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Journal of Bacteriology, November 2001, p. 6444-6453, Vol. 183, No. 21
Biology Department, Massachusetts Institute
of Technology, Cambridge, Massachusetts 02139
Received 22 May 2001/Accepted 10 August 2001
Sinorhizobium meliloti strains lacking BacA function
are impaired in symbiosis with alfalfa host plants and display altered sensitivities to a number of compounds relative to wild-type strains. With the goal of finding clues to the currently unknown biological function(s) of BacA, we carried out a genetic analysis to determine which amino acids are critical for protein function and to attempt to
ascertain whether the multiple phenotypes that result from a
bacA-null allele were the result of a common
cause or whether BacA has multiple functions. We have created a set of
20 site-directed mutants in which selected individual amino acids in
bacA were replaced with glycine residues. The resulting
mutants were characterized to determine how the various amino acid
changes affected a number of phenotypes associated with loss of BacA
function. Mutants H165G, W182G, D198G, and R284G had null phenotypes
for all functions assayed, while mutants W57G, S83G, S231G, and K350G
were indistinguishable from wild-type strains. The remaining 12 site-directed mutants demonstrate mixed phenotypic characteristics and
fall into a number of distinctly different groups. These observations
may be consistent with a role for BacA in multiple, nonoverlapping functions.
The bacterial protein BacA is a
putative transporter of unknown function that is unusually interesting
because it is absolutely required for both the virulence of an animal
pathogen (18) and the symbiotic capacity of an
agriculturally beneficial plant endosymbiont (9). As part
of our efforts to elucidate the biological role of this intriguing
protein, we have initiated a genetic dissection of BacA in the
gram-negative bacterial endosymbiont of alfalfa, Sinorhizobium
meliloti, because of its genetic tractability and the ease with
which one can monitor its ability to establish a persistent infection
with its eukaryotic host.
Nitrogen fixation is the end result of a complex symbiotic relationship
between rhizobia and leguminous plants (23, 26), in which
the bacterial partner is harbored within plant root nodules and
exchanges reduced atmospheric nitrogen, necessary for host plant
growth, for photosynthetically derived carbon compounds. bacA, a key gene involved in nodule development in the
S. meliloti-alfalfa symbiosis, was isolated in a screen that
identified bacterial mutants with symbiotic deficiencies
(21). Rhizobia invade the nodules they elicit on legumes
via specialized plant-derived structures called "infection
threads." Upon release from infection threads into plant
membrane-bound compartments, wild-type rhizobia begin differentiating
into nitrogen-fixing bacteroids. Electron microscopy has shown that
S. meliloti mutants that lack bacA function
invade nodules and are released properly from infection threads, but then appear to lyse and die at this intermediate developmental time
point before they can differentiate and establish a functional symbiosis (9).
bacA mutants from Brucella abortus, an animal
pathogen and close phylogenetic relative of S. meliloti
(5), are similarly unable to persist in host tissues in
experimentally infected mice and are unable to replicate and survive in
vitro in murine macrophages (18). In the BALB/c mouse
infection model, wild-type brucellae replicate to high levels in the
liver and spleen during the first 2 weeks postinfection
(24). After this time point, brucellae are hypothesized to
switch from this acute phase of infection to a chronic one, in which
tissue colonization decreases slightly and then plateaus, and brucellae
undergo large changes in gene regulation and protein expression
(19, 27-29). B. abortus bacA-null mutants
behave like wild-type bacteria during the initial stages of host
infection, but begin to be cleared by host mice beginning at around 2 weeks postinfection. Thus, bacA-deficient mutants of
S. meliloti and B. abortus each have parallel
survival patterns in their respective host organisms: both are able to
invade and survive within their host environments at early
developmental time points, but are unable to persist in their
respective hosts during the chronic phase of infection, where they
would each normally carry out long-term infections.
As originally suggested by Southern blots (9), a number of
bacteria encode proteins that are related to the S. meliloti and B. abortus bacA gene products. The most closely related
are the SbmA proteins of Escherichia coli (16)
and Salmonella enterica serovar Typhimurium (A. Ichige and
K. LeVier, unpublished data). When aligned pairwise, these four
proteins show a high degree of similarity (79 to 97%), despite the
substantial divergence of the The molecular functions of the S. meliloti and B. abortus BacA proteins are not known, yet the proteins are of great
interest, since they are critically important for these bacteria to
establish their chronic intracellular relationships with their
respective eukaryotic hosts. The presence of BacA-related proteins in a
variety of bacteria, some of which are not known to enter into
long-term associations with eukaryotic cells (e.g., Alcaligenes
eutrophus and Synechocystis sp.) suggests that
functions related to that of BacA must confer an important advantage in
a variety of environmental conditions. The observation that E. coli sbmA mutants are resistant to bleomycin (32),
microcin B17 (16), and microcin J25 (30) led
to the suggestion that the SbmA protein is the transporter that brings
these antibiotics into the cells. We have previously shown that the
E. coli SbmA protein is functionally interchangeable with
R. meliloti BacA (15) and had postulated
that the symbiotic role of BacA might involve the transportation of
some compound from the eukaryotic cytoplasm into the bacterial cell.
However, our more recent characterizations of additional phenotypes of
the S. meliloti bacA mutant, including resistance to certain
aminoglycoside antibiotics and increased sensitivity to ethanol and
detergents, have led us to conclude that loss of BacA function affects
the integrity of the bacterial cell envelope (15; G. P. Ferguson, K. LeVier, R. M. Roop, and G. C. Walker, unpublished data). In this paper, we describe a site-directed mutagenesis study of the S. meliloti bacA gene, which we
carried out not only to identify critical amino acids of BacA, but also to investigate whether the various effects of bacA result
from one underlying molecular function or from multiple genetically separable functions.
Strains and media.
The bacterial strains and plasmids used
in this study are described in Table 1.
S. meliloti strains were grown in liquid LB/MC
(Luria-Bertani broth supplemented with 2.5 mM
MgSO4 and 2.5 mM
CaCl2) or on LB or LB/MC plates at 30°C
unless otherwise stated. E. coli strains were grown in LB at
37°C. When required, antibiotics were added at the following
concentrations: ampicillin, 100 µg/ml; spectinomycin, 100 µg/ml;
streptomycin, 500 µg/ml; tetracycline, 10 µg/ml.
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.21.6444-6453.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Genetic Analysis of the Sinorhizobium
meliloti BacA Protein: Differential Effects of Mutations
on Phenotypes
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-Proteobacteria (S. meliloti and B. abortus) from the 
-Proteobacteria (E. coli and S. enterica serovar Typhimurium). The four proteins are approximately
the same size (ca. 400 amino acids), and all are predicted to span the
cytoplasmic membrane seven times (2). In the past 3 years,
Basic Local Alignment Search Tool (BLAST) (1) searches of
the sequence databases have shown that there is a second class of
proteins related to BacA or SbmA (which will be referred to as
"BacA-related proteins"). These BacA-related proteins are
significantly more diverged from S. meliloti BacA (38 to
59% similarity), yet show large blocks of similar residues along long
stretches of the proteins. These more diverged BacA-related proteins
are all approximately 200 amino acids longer than the BacA/SbmA
proteins and have highly conserved motifs common to bacterial ABC
transport proteins (7) at their C termini. Interestingly,
both S. meliloti and E. coli have a BacA-related
protein as well as BacA/SbmA. The S. meliloti BacA-related
protein ExsE was identified as a part of the sequence analysis of a
cluster of genes involved in succinoglycan biosynthesis (GenBank
accession no. AJ225561); however, exsE does not appear to
play a role in synthesis of this polysaccharide and is not necessary
for successful symbiosis with alfalfa (22). The E. coli BacA-related protein YddA is a predicted cytoplasmic membrane exporter of unknown function (20) that has been
demonstrated to be regulated by the SOS response to DNA damage
(4). The biological roles have not been determined for any
of the BacA-related proteins, and it is not known if the more diverged
BacA-related proteins perform the same function(s) as the BacA/SbmA proteins.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
TABLE 1.
Bacterial strains and plasmids used in this study
Construction of site-directed mutants.
Site-directed
mutagenesis was carried out via PCR with mutagenic primers to direct
the change of a single amino acid to glycine. Plasmid pJG52B
(9), consisting of the S. meliloti bacA gene flanked by 1,580 bp of upstream sequence and 181 bp of downstream sequence cloned into the BamHI site of pBluescript
SK+, was used as template DNA. A pair of matched
complementary synthetic mutagenic oligonucleotides (33- to 35-mers)
containing the desired mutation flanked by at least 15 bp of wild-type
sequence on either side of the mutation were used as primers for PCR
amplification of the entire pJG52B plasmid for each mutant to be made.
All codons for the targeted amino acids were changed to GGA (glycine),
with the exception of tryptophan 57 (W57), which was changed to GGC (glycine) to prevent the formation of a BamHI site in
bacA, which would have disrupted subsequent cloning steps.
DNA was amplified with 50 ng of purified pJG52B DNA and 10 pmol of each
primer with the Pfu Turbo DNA polymerase and buffer
(Stratagene) with the following cycles: 95°C for 30 s,
95oC for 30 s, 44oC
for 1 min, and 68oC for 14 min, with steps 2 through 4 repeated 18 times. The PCR products were digested with
DpnI to cut parent plasmid DNA, and 10 µl of this DNA was
transformed into competent E. coli DH5- cells. DNA was
prepared from Apr colonies, and clones with the
correct restriction digest patterns were sequenced. Sequencing was
performed at the Massachusetts Institute of Technology Biopolymers
Laboratory with an ABI 377 sequencer and ABI BigDye kit version 2 AmpliTaq chemistry. Clones with the correct mutations were cut from
pJG52B with BamHI and cloned into the BamHI-cut,
calf alkaline phosphatase-treated, broad-host-range plasmid pRK404. The
resulting plasmids were transformed into competent E. coli
DH5- cells and plated onto LB mixed with tetracycline (LB Tc), IPTG
(isopropyl-
-D-thiogalactopyranoside), and
X-Gal
(5-bromo-4-chloro-3-indolyl--D-thiogalactopyranoside). DNA was prepared from white, Tcr colonies.
Plasmids with correct restriction digest patterns were transferred into
S. meliloti strains Rm8654 and Rm8002 via triparental conjugation with pRK600 to provide transfer functions
(17).
Sensitivity assays. For all assays, cultures were grown in LB/MC with antibiotics, adjusted to an optical density at 600 nm (OD600) of 0.1 or 0.2, and washed once in 0.85% saline. Plates were incubated at 30°C for 3 days, at which time, growth was evaluated or zones of bacterial growth inhibition were measured.
For bleomycin assays, 100-µl aliquots of cells adjusted to an OD600 of 0.2 were mixed with soft agar (nutrient broth, 8 g/liter; Bacto agar, 6.5 g/liter [both Difco]; NaCl, 5 g/liter) containing MC and tetracycline (MC Tc) and plated onto LB/MC Tc. After 30 min, sterile filter paper disks (6-mm diameter; Becton Dickinson) were placed on plates and then spotted with 1 µl of 10 mg of bleomycin A2 hydrochloride per ml (Calbiochem) diluted in 0.85% saline. Sodium dodecyl sulfate (SDS) assays were carried out as for the bleomycin assay, except soft agar and plates were not supplemented with MC. SDS (Gibco BRL) was diluted to 10% (wt/vol) in water, and disks were spotted with 5 µl. For ethanol assays, an LB Tc plate containing 4% ethanol was spotted with 10 µl of cells adjusted to an OD600 of 0.1. An LB Tc plate was duplicate spotted with diluted cells as a control. Gentamicin assays were carried out as for the SDS assay. Filter disks were spotted with 5 µl of a 5-mg/ml stock of gentamicin sulfate (Sigma) diluted in water. An LB Tc plate containing 15 µg of gentamicin per ml was spotted with cells prepared as for the ethanol assay, and an LB Tc plate was duplicate spotted with these cells as a control.Plant nodulation assay.
Alfalfa (Medicago sativa
cv. Iroquois) seeds (Agway, Inc., Plymouth, Ind.) were germinated,
inoculated, and grown on Jensen's nitrogen-free medium as described
previously (17). Plant height, leaf color, and nodule
characteristics were scored at 4 weeks postinfection. Plants with green
foliage and pink root nodules were scored as proficient for nitrogen
fixation (Fix+). Fix
plants were stunted, pale yellow, and devoid of pink nodules.
Microdissection of nodules and quantitation of S. meliloti content. For each set of nodules to be evaluated, six nodules were aseptically removed from plant roots with a razor blade. Nodules were placed on a clean petri dish under a dissecting microscope, the white tip was cut from the pink base of the nodule, and each of these fractions was processed separately. (The white portion of the nodule invariably included the topmost one-half to one-third of the nodule.) For the wild-type control, the uppermost one-third of the uniformly pink nodule was separated from the lower two-thirds of the nodule. For the Rm8654 bacA-null control, the small white nodules were not dissected and were processed whole. Nodules or nodule fractions were soaked in a solution of 50% Clorox bleach for 1 min in a well in a 96-well plate and then gently washed three times in sterile distilled water and moved to a well containing liquid LB supplemented with 0.3 M sucrose. Nodules were then crushed with forceps until completely macerated. Three stepwise 1:10 dilutions were then made in the same growth medium, and LB plates containing streptomycin (LB Sm) and LB Sm Tc plates were spotted with 25-µl aliquots of various dilutions to quantitate total rhizobium content and the content of Tcr plasmid-bearing rhizobia in nodules. Plates were scored after 4 days of growth at 30°C.
Microscopy. Nodules from alfalfa plants inoculated 4 weeks prior were viewed under a Nikon ECLIPSE E600 microscope by using the bright field with nodules illuminated by an external fiber optic light source. Nodules were placed on a microscope slide covered with a single layer of green laboratory tape (VWR) for the best contrast. Images were collected with SPOT RT software version 3.0 (Diagnostic Instruments, Inc., Sterling Heights, Mich.). Images were resized and optimized with Adobe Photoshop version 4.0.1 and combined in Canvas 5 (Deneba Systems).
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Choice of residues for mutagenesis.
Figure
1 shows an alignment of
11 BacA/SbmA and BacA-related proteins from a variety of bacteria, in
which the bottommost six proteins belong to the BacA-related grouping.
The Campylobacter jejeuni protein lacks the C-terminal
extended region of the BacA-related proteins and appears to be more
similar to the tightly grouped BacA/SbmA proteins (40 to 59% similar).
The C. jejeuni protein may be more diverged from the
BacA/SbmA proteins from the top four organisms in the alignment than
the four are from one another as a result of the much lower percent G+C
content of its genome (30 to 38% for C. jejeuni versus 62%
for S. meliloti, 56% for B. abortus, and 50 to
53% for E. coli and S. enterica serovar Typhimurium).
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Sensitivity of site-directed mutants to bleomycin.
BacA/SbmA
mutants from S. meliloti, B. abortus, E. coli, and S. enterica serovar Typhimurium are all more
resistant to the glycopeptide anticancer agent bleomycin than are their
isogenic parent strains (15, 18, 32; A. Ichige and K. LeVier, unpublished data). It has been proposed that BacA/SbmA serves
as a transporter to bring this drug into cells (32), where
it then leads to DNA damage and subsequent cell death
(10). To determine whether the residues chosen in this
study were involved in bleomycin sensitivity, we introduced the 20 site-directed mutants of S. meliloti bacA on the
low-copy-number vector pRK404 into the Rm8654 
bacA
background and tested for sensitivity to the drug. As shown in Fig.
2, providing the
bacA+ gene on pRK404 made S. meliloti bacA mutants more sensitive to killing by
bleomycin. The responses of the strains carrying the 20 site-directed
mutants to bleomycin ranged from close to the same degree of
sensitivity to killing, as exhibited by Rm8654 bacA
carrying the wild-type bacA+ gene (W57G,
S83G, S231G, and K350G), to levels of resistance equivalent to that of
the bacA mutant (H165G, W182G, Q193G, R194G, D198G,
F223G, R284G, and R389G), with other mutants having intermediate phenotypes. Thus, a number of the residues altered in this study are
necessary for the function of BacA that makes S. meliloti sensitive to bleomycin. With the exception of two mutants, all strains
showed very clear delineations on plates between the zone of bacterial
growth inhibition (proximal to where the bleomycin was spotted) and the
zone of confluent bacterial growth. Q193G and R194G had very unusual
zones of growth inhibition in which a small zone was completely devoid
of visible bacterial growth (indicating bleomycin resistance), but this
zone was surrounded by a much larger zone of very sparse bacterial
growth, which was surrounded by a zone of confluent bacterial growth.
In our previous studies, we had not encountered this resistance
pattern. To be consistent with the method used to score all other
plates in this assay, we measured the completely cleared innermost zone
of growth inhibition on these plates.
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Sensitivity of site-directed mutants to SDS and ethanol.
In a
similar fashion, we then tested the mutants for sensitivity to other
agents known to affect bacA mutants differently from the
wild-type parent strain (15; G. P. Ferguson, K. LeVier, R. M. Roop, and G. C. Walker, unpublished data). The
20 mutants showed a variety of sensitivities to SDS (Fig.
3): four mutants showed severe detergent
sensitivity (H165G, W182G, D198G, and R284G), and three more showed
intermediate sensitivity (R194G, F223G and R389G). Twelve of the
site-directed mutants grew as well on plates supplemented with 4%
ethanol as did the bacA+ strain Rm8002, and
four were as sensitive to ethanol as the bacA mutant
strain and showed no growth on plates (Table
2). Mutants R194G and R389G grew poorly
on ethanol, and Q193G had medium to light growth. Overall, the degrees
of sensitivity of the mutants to SDS and ethanol correlate well with
one another.
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Sensitivity to gentamicin.
BacA mutants of S. meliloti had previously been shown to have increased resistance to
low levels of the aminoglycoside antibiotics gentamicin, netilmicin,
and tobramycin (15). We therefore tested the site-directed
mutants for sensitivity to gentamicin by using a disk sensitivity
assay. However, plates did not have clear boundaries between zones of
bacterial growth versus nongrowth around gentamicin-containing filter
disks, but rather had a gradient of increasing growth as cells grew
more distant from the disk (data not shown; n = 3). There were clear visual differences between gentamicin-sensitive and
-resistant strains, but the indistinct nature of the edges of the zones
of growth inhibition made precise quantitation impossible. We therefore
used plates containing 15 µg of gentamicin per ml spotted with the
strains, evaluated them for growth, and saw a range of sensitivities
for the various mutants (Table 2). As in the bleomycin assay, mutants
Q193G and R194G had unusual behavior. Each was able to grow quite well
on gentamicin-containing media, reminiscent of the bacA
strain, but also showed a large, indistinct gradient of growth
inhibition in the crude disk sensitivity assay, suggesting that the
strains were quite sensitive to gentamicin, like the wild-type strain.
In general, however, strains resistant to bleomycin also showed
gentamicin resistance.
Symbiotic properties of site-directed mutants.
To determine
whether the residues chosen for this study were required for symbiosis,
alfalfa plants were inoculated with site-directed mutants, and the
mutants were evaluated 4 weeks postinfection for the ability to elicit
nitrogen-fixing symbioses with host plants (Table
3). A mixture of phenotypes was observed
with these point mutants. At 4 weeks postinfection, plants inoculated
with wild-type S. meliloti (Rm8002 carrying the control
vector pRK404) had dark green leaves, elongated pink nodules, and an
average height of 13 cm, whereas plants inoculated with the
bacA mutant (Rm8654 plus vector) were yellow, had small
round white nodules, and had an average height of 4 cm. Ten of the
site-directed mutants cloned into vector pRK404 and introduced into the
bacA strain Rm8654 were clearly able to fix nitrogen
(Fix+) when plants were inoculated with them.
Pink nodules were present on all plants, leaf colors ranged from light
to medium green, and plant heights varied from 4 to 11 cm. Mutants
Q193G and N312G appeared to be greatly reduced in their capacity for
nitrogen fixation, with each forming pale pink nodules on only a
fraction of the plants in the group. All of the plants in these groups were short and pale green. The remaining eight mutants had
Fix phenotypes when plants were inoculated with
them: all plants were short, yellow, and devoid of pink nodules.
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Dominant-negative properties of site-directed mutants. Many of the BacA-related proteins identified in BLAST searches have the highly conserved motifs diagnostic of ABC transport proteins, and recent work has demonstrated that a number of ABC proteins within this superfamily function as dimers (for examples, see references 13 and 14). In a wild-type genetic background, overproduction of a nonfunctional variant of a protein that functions as a dimer could lead to the formation of mutant-wild-type heterodimers, leading to dominant-negative inhibition of wild-type protein function (11). We were interested in learning whether our site-directed bacA mutants carried on the low-copy-number plasmid pRK404 would behave in a dominant-negative fashion when moved into a bacA+ background (Rm8002).
Of the eight bacA mutants whose phenotypes most resembled those of abacA mutant in the assays performed in this
study (H165G, W182G, Q193G, R194G, D198G, F223G, R284G, and R389G),
four were clearly dominant for bleomycin sensitivity (W182G, D198G,
F223G, and R284G) in this assay, because they increased the resistance of the bacA+ parent strain Rm8002 to
bleomycin (Fig. 5). Mutants Y120G, H165G, N312G, and R389G also showed mild dominant characteristics. These results indicate that the altered BacA proteins encoded by these mutants are being expressed and are consistent with the suggestion that
the dominance of these proteins is due to them forming dimers with
wild-type BacA proteins. The behavior of the Q193G and R194G mutants
was unexpected, since the bacA+
derivatives carrying these mutants showed a greater degree of sensitivity to bleomycin than the bacA+
parent alone. This observation suggests that the defects of these mutant BacA proteins can be suppressed when they interact with a
wild-type BacA protein to form a dimer.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Work with the 20 individual site-directed mutants constructed for
this study has shown that the S. meliloti BacA protein
requires different subsets of nonoverlapping amino acids for full
wild-type behavior in the various assays carried out in this work
(summarized in Fig. 6). Of the assays
performed in this work, the bleomycin sensitivity assay had the largest
number of site-directed mutants with phenotypes that differed from
those of wild-type strains. The data generated here are not
inconsistent with the previous hypothesis that BacA serves as a
transporter used by bleomycin to gain entry into S. meliloti
cells and that strains lacking full BacA function are unable to bring
the drug into cells at wild-type levels and are therefore more
resistant to bleomycin killing. However, several facts suggest that it
would be worth considering alternative hypotheses for the molecular
basis of the bleomycin resistance of bacA mutants. The mode
of bleomycin transport has not been fully elucidated in any bacterial
system to date, and the uptake of this drug is affected by changes in the bacterial cell membrane. In E. coli, mutations in three
separate steps in the biosynthetic pathway for ubiquinone, a part of
the cytoplasmic membrane electron transport chain that plays an
important role in the maintenance of membrane potential, all showed
increased resistance to phleomycin E, a bleomycin analog
(3).
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We monitored the site-directed mutants constructed here for sensitivity
to gentamicin, an aminoglycoside antibiotic to which bacA
mutants had previously been shown to have low levels of resistance (15). In this study, single amino acid changes in 8 out of
20 site-directed mutants led to significantly increased gentamicin resistance relative to the wild-type strain. Despite much study, the
mechanism by which aminoglycosides penetrate the cytoplasmic membranes
of gram-negative bacteria has not yet been determined, but under normal
growth conditions, it appears to be dependent on 
, the electrical
component of the proton motive force (31). The cytoplasmic
membrane electron transport chain component ubiquinone itself has been
proposed to be directly involved in aminoglycoside movement across the
cytoplasmic membrane.
Work in this study has shown that sensitivity to bleomycin and gentamicin is similarly affected by mutational alteration of BacA, with the exceptions of mutants Y120G and N312G, which have intermediate resistance to bleomycin, but wild-type levels of sensitivity to gentamicin. Additionally, mutants Q193G and R194G each had very odd growth patterns in response to these drugs in disk sensitivity assays. However, the overall similarity of responses of mutants to bleomycin and gentamicin may be accounted for by the fact that, although structurally dissimilar, both drugs are hydrophilic and cationic and may be taken into cells by a similar mode of action that is dependent on cytoplasmic membrane potential. It has also been proposed that aminoglycosides cross the outer membrane barrier of gram-negative bacteria by first binding to lipopolysaccharide and then disrupting and/or disorganizing the outer membrane, a mechanism also used by the polycationic polymyxin B (31). This mechanism may also be employed by bleomycin and gentamicin in wild-type S. meliloti cells.
The majority of site-directed mutants with the strongest bacA-null phenotypes cluster to what are predicted to be cytoplasmic loops of the BacA protein. This may suggest that one requirement for BacA that could manifest itself in the multiple phenotypes seen for this protein is for an interaction with an as yet unidentified cytoplasmic protein. A strong possibility would be for an ATPase necessary to form the full complement of an ATP-binding cassette (ABC) transport system. In bacteria, ABC transporters use the energy of ATP binding and hydrolysis to energize the transport of a wide range of substrates across the cytoplasmic membrane (20, 33). The basic unit of an ABC transporter is made up of a hydrophobic transmembrane domain (TMD) that spans the cytoplasmic membrane multiple times and forms a putative channel, and a highly conserved cognate soluble ABC-ATP-binding domain (ABC-ATPase) peripherally associated at the cytoplasmic face of the inner membrane. The ABC-ATPases are highly conserved proteins that are present in all organisms and have characteristic conserved A and B sites that form an ATP-binding pocket (12). In bacteria, the TMD and ABC-ATPase domains can be encoded by the genes of separate polypeptides, the products of which assemble into a multicomponent membrane-bound complex. The very strong conservation seen in the last two proposed cytoplasmic loops of BacA/SbmA proteins may reflect the interaction of these regions of BacA with a cognate ABC- ATPase. The BacA-related proteins, which carry both a TMD and an ABC-ATP-binding domain on the same polypeptide, show strong similarity to S. meliloti BacA in these conserved cytoplasmic loops as well. This may be an indication that the BacA-related proteins fold in such a way that their own ABC-ATPases bind to the cytoplasmic loops of the TMD portion of the same protein.
Recent work with a number of proteins has confirmed the model that ABC transporters function as dimers, with each half of the dimer consisting of one membrane-spanning TMD and one ATPase (for examples, see references 14 and 25). This situation is expected to be the case for other ABC transporters as well. Dimerization has also been demonstrated for Rad50, an ABC protein involved not in transport, but in DNA double-strand break repair (13). ATP promotes the dimerization of two Rad50 catalytic domains in a head-to-tail conformation, in which the highly conserved signature motif from each subunit binds the ATP bound to the opposite half of the dimer, with both ATP molecules buried in the dimer interface. The fact that our work with several site-directed mutants of the S. meliloti BacA protein with alterations in only a single amino acid led to dominant-negative effects when expressed in a wild-type background is consistent with the hypothesis that BacA (presumably bound to a cognate ABC-ATPase) may be acting as a dimer, with the dominant-negative phenotype seen suggesting that heterodimers formed between wild-type BacA and some site-directed mutants lead to defects in BacA function.
Alternatively, BacA could function as a transporter, but use a different, non-ATPase mode of energization for this process, such as from the proton motive force. The highly conserved cytoplasmic loops of BacA may be necessary for interactions with a non-ATPase protein of unknown function or may be involved in recognition or binding of a transport substrate. The BacA-related proteins could carry out the same function as BacA/SbmA proteins, but may have evolved to energize this process in an ATP-dependent manner instead.
Of the 20 site-directed mutants constructed for this study, 12 mutants had intermediate phenotypes that differed from the wild-type phenotype in at least one of the assays and showed a variety of patterns of phenotype mixtures. Such intermediate phenotypes could arise from alleles causing different degrees of loss of a single BacA function, or they could arise from individual mutations differentially affecting different functions of the BacA protein. The strongest trends seen in the assays performed here are that mutations that affect bleomycin resistance generally also affect gentamicin resistance to some degree, and mutants that are sensitive to ethanol are generally also sensitive to SDS. The bleomycin resistance assay seems to be the most sensitive assay, followed by the tests for nitrogen fixation ability and gentamicin sensitivity.
In the case of the phenotypes of some of the mutants examined in this
study, it would be easier to account for the data by postulating that
BacA has more than one function. For example, mutant N312G behaves like
wild-type strains for sensitivity to SDS, ethanol, and gentamicin, but
has intermediate sensitivity to bleomycin and carries out very
inefficient nitrogen fixation in association with alfalfa. Mutant Q332G
has almost identical bleomycin sensitivity to N312G, but grows
moderately well on 15 µg of gentamicin per ml, like
bacA mutant strains, and is apparently wild type with
regard to symbiosis. Mutants F223G and R389G each have
bacA mutant responses in all assays, except for the test for ethanol sensitivity, in which both strains show some wild-type capacity for growth. Mutant F363G shows intermediate phenotypes for
sensitivity to bleomycin and SDS and behaves like a bacA mutant for sensitivity to gentamicin and symbiosis with alfalfa, but
has full wild-type levels of resistance to ethanol. Mutant R194G
primarily has bacA behavior in all assays, and Q193G has intermediate or null behavior in all assays, except for sensitivity to
ethanol and SDS. However, both strains have very unusual growth patterns in response to bleomycin and gentamicin in disk sensitivity assays, and both lead to distinctly wild-type levels of bleomycin sensitivity when these mutations are moved into the wild-type Rm8002
background. Mutations in Q193, R194, and possibly F363 appear to be in
a minority class that lead to strong bacA
characteristics, yet can apparently be suppressed by wild-type BacA in
a dominant-negative assay. For the mutants discussed above, it is not
easy to explain the differences in phenotype combinations by different
degrees of loss of a single function.
We have demonstrated that single amino acid changes in the BacA protein can profoundly influence both responses to stressful compounds and symbiotic interactions with alfalfa plants. The data from the assays performed here are compatible with bacA mutants having some bacterial cell surface alterations, but the data from some of the mutants with intermediate phenotypes suggest that the situation could be more complex and that BacA carries out multiple functions.
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ACKNOWLEDGMENTS |
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We thank Mary Lou Pardue and Janet George for help with nodule imaging. We also thank Gail Ferguson and Brett Pellock for critical review of the manuscript and Gail Ferguson for collaboration and discussion regarding some of the mutant phenotypes.
This work was supported by U.S. Public Health Service grant GM31030 to G.C.W. from the National Institute of General Medicinal Science. K.L. was supported by a U.S. Department of Energy-Biosciences Fellowship from the Life Sciences Research Foundation.
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FOOTNOTES |
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* Corresponding author. Mailing address: Biology Department, 68-659, Massachusetts Institute of Technology, 77 Massachusetts Ave., Cambridge, MA 02139. Phone: (617) 253-6716. Fax: (617) 253-2643. E-mail: gwalker{at}mit.edu.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Journal of Bacteriology, November 2001, p. 6444-6453, Vol. 183, No. 21
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.21.6444-6453.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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