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J Bacteriol, January 1998, p. 128-135, Vol. 180, No. 1
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Departments of
Medicine3 and of
Molecular Biology and
Microbiology,
Received 19 June 1997/Accepted 18 October 1997
Providencia stuartii contains a chromosomal
2'-N-acetyltransferase [AAC(2')-Ia] involved in the O
acetylation of peptidoglycan. The AAC(2')-Ia enzyme is also capable of
acetylating and inactivating certain aminoglycosides and confers
high-level resistance to these antibiotics when overexpressed. We
report the identification of a locus in P. stuartii,
designated aarF, that is required for the expression of
AAC(2')-Ia. Northern (RNA) analysis demonstrated that
aac(2')-Ia mRNA levels were dramatically decreased in a
P. stuartii strain carrying an
aarF::Cm disruption. The
aarF::Cm disruption also resulted in a deficiency
in the respiratory cofactor ubiquinone. The aarF locus
encoded a protein that had a predicted molecular mass of 62,559 Da and
that exhibited extensive amino acid similarity to the products of two
adjacent open reading frames of unknown function (YigQ and YigR),
located at 86 min on the Escherichia coli chromosome. An
E. coli yigR::Kan mutant was also deficient in
ubiquinone content. Complementation studies demonstrated that the
aarF and the E. coli yigQR loci were
functionally equivalent. The aarF or yigQR
genes were unable to complement ubiD and ubiE mutations that are also present at 86 min on the E. coli
chromosome. This result indicates that aarF
(yigQR) represents a novel locus for ubiquinone production
and reveals a previously unreported connection between ubiquinone
biosynthesis and the regulation of gene expression.
The gram-negative bacterium
Providencia stuartii is a member of the Proteeae,
which includes the genera Proteus, Morganella, and Providencia. Members of the Proteeae possess
peptidoglycan that is O acetylated at the C-6 hydroxyl position of
N-acetylmuramyl residues (8). This modification
confers resistance to muramidases such as lysozyme and has been
speculated to modulate the activity of endogenous
peptidoglycan-specific hydrolases, termed autolysins (8, 9,
16). P. stuartii contains a chromosomal
2'-N-acetyltransferase, encoded by the aac(2')-Ia
locus, that has been implicated in this process (7, 29, 34,
38). This enzyme is also capable of acetylating and inactivating
certain aminoglycoside antibiotics and was originally identified in
clinical strains of P. stuartii overexpressing the enzyme
(7, 38).
The aac(2')-Ia gene is expressed at low levels in wild-type
P. stuartii (34). The expression of
aac(2')-Ia is controlled in part by a small transcriptional
activator, AarP, that is related to members of the XylS-AraC family of
positive activators (18, 24). Recessive mutations that
result in increased aac(2')-Ia mRNA accumulation have also
been identified in five loci (aarA, aarB,
aarC, aarD, and aarG) (25,
32-35). The expression of aarP has been shown to be
increased in the aarB, aarC, and aarG
mutant backgrounds. These results suggest that aarP may play
a central role in the activation of aac(2')-Ia expression
(32, 35).
In this study, we report the identification of the aarF gene
of P. stuartii and demonstrate that aarF function
is required for the expression of aac(2')-Ia. We also
present evidence suggesting that aarF is functionally
equivalent to Escherichia coli yigQR and that both
aarF and yigQR represent novel loci required for the production of ubiquinone.
Bacterial strains and plasmids.
All bacteria,
bacteriophages, and plasmids used in this study are described in Table
1.
ABSTRACT
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
TABLE 1.
Bacterial strains and plasmids
Media and bacterial growth. Bacteria were routinely grown in Luria-Bertani (LB) broth at 37°C. To test for the aerobic utilization of nonfermentable carbon sources, M9 minimal agar plates (26) containing either 0.2% glucose or 0.5% succinate were used. For the growth of E. coli AN66 ubiD and AN70 ubiE, M9 plates were supplemented with L-leucine, L-threonine, and L-methionine each at a final concentration of 0.2 mM and with thiamine at a final concentration of 0.02 µM.
Gentamicin resistance determinations. MICs for gentamicin were determined by an agar dilution method with twofold increasing concentrations of gentamicin. The MIC was defined as the lowest concentration of gentamicin that prevented the formation of single colonies.
Plasmid constructions.
A genomic library of P. stuartii DNA was constructed by ligation of partial
Sau3AI fragments into BamHI-digested and
dephosphorylated pACYC184 and was described previously (6,
24). Plasmid pAFM12 is a pACYC184 recombinant with a 3.6-kb
Sau3AI fragment of P. stuartii DNA containing the
aarF gene. Plasmid pSK.aarF was constructed by inserting a
1.9-kb SphI fragment from pAFM12 into pBluescript SK(
)
linearized with SmaI. A genomic library of E. coli partial Sau3AI fragments constructed in pET21a was
kindly provided by P. deBoer, Case Western Reserve University. Plasmid
pEF1 is a pET21a recombinant and contains a 3.5-kb insert. Plasmid
pSK-2.6 contains a 2.6-kb SalI fragment from pEF1 ligated
into the SalI site of pBluescript SK(). Plasmid pSK.yigQR
was constructed by digesting pSK-2.6 with EcoRV to release a
457-bp fragment and religating the linearized plasmid. Plasmid
pSK.yigQR
DraI was constructed by linearizing pSK.yigQR
with HincII followed by partial digestion with
DraI to release a 467-bp fragment and religation. Plasmid
pSK.yigR was constructed by digesting pSK-2.6 with ClaI and
NarI to release a 701-bp fragment and religating the
linearized plasmid.
Identification of AarF.
To identify the aarF gene
product, a XhoI-XbaI fragment containing the
aarF gene was excised from pSK.aarF and ligated into pBluescript KS() to create pKS.aarF. In pKS.aarF, the aarF
gene is downstream from and in the same orientation as the T7 promoter. To create a negative control plasmid, pKS.aarF was linearized with
NheI, which cuts internal to the aarF coding
region, end filled with the Klenow fragment and deoxynucleoside
triphosphates (dNTPs), and religated. The resulting plasmid,
pKS.NheI, carries a frameshift mutation that truncates the
predicted AarF protein after amino acid 99. To ensure that the
aarF gene would not be expressed in the absence of
isopropyl-
-D-thiogalactopyranoside (IPTG), the
lacIq gene was introduced into plasmid pACYC184
(6) as follows. A 1.3-kb fragment containing the
lacIq gene was released from plasmid pMJR1560
(Amersham) by digestion with EcoRI and
HindIII and was cloned into pBluescript SK() that had
been digested with the same enzymes to create pSK.lacIq.
The lacIq gene was then excised from
pSK.lacIq as a 1.3-kb XbaI-ClaI
fragment and was cloned into pACYC184 that had been digested with the
same enzymes to create pACYC184.lacIq. Plasmid
pACYC184.lacIq and each of the aarF derivative
plasmids were cointroduced into E. coli BL21(DE3) (Novagen).
Cultures were shaken in LB broth at 37°C to an optical density at 600 nm (OD600) of 0.6 and induced with 1 mM IPTG. After 30 min,
rifampin was added to a final concentration of 100 µg/ml, and
cultures were shaken for an additional 2.5 h. Cells were
harvested, and 15-µl aliquots were dissolved in sodium dodecyl
sulfate (SDS) loading dye, boiled, and run on SDS-10% polyacrylamide
gels. Total cellular protein was visualized after Coomassie blue
staining.
Construction of chromosomal aarF and yigR disruptions. To construct an aarF null allele in P. stuartii, plasmid pSK.aarF was linearized at a unique NruI site present midway in the aarF coding region at position 956. A chloramphenicol resistance cassette from pUT::mini-Tn5Cm (15), present as a 3.6-kb HindIII fragment, was end filled with the Klenow fragment of DNA polymerase I and dNTPs and ligated into NruI-linearized pSK.aarF to produce pSK.aarF::Cm. To recombine the aarF::Cm disruption into the P. stuartii chromosome, a 6-kb BamHI-ApaI fragment was excised from pSK.aarF::Cm and ligated into suicide vector pKNG101 (22) that had been digested with the same enzymes. The resulting plasmid, designated pKNG101.aarF::Cm, was integrated into the chromosome of strain PR50 by conjugal mating as described previously (24). The merodiploid was resolved by selection on 5% sucrose, and strains containing the disrupted aarF locus were identified on the basis of chloramphenicol resistance. Southern analysis confirmed that the chromosomal aarF locus had been disrupted by the chloramphenicol resistance cassette.
To construct a yigR null allele in E. coli, plasmid pSK-2.6 was linearized at a unique BsmI site internal to the yigR open reading frame and treated with T4 DNA polymerase and dNTPs to produce blunt ends. A 1.3-kb SmaI fragment containing a kanamycin resistance cassette was excised from pUC4::KIXX (Pharmacia) and ligated into linearized pSK-2.6 to produce pSK.yigR::Kan. The 3.8-kb yigR::Kan disruption was then excised from pSK.yigR::Kan with SalI and ligated into the unique SalI site of suicide vector pKNG101. The resulting plasmid, designated pKNG101.yigR::Kan, was introduced into the chromosome of strain DM113 by conjugal mating essentially as described previously (24), with the exception that rifampin was used at 100 µg/ml to counterselect against the donor strain. The merodiploid was resolved by selection on 5% sucrose, and strains containing the disrupted yigR locus were identified on the basis of kanamycin resistance. Southern analysis confirmed that the chromosomal yigR locus had been disrupted by the kanamycin resistance cassette. The chromosomal yigR::Kan disruption was then introduced into wild-type E. coli RM1734 via a P1 lysate derived from DM115. Transductants were obtained on LB agar plates containing 50 µg of kanamycin per ml, and the yigR::Kan disruption was confirmed by Southern analysis. A representative strain was designated DM123.-Galactosidase assays.
Plasmid pR401 containing an
aac(2')-lacZ transcriptional fusion was described previously
(33). -Galactosidase assays were performed in triplicate
with cell samples harvested at the early log phase, and activity was
expressed in Miller units (26). Reported values represent
the average for triplicate samples.
RNA analysis. To examine aac(2')-Ia mRNA levels in P. stuartii strains, cultures were grown in LB broth at 37°C to an A600 of 0.2, and RNA was prepared with TRIazol reagent (Gibco/BRL). RNA was loaded in duplicate, fractionated on a 1% agarose gel containing 2.2 M formaldehyde, and transferred to a nylon membrane by capillary transfer. Filters were probed with a digoxigenin-labeled 602-bp TaqI-SspI fragment containing the aac(2')-Ia coding sequence. As an internal control for loading, probes were "spiked" with a labeled fragment internal to the E. coli 23S rRNA coding sequence. Filters were developed with Lumi-Phos 530 (Boehringer Mannheim Biochemicals) and exposed to autoradiography film.
Ubiquinone analysis.
Cells were first grown in LB medium
supplemented with 0.5% glucose in 2-liter flasks. The cultures were
shaken overnight as starter cultures of 50 ml in 250-ml flasks. Cells
were then inoculated into 500 ml of the same medium to an
OD600 of 0.05 and shaken at 37°C. Cells were harvested at
an OD600 of 2.0. Typically, 3 liters of culture was used
for analysis. Cells were harvested, and pellets were washed twice in 50 mM potassium phosphate buffer and stored at 20°C. Quinone
extraction was performed as described by Collins (10).
Thawed cells, 5 g (wet weight), in 10 ml of phosphate buffer were
broken by sonication at 1-min intervals, with 1 min of cooling in
between the intervals, for 5 min. Lysis was confirmed by microscopic
examination. Lysed cells were resuspended in 100 ml of acetone and left
to digest for 12 h at 4°C with stirring. Cell debris was removed
by filtration through Whatman no. 1 filter paper. The filtrate was then
evaporated to 1 ml in a rotary evaporator at 40°C. The sample was
freeze-dried, and the residue was dissolved in 2 ml of acetone. Samples
(100 µl) were applied to a Silica Gel F254 plastic-backed
thin-layer chromatography plate (Merck item 5735), which was developed
in hexane-diethyl ether (85:15, wt/vol). Coenzyme Q8 was used as a
standard. The coenzyme Q8 spots were visualized by UV illumination. The
spots were cut out, and quinones were eluted with 100% ethanol. The
silica gel powder was removed by centrifugation, and the spectra of the
clear supernatants were recorded with a Variant DMS-90
spectrophotometer.
Nucleotide sequence accession number. The nucleotide sequence of aarF has been deposited in the EMBL/GenBank/DDBJ Nucleotide Sequence Data Library under accession no. AF002165.
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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|---|
Identification of the aarF locus.
PR50.AFM12
is a spontaneous gentamicin-resistant derivative of wild-type P. stuartii PR50. Gentamicin resistance in PR50.AFM12 was
increased 256-fold (1,024 µg/ml) over that observed for wild-type PR50 (4 µg/ml). To determine whether aac(2')-Ia
expression was increased in PR50.AFM12, plasmid pR401, containing
an aac(2')-lacZ transcriptional fusion, was
introduced. PR50.AFM12/pR401 formed dark blue colonies when grown
on LB agar plates containing
5-bromo-4-chloro-3-indolyl--D-galactopyranoside. In
contrast, isogenic strain PR50/pR401 formed white colonies when grown
on the same plates. The mutant allele in PR50.AFM12 was therefore
designated aarF1. The regulatory effects of aarF1 on aac(2')-Ia expression were examined in further detail
(see below).
DNA sequence analysis.
A 1.9-kb SphI fragment
from pAFM12 was subcloned into pBluescript SK(), resulting in plasmid
pSK.aarF. The introduction of pSK.aarF into pAFM12 also resulted in
transformants exhibiting a wild-type growth rate (Fig.
1B). The nucleotide sequence of the
1,877-bp fragment in pSK.aarF was determined on both strands. A single
open reading frame of 1,632 bp, predicted to encode a 544-amino-acid
polypeptide (Fig. 1A), was identified. To determine whether this open
reading frame encoded aarF, a chloramphenicol resistance
cassette from pUT::mini-Tn5Cm (15) was
inserted into a unique NruI site within this open reading
frame. The resulting plasmid, pSK.aarF::Cm, was unable to
restore a wild-type growth rate when introduced into PR50.AFM12 (Fig.
1B). Based on this result and the data presented below, this open
reading frame has been designated aarF.
|
Identification of the aarF gene product.
To
determine whether the aarF locus encoded a polypeptide of
the predicted size, the aarF gene was excised from pSK.aarF
and subcloned into pBluescript KS() to enable transcription to be driven from the T7 promoter. The resulting plasmid, pKS.aarF, was
transformed into the expression strain E. coli
BL21(DE3)/pACYC184.lacIq. A 67-kDa polypeptide observed
upon induction with IPTG was not observed in an uninduced control
culture (Fig. 2). No induction was
observed in a control strain that was transformed with pBluescript KS(). The size of the observed polypeptide correlated with the predicted size of 62.5 kDa. To confirm that the observed polypeptide was encoded by the aarF gene, a small insertion was
introduced at a unique NheI site (Fig. 1B). This insertion
resulted in a frameshift leading to a severe truncation of the putative
AarF protein. When the resulting plasmid, designated
pKS.NheI, was introduced into the E. coli
expression strain, no induced polypeptide was observed upon the
addition of IPTG (Fig. 2). The introduction of plasmid
pKS.NheI into PR50.AFM12 also failed to restore a wild-type growth rate (Fig. 1B).
|
Cloning and analysis of the E. coli yigQR locus.
The predicted amino acid sequence of the aarF open reading
frame exhibited a high degree of homology to two putative adjacent open
reading frames of unknown function, present at 86 min on the E. coli chromosome, and designated yigQ (75% identity)
and yigR (77% identity) (14). The amino acid
alignment of AarF with YigQ and YigR is illustrated in Fig.
3. Because of the high degree of homology
between AarF and the putative YigQ and YigR proteins, it was
hypothesized that the yigQR locus may be able to
functionally substitute for aarF in P. stuartii.
To test this hypothesis, a partial Sau3AI library prepared
from a wild-type E. coli strain was introduced into
PR50.AFM12, and transformants forming wild-type-size colonies were
selected. Plasmids from 11 individual large colonies were analyzed by
restriction mapping, and all were shown to contain inserts with a
common region of DNA (data not shown). One plasmid, designated pEF1,
contained a 3.5-kb insert and was chosen for further study. A 2.6-kb
SalI fragment from pEF1 was subcloned into pBluescript
SK(), creating pSK-2.6. The introduction of pSK-2.6 into PR50.AFM12
also restored a wild-type growth rate. To determine the identity of the
cloned E. coli DNA in pSK-2.6, sequence data were obtained
from both ends and was compared to the GenBank sequence databases. The
cloned E. coli fragment in pSK-2.6 extends from the
SalI site at nucleotide 72625 to the Sau3AI site
at nucleotide 75101, as reported by Daniels et al. (14).
This fragment contains the yigQ and yigR open
reading frames as well as an upstream open reading frame, designated
yigP (14). To determine which open reading
frame(s) was required for the complementation of PR50.AFM12, a series
of derivatives of pSK-2.6 were created as described in Materials and
Methods. These derivatives were introduced into PR50.AFM12 and scored
for complementation by the ability of the insert to restore a wild-type growth rate (Fig. 4). Plasmid pSK.yigQR,
which has a deletion of yigP, retained the ability to
complement the aarF1 mutation. In contrast, a deletion
removing both the yigP open reading frame and the initiating
ATG codon of the yigQ open reading frame (plasmid pSK.yigR)
resulted in partial complementation of the growth defect in PR50.AFM12.
Similarly, a deletion removing the C-terminal 96 amino acids of the
yigR open reading frame (plasmid
pSK.yigQRDraI) also resulted in partial complementation
of PR50.AFM12. Finally, insertion of a kanamycin resistance
cassette into a unique BsmI site internal to the
yigR open reading frame (plasmid
pSK.yigR::Kan) abolished the complementation of PR50.AFM12.
These data indicate that yigP is not required for the
complementation of PR50.AFM12, whereas both the yigQ and
yigR open reading frames are required for the
complementation of PR50.AFM12.
|
|
Analysis of chromosomal aarF and yigR null
mutants.
A chromosomal aarF::Cm disruption in
wild-type PR50 was constructed by allelic replacement as described in
Materials and Methods, resulting in strain PR54. PR54 exhibited a slow
growth phenotype similar to that of PR50.AFM12 (aarF1) and
demonstrated resistance to gentamicin (1,024 µg/ml) that was equal to
that of PR50.AFM12. The introduction of pSK.aarF into PR54 restored a
wild-type growth rate, whereas the introduction of control plasmid
pBluescript SK() did not affect either growth rate or gentamicin
resistance (data not shown). Plasmid pSK-2.6, containing the wild-type
yigPQR locus from E. coli, also restored a
wild-type growth rate when introduced into PR54 (data not shown). The
ability of the E. coli yigQR locus to substitute for
aarF in PR54 suggested that the two loci are functionally
equivalent. To examine the role of the yigQR locus in
E. coli, the yigR::Kan disruption from
pSK.yigR::Kan was introduced into the chromosome of wild-type
E. coli RM1734 as described in Materials and Methods to
produce DM123. DM123 exhibited a slow growth phenotype similar to that
of the P. stuartii aarF::Cm mutant PR54. The
introduction of either pSK-2.6 or pSK.aarF restored wild-type growth to
DM123, whereas the introduction of the cloning vector pBluescript
SK() did not affect the growth of DM123 (data not shown).
Effects of aarF::Cm on aac(2')-Ia
expression.
Preliminary data suggested that the aarF1
allele increased aac(2')-Ia expression. To determine the
phenotype of an aarF::Cm disruption, plasmid pR401
[aac(2')-lacZ] was introduced into PR54. PR54/pR401 formed
dark blue colonies when grown on LB agar plates containing
5-bromo-4-chloro-3-indolyl--D-galactopyranoside, whereas PR50/pR401 formed white colonies when grown on the same plates. In
liquid assays, the accumulation of -galactosidase in PR54/pR401 was
measured at 19.9 ± 0.74 U and represented a 17-fold increase over
the value for PR50/pR401 (1.14 ± 0.05 U). However, a control construct containing a lacp-lacZ transcriptional
fusion resulted in a 102-fold increase in -galactosidase levels in
PR54 relative to those observed in PR50 (data not shown). This result
indicated that the aarF::Cm allele increased
-galactosidase expression or activity independently of the
aac(2')-Ia promoter. Preliminary data indicated that the
copy number of pR401 is significantly higher in the
aarF::Cm background (32). In addition,
these data also suggested that aarF::Cm may
actually decrease aac(2')-Ia promoter activity. To confirm
these results at the level of aac(2')-Ia mRNA accumulation,
RNA was prepared from PR54 and the parental strain, PR50, and was
analyzed by Northern analysis with a probe specific to
aac(2')-Ia. The results shown in Fig.
5 demonstrated that aac(2')-Ia
mRNA levels were significantly lower in PR54 than in PR50.
|
aarF and yigR mutants are deficient in ubiquinone. Because aac(2')-Ia mRNA levels in the aarF mutant background are not increased above wild-type levels, an alternative mechanism must be responsible for the high-level gentamicin resistance. Mutations that disrupt the aerobic respiratory electron transport chain have been reported to result in increased aminoglycoside resistance (2-5, 25, 27). One such class of mutants are those that are defective in ubiquinone biosynthesis (3, 4). Mutants that are defective in ubiquinone biosynthesis are unable to grow aerobically on nonfermentable carbon sources, such as malate or succinate (11). To determine whether PR54 was defective in ubiquinone production, the growth of PR50 and PR54 was compared aerobically on minimal media containing either glucose or succinate as the sole carbon source. Wild-type PR50 was able to utilize either glucose or succinate as a sole carbon source (Table 2). In contrast, PR54 was unable to utilize succinate as a sole carbon source aerobically. Similarly, E. coli RM1734 was able to utilize either glucose or succinate as a sole carbon source, whereas DM123 was unable to utilize succinate as a sole carbon source. The introduction of the complementating plasmids pSK.aarF and pSK-2.6 into PR54 and DM123, respectively, restored the ability to utilize succinate (Table 2).
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DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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In a search for regulators of the aac(2')-Ia gene of P. stuartii, we identified aarF, a gene required for the production of the respiratory cofactor ubiquinone (coenzyme Q). The aarF1 and aarF::Cm mutations resulted in a 256-fold increase in gentamicin resistance above wild-type levels and caused a severe defect in aerobic growth on rich media. Initial observations obtained through the use of an aac(2')-lacZ transcriptional fusion suggested that aac(2')-Ia expression was increased in the aarF mutant background. However, this expression appeared to be an artifact due to increased plasmid copy number in the aarF mutant background. Direct examination by Northern analysis revealed that aac(2')-Ia mRNA levels in PR54 (aarF::Cm) were dramatically lower than those in wild-type PR50. To our knowledge, ubiquinone has never been implicated in gene regulation, so this finding is a novel one.
In light of the above data, it seems unlikely that ubiquinone is directly involved in the regulation of aac(2')-Ia. We recently identified a locus in P. stuartii, designated aarE, that is also required for the expression of aac(2')-Ia. The aarE gene was found to be the P. stuartii homolog of ubiA (32, 37). In contrast, the aarD locus (25), representing the P. stuartii homolog of cydD (30, 31), is required for the function of the cytochrome d terminal oxidase and is a negative regulator of aac(2')-Ia expression. We propose a model for the regulation of aac(2')-Ia expression by a regulatory cascade in which ubiquinone acts as an effector molecule (Fig. 6). In this model, the reduced form of ubiquinone (ubiquinol) serves as a signal to activate aac(2')-Ia expression through an uncharacterized pathway. It is important to note that this pathway appears to be independent of the previously identified activator AarP (24). According to this model, in a cytochrome d-deficient strain, ubiquinol is predicted to accumulate and to result in the activation of aac(2')-Ia expression. In ubiquinone-deficient aarE and aarF mutant strains, the regulatory cascade would be disrupted, resulting in decreased aac(2')-Ia expression. Further studies with inhibitors of electron transport may provide evidence to support this model.
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Because aac(2')-Ia mRNA levels are decreased in PR50.AFM12 (aarF1) and PR54 (aarF::Cm), an alternative mechanism must be responsible for the large increase in gentamicin resistance observed in the aarF mutant background. Aminoglycoside uptake requires a sufficiently negative membrane potential as well as active electron transport (3, 13, 17). High-level, nonenzymatic resistance to the aminoglycosides usually arises from mutations in components of the aerobic respiratory chain (1, 3, 4, 13, 19). PR54 was unable to utilize succinate as a sole carbon source aerobically, and extracts from this strain were found to be devoid of ubiquinone. Ubiquinone-deficient E. coli mutants were previously shown to exhibit increased gentamicin resistance and were found to accumulate gentamicin poorly (3, 4). Therefore, the high-level gentamicin resistance observed in PR54 is likely associated with decreased accumulation of the drug resulting from the absence of aerobic electron transport.
The aarF locus was found to encode a single 544-amino-acid protein. The AarF polypeptide was identified with a T7 expression system and exhibited an apparent molecular mass of 67 kDa, in agreement with the predicted size of 62.5 kDa. The predicted AarF protein exhibited extensive amino acid identity with the products of two putative adjacent open reading frames, yigQ and yigR, present at 86.6 min on the E. coli chromosome (14). This region of the chromosome has been sequenced as part of the E. coli sequencing project, and frameshifts that could merge yigQ and yigR into one contiguous open reading frame are possible. It should be noted that we have no evidence suggesting that yigQ and yigR are contiguous.
An E. coli yigR::Kan mutant was found to be defective in ubiquinone biosynthesis. Three ubiquinone biosynthesis genes, ubiB, ubiD, and ubiE, map near yigQ and yigR at min 86 on the E. coli chromosome (12, 14, 23, 39). Complementation studies showed that the yigQR genes did not complement ubiD and ubiE mutations. In addition, the ubiB gene lies upstream of yigQR (14). Therefore, aarF (yigQR) represents a novel gene in the ubiquinone biosynthetic pathway. Extracts from both P. stuartii aarF and E. coli yigR mutants contained significant amounts of a ubiquinone precursor. Future studies to determine the identity of this precursor will be required to assign a function to the aarF (yigQR) locus.
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ACKNOWLEDGMENTS |
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We are grateful to Frank Gibson for the gifts of bacterial strains.
This work was supported by grant MCB9405882 from the National Science Foundation.
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FOOTNOTES |
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* Corresponding author. Mailing address: Infectious Diseases Section 1110W, Wade Park Medical Center, 10701 E. Blvd., Cleveland, OH 44106. Phone: (216) 368-0744. Fax: (216) 368-2034. E-mail: pxr17{at}po.cwru.edu.
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REFERENCES |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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| 1. |
Bryan, L. E., and H. M. V. D. Elzen.
1976.
Streptomycin accumulation in susceptible and resistant strains of Escherichia coli and Pseudomonas aeruginosa.
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