to a final concentration of 1% (wt/vol). Samples were incubated at room temperature without shaking for 1 h. After the incubation, cells were harvested by centrifugation and washed twice with the KPi buffer, immediately. The pellets were solubilized in 2× concentrated electrophoresis sample buffer (8) and either heated at 65°C for 10 min to maintain the formaldehyde cross-linkings or boiled for 30 min to break the chemical cross-links; boiling for 10 min was not enough to break all the cross-links. Samples obtained from formaldehyde-treated cells or controls (100 µg of protein per lane) were subjected to Western blotting. Antibodies bound to proteins were detected with secondary antibodies conjugated with horseradish peroxidase.
Native gel electrophoresis. Native gel electrophoresis was used to assess interactions among Sus outer membrane proteins. Polyacrylamide gels (6%) without the stacking gel were used to separate native proteins or protein complexes. The Sus outer membrane proteins were solubilized with 1.5% octyl-glucoside, and octyl-glucoside (0.75%) was added to the native gels and the electrophoresis buffer (25 mM Tris, 192 mM glycine) to ensure that the outer membrane proteins remained solubilized when they were electrophoresed. The samples were loaded on a native gel after being mixed with the sample buffer (62.5 mM Tris-HCL, 7.5% Ficoll type 400, 0.001% bromophenol blue [pH 6.8]) without boiling. The gels were electrophoresed in a cold room (4°C) for 8 to 10 h at 15 mA and then subjected to Western blotting. Antibodies bound to proteins were detected with secondary antibodies conjugated with horseradish peroxidase. A large amount of protein (600 µg), compared to that loaded on the sodium dodecyl sulfate (SDS) gels, had to be loaded on these gels to achieve reproducibly detectable bands on the Western blot. This much protein was probably needed because the poorer resolution of a nondenaturing gel makes the bands spread out more, and blotting was less efficient than with the SDS gels.
Denaturing gel electrophoresis. The gel used in the cross-linking experiment was 12% acrylamide with a 5% stacking gel. The gel was 1.5 mm thick. For other experiments involving SDS-polyacrylamide gel electrophoresis (PAGE) 10% acrylamide gels were used. Electrophoresis was done either overnight at 5 mA or for 4 to 7 h at 15 mA. The amount of protein placed in each lane was 50 µg.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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SusG was slightly overexpressed in the
susG-complemented strains.
The susG gene,
which is essential for growth on starch, is also the last gene in the
susB operon. Accordingly, disruption of any gene upstream of
susG makes the cells unable to grow on starch due to a polar
effect of the insertion on susG. For this reason, it was
necessary to express susG in trans in order to determine whether susD, susE, or susF
is essential for starch utilization. To this end, pSGC23A, a plasmid
containing the susG gene, was transferred into various
sus gene disruption strains, including BTsusC,
BTsusD, BTsusE, BTsusF,
and BTsusG. pSGC23A has a copy number of about 5 per cell in Bacteroides. The level of SusG cells
containing pSGC23A was about twofold higher than that in a
wild-type strain with only a single copy of susG, but the
levels of SusG in all of the disruption strains were the same (Fig.
1).
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Only three of the five Sus outer membrane proteins are needed for
starch utilization.
The abilities of the various disruption
mutants to grow on starch (amylopectin and pullulan) were tested. The
wild-type control strain used for comparison was BT4007; it contained
pNLY1::PsusA, the shuttle vector into which
susG was cloned to produce pSGC23A. The strain also
contained a tetracycline resistance gene (tetQ). Thus, the
control strain not only contained multiple copies of the
susA promoter but also contained both antibiotic resistance genes that are present in the disruption mutant strains. The presence of the susA promoter in multiple copies and the need to
select for two antibiotics combine to reduce the rate of growth
on starch by about 10%. All the
susG-complemented strains grew as well as the control
on starch except for BTsusD(pSGC23A). This result indicated that SusD is essential for starch utilization, since BTsusE(pSGC23A), which has only one additional Sus
protein (SusD) compared to BTsusD(pSGC23A), grew well
on starch (Fig. 2). The fact that
BTsusE(pSGC23A) grew on starch as well as the control did shows that only SusC, SusD, and SusG are needed for growth on
starch and that SusE and SusF are dispensable. We designate SusC, SusD,
and SusG the minimal starch utilization system. The growth rate of
BTsusF(pSGC23A) on starch was lower than that of
BTsusE(pSGC23A) or BTsusG(pSGC23A).
BTsusF(pSGC23A) produces SusE but not SusF. This result
suggested that SusE and SusF might be interacting.
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susE(pSGC23A) grew as well as the control or
BTsusG(pSGC23A). Thus, SusE and/or SusF is not
required for malto-oligosaccharide uptake.
BTsusD(pSGC23A) grew on malto-oligosaccharides, but
much more slowly than the other mutants or the wild type.
BTsusD showed the same growth pattern as
BTsusD(pSGC23A), indicating that SusG was not
involved. Therefore, even though SusD is not essential for growth on
malto-oligosaccharides, it affects the uptake of malto-oligosaccharides. This finding supports the hypothesis that SusC
and SusD interact with each other in the outer membrane.
The starch-binding activities of cells containing the minimal
starch utilization system were higher than that of the wild-type
control.
Starch-binding activities of the
susG-complemented strains were compared (Fig.
3). BTsusG(pSGC23A) had
binding activity similar to that of the wild-type control strain,
BT4007(pNLY1::PsusA). BTsusD(pSGC23A), which produces only SusC and SusG,
had no starch-binding activity. Thus, it appeared that SusC and SusG
alone do not bind to starch, and the failure of this strain to grow on
starch is probably due to its inability to bind starch. By contrast,
BTsusE(pSGC23A), which carries the minimal starch
utilization system, had starch-binding activity that was nearly twofold
higher than that of the wild-type control. The growth rate of
BTsusE(pSGC23A) was almost the same as that of the
wild-type control. Thus, the higher starch-binding activity of
BTsusE(pSGC23A) did not affect the growth rate of the
strain.
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SusC in the strain carrying the minimal starch utilization system
exhibited a pattern of proteolytic digestion different from that of
SusC in the wild-type strain.
The proteolytic sensitivities of
SusC, SusD, and SusG in the strain that carried the minimal starch
utilization system was compared to that of these proteins in wild-type
cells (Fig. 4). Since the starch-binding
activity of the strain carrying the minimal system was higher than that
of the wild type, it was possible that the topology of one or more of
the Sus outer membrane proteins, in susE(pSGC23A) was
different from that of the same protein in wild-type cells. SusC in the
wild-type cells appeared to be degraded sooner than SusC in
susE(pXGC23A), although it was also possible that the
proteolytic fragments of SusC were stabilized compared to the wild
type. There was no change in the proteolysis patterns of SusD.
Previously, we had reported that SusD was not exposed on the cell
surface in wild-type cells (13). The absence of SusE and
SusF did not change this result. SusG in the
susG-complemented strain was degraded rapidly, as was SusG
in wild-type cells. The apparent difference between the proteolytic
sensitivities of SusG in the two strain backgrounds is probably not
significant. The higher initial level of SusG in the
susG-complemented strain would be expected to cause a delay
in the complete disappearance of SusG from this strain compared with
the wild type. The fact that SusG in the susG-complemented
strain was entirely degraded shows that all of the SusG produced from
the gene carried on the plasmid was localized to the cell surface.
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The results of formaldehyde cross-linking experiments show that
SusC and SusD interact.
To examine the physical interactions of
the outer membrane proteins of the minimal starch utilization system, a
formaldehyde cross-linking experiment was performed (Fig.
5). The sizes of protein bands were
calculated on the basis of the sizes of standard markers. Strain Ms-2,
which produces no Sus outer membrane proteins, was used as a negative
control. When the strain carrying the minimal system was treated with a
1% formaldehyde solution, three protein bands with molecular sizes
higher than 250 kDa reacted with both anti-SusC and anti-SusD antisera.
These appear to be complexes that contain both SusC and SusD; the band
estimated to be migrating at approximately 270 kDa is the darkest. SusC
is 115 kDa and SusD is 65 kDa, so a simple 1:1 complex of SusC and SusD
would have been expected to be about 180 kDa. Thus, the complex that
migrates at a molecular size above the 250-kDa band may contain 2 copies of SusC. There were two dark bands of about 150 to 160 kDa that reacted only with the anti-SusC antisera. These might have been dimers
of SusC. If so, the complex runs as a smaller unit that the
230-kDa complex predicted from the molecular weight of SusC. We
cannot rule out the possibility that SusC is binding to an as-yet-unidentified protein.
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Native gel electrophoresis confirms the existence of the SusC/SusD
complex.
Native gel electrophoresis was another approach used to
test for interactions between SusC, SusD, and SusG. The gel contained 0.75% octyl-glucoside to keep the outer membrane proteins solubilized. Resolution of protein bands on a native gel is much poorer than on an
SDS gel because of the lack of a stacking gel and the high concentration of protein applied to the gel. Nonetheless, the gel was
able to resolve differences between SusC or SusD alone and the complex
they formed. When both SusC and SusD were present, the anti-SusC and
anti-SusD antisera detected the same band, which migrated differently
than bands corresponding to SusC or SusD alone (Fig.
6). Anti-SusG antiserum did not detect
the band corresponding to the SusC/SusD complex. These findings support
the hypothesis that SusC and SusD interact with each other but provide
no evidence for interaction of SusG with either SusC or SusD.
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Effects of SusE and SusF.
The finding that a strain that
produced SusE but not SusF grew more slowly than the wild type raised
the question of what effect SusE was exerting on SusC, SusD, and SusG.
Also, restoring SusF to the strain restored growth to normal, an
observation that raises the possibility of an interaction between SusE
and SusF. Evidence that SusE without SusF might be destabilizing the
SusC/SusD complex came from native gel analysis of the effect of adding back SusE and SusF to a strain that was producing SusC and SusD (Fig.
7). In the presence of SusE, less SusD
was incorporated into the SusC/SusD complex. Restoration of SusF did
not reverse this apparent destabilization of the SusC/SusD complex.
Comparison of the proteolytic sensitivity of SusE in the absence of
SusF with that of SusE in a strain that was producing SusF revealed that SusE in intact cells was degraded much more rapidly if SusF was
absent than if SusF was present (Fig. 8).
This result supports the hypothesis that SusE and SusF interact with
each other in the outer membrane. Native gel experiments confirmed this
finding (data not shown).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Since the genes encoding the Sus outer membrane proteins are in the same operon, it seemed likely that the proteins they encode would be working together, possibly as part of a complex. The results of experiments reported here provide the first direct support for the hypothesis that SusC and SusD interact to form a complex and that this complex interacts with SusE. Since results of nondenaturing gel electrophoresis indicated that SusE and SusF interact with each other, the finding that SusE interacts with SusC/SusD suggests that all four proteins are present in the complex.
In the studies reported here, not only was SusE found not to be essential for binding, but bacteria lacking it and SusF actually exhibited increased ability to bind starch compared with the wild type. This is consistent with the results of nondenaturing gel experiments, which indicate that SusE destabilizes the SusC/SusD complex. Also, SusE in a strain producing SusC, SusD, SusE, and SusG was more susceptible to proteoloysis than it was in the wild type (Fig. 8), a finding that indicates there is some change in the interaction of SusE with the complex when SusG is present. In a previous study (14), SusE seemed to make a positive contribution to starch binding, because a strain that produced SusC, SusD, and SusE bound starch as well as the wild type, but a strain producing only SusC and SusD bound only about half as much starch. A difference between the previous binding experiments and those reported here is that the strains used in the present study contained multiple copies of susG. Thus, it is possible that the increased starch binding of the strain containing only SusC, SusD, and SusG was due as much to increased concentrations of SusG as to the absence of SusE and SusF. We still do not know the stoichiometry of different members of the complex. Results of cross-linking experiments and nondenaturing gel experiments suggest the possibility that there may be multiple copies of SusC in the complex. Some of the confusion about the role of SusE could be due to the fact that different strains had different relative levels of proteins in the complex.
One would expect SusG to interact with the SusC/SusD complex, but none of our assays detected any direct evidence for such a physical interaction. SusG did not cross-link with SusC or SusD, nor was it part of the complex detected on nondenaturing gels. Although these results are all negative, they raise the possibility that SusG is not interacting closely with SusCDEF. It may be that once a starch molecule is bound to the cell surface, it is so large that SusG only has to be nearby. Starch is very tightly bound to the surface of B. thetaitaomciron even in the absence of SusG, so SusG is not needed to tether the polysaccharide to the cell surface.
The B. thetaiotaomicron starch utilization complex appears to be quite different from the cellulosome complex of cellulolytic clostridia, which is also located on the surface of the bacterium. First, enzymes and cellulose binding proteins in the cellulosome complex are attached to a scaffolding protein (scaffoldin), and it seems that there are no interactions among the enzymes and cellulose binding proteins (3). However, the proteins in the starch utilization system seem to interact with each other. Second, the cellulosome complex is anchored on the cell surface and protrudes from the cell surface by 100 to 500 nm (16). In contrast, the proteins of the Bacteroides starch utilization system are embedded in the outer membrane.
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ACKNOWLEDGMENTS |
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We thank Joseph Shipman for excellent technical advice on the proteolytic sensitivity experiments.
This work was supported by grant AI/GM 17876 from the National Institutes of Health.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Microbiology, 601 S. Goodwin Ave., CLSL 103, University of Illinois, Urbana, IL 61801. Phone: (217) 333-7378. Fax: (217) 244-8485. E-mail: abigails{at}uiuc.edu.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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