From the Department of Biology, Georgia State University, Atlanta, Georgia 30303
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ABSTRACT |
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The drrAB operon of
Streptomyces peucetius encodes for resistance to the
antibiotics doxorubicin and daunorubicin. Subcloning of the
drrAB genes in Escherichia coli has previously
been shown to result in expression of DrrA and DrrB proteins and
resistance to doxorubicin in a sensitive strain of E. coli.
DrrA, a peripheral membrane protein, binds ATP in a UV-catalyzed
reaction in a doxorubicin-dependent manner; DrrB, a
hydrophobic protein, is localized to the inner membrane of E. coli (Kaur, P. (1997) J. Bacteriol. 179, 569-575). The present study provides evidence that DrrB, the membrane component of the complex, is stably maintained in the cell only if DrrA is
present. Furthermore, it was found that the catalytic component DrrA is
in an active conformation only when it is in a complex with DrrB. In a
subclone containing the drrB gene by itself, no DrrB
protein could be detected, although a translational fusion of the first
15 amino acids of DrrB to -galactosidase indicated that DrrB is
translated in the absence of DrrA. Upon co-transformation with a
plasmid containing the drrA gene in trans, DrrB
could again be detected in these cells. UV cross-linking studies with
[
-32P]ATP showed that only the membrane-bound form of
DrrA in cells containing both DrrA and DrrB was in a conformation
competent to bind ATP. Chemical cross-linking studies also provided
direct evidence for interaction between the two proteins. Based on
these analyses, a model for interaction between DrrA and DrrB
proteins is presented.
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INTRODUCTION |
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Doxorubicin and daunorubicin, two antibiotics produced by Streptomyces peucetius, are widely used in chemotherapy. S. peucetius is itself resistant to the inhibitory action of these drugs. Resistance in S. peucetius is encoded by the drr operon that contains two open reading frames, drrA and drrB (1). DrrA and DrrB proteins have been hypothesized to form an efflux pump that confers resistance by transport of the drugs out of the cell (1, 2). DrrA protein consists of one nucleotide binding domain with homology to the ABC family of proteins to which P-glycoprotein (Pgp1; Ref. 3) belongs. The product of the drrB gene is a membrane protein (1, 2) with homology to membrane components of the bacterial ABC transporters (4). Pgp is expressed in human cancer cell lines, where it confers resistance to a variety of structurally unrelated chemotherapeutic drugs, including doxorubicin and daunorubicin (3). This phenomenon is referred to as multidrug resistance. Pgp contains a drug-stimulated ATPase activity (5); however, its mode of action and the mechanism by which it can transport structurally unrelated substrates is not understood. Since DrrA and Pgp are homologous proteins and both confer resistance to doxorubicin and daunorubicin, an understanding of the structure and function of Drr pump is expected to contribute to a better understanding of the function and evolution of Pgp.
The drr operon has previously been subcloned in an Escherichia coli expression vector, and both proteins have been identified using antisera raised in rabbits (2). Expression of the proteins in an acr strain of E. coli resulted in doxorubicin resistance in these cells, indicating that the proteins expressed in E. coli retain proper conformation and function. Isolation of active alkaline phosphatase fusions in DrrB showed that DrrB is an integral membrane protein (2). DrrA, a peripheral membrane protein was shown to bind ATP or GTP in the presence of Mg2+. The nucleotide binding to DrrA was found to be doxorubicin-dependent (2), indicating that the activity of DrrA is regulated by the substrate of the pump.
Most ABC transporters, including Pgp, consist of two nucleotide binding
domains and two membrane-spanning domains of six -helices each. In
Pgp, the four domains form one large protein of about 170 kDa (3). The
Drr system, instead, consists of two subunits, DrrA and DrrB, that
carry individual domains. Together, a monomer of DrrA and a monomer of
DrrB form a molecule about half the size of Pgp; however, the
stoichiometry of the DrrA and DrrB proteins in the Drr pump is not
known. The present study focuses on an interaction between DrrA and
DrrB; the data indicate a strong dependence of the proteins on each
other for their expression and function such that the two protein
subunits behave as domains of a larger protein. The DrrB protein was
detected in the cell membrane of these cells only if there was
simultaneous expression of DrrA. In addition, DrrA was in an active
conformation to bind and/or hydrolyze ATP only if it was in a complex
with DrrB in the membrane. Chemical cross-linking studies also suggest
a direct interaction between DrrA and DrrB with the suggested
stoichiometry of the complex being DrrA2B2.
These results bear important implications for the evolution of
multidomain proteins, including Pgp, and for understanding the
interaction between their domains.
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EXPERIMENTAL PROCEDURES |
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Bacterial Strains and Plasmids-- The E. coli strains and plasmids used in this study are described in Table I.
Media and Growth Conditions-- The cells were grown in LB medium (6) at 37 °C. Chloramphenicol was added to 20 µg/ml, and ampicillin was added to 100 µg/ml.
DNA Manipulations-- The conditions for plasmid isolation, DNA endonuclease restriction analysis, ligation, and sequencing have been described elsewhere (7).
Subcloning of the drrA Gene-- The 1.0-kilobase pair NdeI-HindIII fragment from pDX102 was subcloned behind the lac promoter in pUC18 vector by substitution of the arsA gene in pUC18arsA. This clone has been designated pDX108. The drrA gene in this construct utilizes the translational start signals of the arsA gene.
Creation of Translational Fusions of DrrB to
-Galactosidase--
A translational fusion of the first 15 amino
acids of DrrB to the 8th amino acid of
-galactosidase was created.
Using pDX101 or pDX103 as the template (Fig. 1 and Table I), the region
contained between the lac promoter and the 45th nucleotide
of the drrB gene was polymerase chain reaction-amplified.
Polymerase chain reaction primers had the following nucleotide
sequence, and each primer contained the following HindIII
restriction site: I, 5'-GCCGCCAAGCTTCCTCTCCCCGCGCGTTGG-3'; II,
5'-GCCGCCAAGCTTCGCTCACAGGGGTCGTGG-3'. The amplified product was ligated
to the translational fusion vector pMC1069 that had been digested with
HindIII. Amplification and subcloning of the fragment from
pDX101 and pDX103 resulted in plasmids pDX109 and pDX110, respectively.
pDX109 contains plac and the ribosome binding site of
arsA, followed by the drrA gene translationally
coupled to drrB-lacZ fusion, as is seen in the
original operon. The drrA gene, however, is missing from
pDX110.
Analysis of Translational Fusions by -Galactosidase
Assay--
CC118 cells containing pDX109 or pDX110 were grown to
mid-log phase and induced with 1 mM IPTG for 3 h. The
cells were harvested and lysed by a single passage through a French
pressure cell at 20,000 p.s.i. The lysed cells were centrifuged at
10,000 × g for 15 min to remove unbroken cells. 100 µg of protein was then added to a tube containing 0.5 ml of Z buffer
containing 60 mM Na2HPO4, 40 mM NaH2PO4, 10 mM KCl,
1 mM MgSO4, 50 mM
-mercaptoethanol, 200 µl of o-nitrophenyl
-D-galactopyranoside, and the reaction was continued for
5 min. The reaction was stopped with 0.5 ml of 1 M
NaCO3.
-Galactosidase units were calculated as described (6).
Fractionation of the Cells into Cytosolic and Membrane Fractions-- E. coli TG1 cells containing the indicated plasmids were grown to mid-log phase and induced with 0.25 mM IPTG. Growth was continued for an additional 4 h at 37 °C. The cells were spun down and lysed by a single passage through a French pressure cell at 20,000 p.s.i. The cell lysates were centrifuged at 10,000 × g for 10 min to remove the unbroken cells. The supernatant fluids were used to prepare the fractions as described earlier (2). The samples were solubilized in 4× Laemmli sample buffer by heating at 55 °C for 10 min. The proteins were analyzed by SDS-PAGE on 12% polyacrylamide gels, followed by Western blotting as described earlier (1). Quantitation of protein bands on the Western blots was carried out by using the Protein and DNA Imageware densitometric package.
Extraction of the Cell Membrane with Urea-- 300 µg of membrane protein was mixed with the indicated concentrations of urea (pH 8.0) in 1 ml of buffer containing 50 mM Tris-HCl, pH 8.0. The samples were incubated on ice for 30 min. The membranes were separated by centrifugation at 100,000 × g for 1 h and resuspended in 50 mM Tris-HCl, pH 8.0. The samples were solubilized by heating at 55 °C for 10 min. The proteins were analyzed by SDS-PAGE on 12% polyacrylamide gels, followed by Western blotting as described above.
ATP Binding to DrrA--
Photolabeling of
[-32P]ATP to the DrrA protein was carried out by the
procedure described earlier (2, 8). Photolabeling was performed in the
cytosolic and membrane fractions prepared from cells expressing DrrA or
both DrrA and DrrB proteins. The fractions were used directly in
photolabeling experiments at the indicated protein concentrations.
Doxorubicin was added to the reactions where indicated. The samples
were analyzed by SDS-PAGE, followed by autoradiography.
Chemical Cross-linking--
The reaction mixture contained 2.5 mg/ml cell membrane protein in a buffer (100 µl) containing 20 mM sodium phosphate and 150 mM sodium chloride,
pH 7.5. DSP or DTSSP was added at the indicated concentrations, and the
samples were incubated at room temperature for 30 min. The reactions
were quenched by the addition of a solution of 1 M
Tris-HCl, pH 8.0, to a final concentration of 50 mM,
followed by an incubation at room temperature for 15 min. 4× Laemmli
sample buffer (9) prepared without the reducing agent was added, and
the samples were analyzed by SDS-PAGE using a 10% polyacrylamide gel,
followed by Western blot analysis with anti-DrrA or anti-DrrB
antibodies (2). To carry out two-dimensional analysis of the
cross-linked species, a lane from the nonreducing gel was excised and
soaked in the 4× Laemmli sample buffer containing 20%
-mercaptoethanol for 20 min at room temperature. The proteins were
analyzed by placing the excised lane on top of an SDS-10% polyacrylamide gel. The Western blots were probed with antiserum to
DrrB, followed by probing with antiserum to DrrA.
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RESULTS |
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Expression of the DrrA or DrrB ProteinBoth DrrA and DrrB
proteins have previously been shown to be expressed in E. coli upon induction from the lac promoter in pDX101
(Table I). In the present study,
expression of DrrA or DrrB alone was examined in pDX102 and pDX103,
which contain the drrA and drrB gene,
respectively. A schematic representation of these clones is given in
Fig. 1A. The genes cloned in
pDX101, -102, or -103 utilize the lac promoter and the
translational start signals of the arsA gene. pDX101 also contains a putative ribosome binding site (RBS) for drrB,
which is contained within the coding sequence of drrA. In
addition, the region between drrA and drrB (shown
as ATGA in Fig. 1A) shows translational coupling such that
the stop codon of drrA overlaps with the start codon of
drrB. Translational coupling is absent in pDX103.
drrB in pDX103 lacks its own putative RBS, and it utilizes the RBS of arsA. E. coli TG1 cells containing the
indicated plasmids were induced with IPTG, and samples were collected
after 3 h of induction. The cells were fractionated into cytosolic
and total membrane fractions. The fractions were analyzed by Western
blotting using anti-DrrA or anti-DrrB serum (Fig. 1B), and
the intensities of the bands were determined by densitometric analysis.
Western blot analysis using anti-DrrA serum suggested that DrrA is
expressed both in pDX101- and pDx102-containing cells; however, the
level of expression in pDX102 (Fig. 1B, a,
lanes 1 and 2) was lower than in
pDX101 (Fig. 1B, a, lanes 3 and 4). Densitometric analysis suggested that the total
level of DrrA in pDX102 was about 70% that of in pDX101. However, in
both situations, i.e. in the presence or the absence of
DrrB, roughly 60% DrrA was membrane-associated. A band of faster
mobility than DrrA that reacts with anti-DrrA antibody (Fig.
1B, a) is unrelated to DrrA, since this band is also observed in the control samples that do not contain either DrrA or
DrrB (2).
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Analysis by Western blotting using anti-DrrB serum suggested that DrrB
is present only in pDX101-containing cells (Fig. 1B, b, lanes 3 and 4). Little
if any DrrB could be detected in the membrane fraction prepared from
cells containing pDX103 (Fig. 1B, b,
lanes 1 and 2). To determine if the
expression of DrrB in pDX101 is the result of translational coupling
with DrrA and the absence of DrrB in pDX103 is a result of the absence
thereof, a translational fusion of the first 15 amino acids of DrrB
with -galactosidase was created. Using pDX101 or pDX103 as a
template, the region starting at the promoter plac and
ending with the 45th nucleotide of drrB was amplified by
polymerase chain reaction, and the amplified fragment was fused to the
eighth codon of
-galactosidase. Two clones resulting from this (Fig.
2), one (pDX109) containing the
drrA gene in cis and the other without (pDX110),
were tested for
-galactosidase activity. The data in Fig. 2 indicate
that drrB in pDX110 can be translated, although the
-galactosidase activity in pDX109, where drrA is present
in cis, was about 2-fold higher as compared with pDX110.
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Since DrrB is translated in the absence of coupled translation with DrrA, but not detected in these cells by Western blot analysis (Fig. 1), we wanted to determine if maintenance of DrrB in the cell depends on simultaneous expression of DrrA. E. coli TG1 cells containing pDX103 were co-transformed with a compatible plasmid pDX108 containing the drrA gene. pDX108 contains the drrA gene in pUC18 and, as in pDX101-pDX103, uses the translational start signals of arsA (Table I and Fig. 1). After induction of the drrA and drrB genes with IPTG, total cell lysates were analyzed for the presence of DrrA and DrrB proteins. Data in Fig. 3 show that the expression of DrrB from pDX103 is restored in cells containing DrrA in trans. The amount of DrrB protein detected was roughly the same whether the drrA gene was present in cis (pDX101-containing cells; lane 4) or in trans (pDX103 and pDX108; lane 5), indicating that the presence of the DrrA protein is required for maintenance of DrrB in the cell. As is also seen in Fig. 1, the level of DrrA in pDX102-containing cells was lower (Fig. 3, lane 2) as compared with pDX101-containing cells (Fig. 3, lane 4). However, expression of DrrA in pDX108 (lane 1) results in the same level of DrrA protein as in pDX101 (Fig. 3, lane 4). This may be due to the the higher copy number of plasmid pUC18 in pDX108 compared with the plasmid pSU2718 in pDX102. The band at around 29 kDa is the protein reacting nonspecifically with the anti-DrrA antibody, and it is present in all of the samples.
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The chemical nature of the association of DrrA or DrrB to the cell membrane was evaluated by extraction with urea (Fig. 4). About 90% DrrA was still membrane-associated after treatment with 1.5 M urea in both DrrA- and DrrAB-containing membranes (Fig. 4, lanes 2 and 5), whereas it could be completely extracted by 6 M urea in both cases (lanes 3 and 6). DrrB was not affected at all by 6 M urea treatment (Fig. 4), confirming the earlier observation that DrrB is an integral membrane protein, whereas DrrA is peripherally associated with the membrane in both DrrA- or DrrAB-containing cells.
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ATP Binding to DrrA--
It has previously been shown that DrrA
can form a UV-activated adduct with ATP or GTP in a
doxorubicin-dependent manner in total cell lysates
containing both DrrA and DrrB (2). To determine if DrrB affects ATP
binding to DrrA, ATP binding was characterized in the cytosolic and
membrane fractions prepared from E. coli cells containing
pDX101 or pDX102. [-32P]ATP binding in a UV-catalyzed
cross-linking experiment showed that DrrA cross-links to ATP only in
membranes prepared from cells containing both DrrA and DrrB (Fig.
5A, lanes
3 and 4). No ATP cross-linking was seen to DrrA
in membranes containing DrrA alone (Fig. 5A,
lanes 1 and 2). Western blot analysis
of a similar gel using antibodies to DrrA or DrrB showed that DrrA was
present in all samples (Fig. 5B, lanes
1-4), whereas DrrB was present only in lanes
3 and 4 (Fig. 5C). Further, it was
tested whether the soluble fraction of DrrA in cells containing both
DrrA and DrrB can be UV-cross-linked to ATP. Data in Fig.
5A, lanes 5 and 7, show
that the soluble fraction of DrrA in DrrAB-containing cells was also
not in a state competent to cross-link to ATP. Only the membrane bound
form of DrrA in DrrAB-containing cells was competent (Fig.
5A, lanes 6 and 8). Again,
Western blot analysis showed that DrrA was present in both the
cytosolic and the membrane fractions (Fig. 5B,
lanes 5-8), whereas DrrB was present only in the
membrane fractions (Fig. 5C, lanes 6 and 8). Two other species in the membrane-containing
samples, that move with slower mobility compared with DrrA, were also
seen to form a UV-activated adduct with ATP (Fig. 5A,
lanes 1-4, 6, and 8). Both
of these species are unrelated to DrrA and bind ATP irrespective of the presence or absence of DrrB.
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Chemical Cross-linking of DrrA and DrrB in the Cell Membrane-- Chemical cross-linking was carried out in the cell membranes prepared from DrrAB-containing cells. Two different types of cross-linkers were used: the membrane-impermeable cross-linker DTSSP and the membrane-permeable cross-linker DSP. Both DTSSP and DSP can be cleaved in the presence of the reducing agents. Concentrations of the cross-linkers ranging from 50 to 1000 µM were used to determine interaction between DrrA and DrrB. Cross-linking patterns observed with both the cross-linkers were similar (Fig. 6). Upon analysis of the cross-linked membranes under nonreducing gel conditions and Western blot analysis using anti-DrrB antibodies, two cross-linked species were identified (Fig. 6A). Uncross-linked DrrB, a 30.6-kDa protein, migrated at around 25 kDa as has also been reported earlier (2). The molecular mass of one cross-linked species was about 60 kDa (marked with an asterisk). Another cross-linked species of about 120 kDa was also observed (marked with a double asterisk). 60-kDa cross-linked species could be detected at concentrations of both cross-linkers as low as as 50 µM (Fig. 6A, lanes 2 and 9), whereas the 120-kDa species became evident at about 100 µM (lanes 3 and 10). Another species with a mass higher than 200 kDa was also observed (marked with a triple asterisk). This high molecular weight species was more evident at concentrations of the cross-linkers higher than 250 µM (lanes 5-7 and 10-13), and it became the major species at 1 mM of DSP (lane 13) and about 5 mM of DTSSP (lane 7). The cross-linked species were not observed when control membranes, prepared from cells containing just the vector, were treated with the same chemical cross-linkers (data not shown). Upon analysis of a similar gel with anti-DrrA antibodies, the uncross-linked DrrA was seen to migrate at about 36 kDa as expected (Fig. 6B). The 60-kDa cross-linked species, seen in Fig. 6A with anti-DrrB antibody, could be clearly seen to cross-react with the anti-DrrA antibody (Fig. 6B, marked with an asterisk), indicating that this species is a complex containing both DrrA and DrrB. The reaction of the 120-kDa species with the Anti-DrrA antibody was less clear in the first dimension nonreducing gel shown in Fig. 6B. Since DTSSP and DSP are cleavable cross-linkers, two-dimensional analysis of the cross-linked samples under reducing and nonreducing conditions was carried out to further characterize the presence of DrrA and DrrB in these species (Fig. 7). An entire lane corresponding to the sample in lane 11 in Fig. 6 was excised and, after incubation in the presence of the reducing agent as described under "Experimental Procedures," was placed on top of another SDS-polyacrylamide gel and subjected to electrophoresis. Under nonreducing conditions on a two-dimensional gel, the proteins migrate on the diagnol. Upon reduction, the cross-linked species fall off the diagnol, whereas the uncross-linked proteins stay on the diagnol. In Fig. 7, panels A and B show Western blots probed with anti-DrrB antibodies. The gel in panel A is the two-dimensional analysis of the unreduced sample, while the sample in panel B has been reduced. Panels C and D in Fig. 7 are the Western blots in panel A and B, respectively, that have been probed further with anti-DrrA antibodies. Four major spots are seen on the diagnol in A. These spots correspond to the uncross-linked DrrB and the three cross-linked moieties described earlier in Fig. 6. These are again marked with an asterisk (60 kDa), double asterisk (120 kDa), and triple asterisk (the high molecular mass moiety). Probing the same blot with anti-DrrA in C shows an additional spot corresponding to the uncross-linked DrrA. Upon reduction of the proteins, followed by two-dimensional analysis and probing with anti-DrrB, uncross-linked DrrB remained on the diagnol (Fig. 6B). Each of the three cross-linked species was reduced to give a species that migrated with the same mobility as DrrB. To determine if the reduction of these species also resulted in DrrA, the blot in B was probed further with anti-DrrA antibody. The data shown in D indicate that the uncross-linked DrrA stayed on the diagnol; however, reduction of each cross-linked species also generated DrrA in addition to generating DrrB as seen in B.
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DISCUSSION |
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In the present study, expression and function of the DrrA and DrrB
proteins was found to be dependent on each other, resulting in a strong
biochemical coupling. In cells containing the plasmid pDX101, which
contains drrA and drrB genes in cis,
both DrrA and DrrB proteins were detected. Upon subcloning of the
drrA gene separately in pDX102, DrrA was detected but at
levels lower than in pDX101, indicating that DrrB might affect the
expression or stability of DrrA. Effect of DrrA on DrrB expression or
stability, however, was much more dramatic. Subcloning of the
drrB gene alone in pDX103 showed the absence of DrrB protein
(Fig. 1). Since pDX101, -102, and -103 all contain the same promoter,
the regulation of expression of drrB appears to be at the
level of translation or post-translational. DrrA and
drrB in the original operon are translationally coupled so
that the stop codon of drrA overlaps with the start codon of
drrB (Fig. 1). To determine if coupling is essential for
expression of drrB, a translational fusion containing first 15 amino acids of DrrB fused to the eighth codon of -galactosidase was created. Analysis of the fusion indicated that DrrB is translated in the absence of DrrA in pDX110 although at levels lower than in
pDX109 that contains DrrA in cis (Fig. 2). Hence,
translational coupling does not seem to be essential for translation of
DrrB, although it appears to have some role in increasing efficiency of
translation of DrrB in pDX109. Further experiments showed that the
simultaneous expression of DrrA, whether from a gene in cis or in trans, was crucial for stable maintenance of DrrB in
the cell. When drrA and drrB genes were
co-transformed into the same cell on compatible plasmids, DrrB protein,
translated from pDX103, was again detected at the same levels as in
pDX101 (Fig. 3), implying that the regulation is mostly
post-translational. To understand the contribution of translational
coupling in pDX101 and pDX109 toward increased translation of DrrB, it
is important to understand the role of the putative RBS of
drrB. This is presently under investigation; however, it is
clear that drrB is translated in pDX103, but the protein is
not detected in these cells by Western blot analysis. When the
drrA gene is co-transformed into these cells, DrrB is again
detected at the same levels as in pDX101. Hence, there appears to be a
default mechanism by which DrrB is degraded in case DrrA is not
present. Previous studies have demonstrated that overexpression of DrrB
by itself as a translational fusion to ArsD results in inhibition of
cell growth within a few minutes of its induction (2). This could be
due to a leaky membrane resulting from a constitutively open channel
formed by DrrB in the absence of DrrA, which might explain the need for
a default mechanism to degrade DrrB, thus preventing its accumulation.
Experiments are currently under way to determine the mechanism by which
DrrA affects DrrB levels in the cell.
Since we found strong evidence for a very specific interaction between DrrA and DrrB, chemical cross-linking studies were carried out to characterize the interaction further and to determine the stoichiometry of the complex in the membrane. Studies carried out with both a membrane-permeable and a membrane-impermeable cleavable cross-linker showed the presence of two cross-linked species: one species of 60 kDa and another species of 120 kDa. Both species were shown by two-dimensional analysis, after reduction, to consist of both DrrA and DrrB. DrrA migrates as a 36-kDa protein, and DrrB, a 30.6-kDa protein, migrates at roughly 25 kDa; hence, the 60-kDa cross-linked species should correspond to a complex consisting of one subunit of DrrA and one subunit of DrrB, whereas the 120-kDa species probably consists of a complex of two subunits of DrrA and two subunits of DrrB. A cross-linked species with a mass greater than 200 kDa, possibly representing a nonspecific aggregate containing DrrA, DrrB, and other membrane proteins, was also observed; the amount of this species was seen to increase at higher concentrations of the cross-linker until it became the major species at 1 mM. Hence, the formation of the 60-kDa chemically cross-linked species suggests a strong interaction between DrrA and DrrB. Based on the available data, it can also be speculated that the DrrAB complex consists of two subunits of DrrA and two of DrrB. The failure to detect species corresponding to (A)2 or (B)2 might imply that in the Drr complex, DrrA only contacts DrrB and not another subunit of DrrA and that the complex has the arrangement of A1B1A2B2 (Fig. 8), where the superscripts 1 or 2 indicate subunit 1 or subunit 2 within the complex. This would make the DrrAB pump equivalent to Pgp in terms of the number of domains and the overall structure, both containing two nucleotide-binding ABC cassettes and two membrane-spanning domains. The 60-kDa cross-linked species indicates that the closest interaction is between A1 and B1 or between A2 and B2. Within the arrangement A1B1A2B2, the species A1B1A2 and B1A2B2 would also be expected upon cross-linking, but these species were not detected, perhaps because a cross-link between B1 and A2 results in the 120-kDa species A1B1A2B2 instead of A1B1A2 or B1A2B2 due to the close proximity of A1 and B1 or A2 and B2.
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Interaction between subunits of transport complexes has been reported
(10); however, such a tight regulation of expression and function as
seen in the DrrAB system has not been observed before. It has generally
been observed that the prokaryotic transport systems exist as complexes
consisting of subunits that are encoded by genes within an operon,
whereas the eukaryotic transporters occur as single large proteins that
contain multiple domains. DrrAB, a typical prokaryotic transporter,
consists of two separately expressed subunits; however, the subunits
are tightly coupled and appear to behave like the domains of a single
protein. In addition to DrrA regulating the stability or membrane
insertion of DrrB, the function of DrrA itself was found to be
dependent upon its interaction with DrrB. DrrA has previously been
shown to be an ATP/GTP-binding protein (2). In the present study, we
have shown that no ATP cross-linking to DrrA was seen in the cytoplasmic or membrane-bound form of DrrA in cells containing only
DrrA. Further, ATP cross-linking to DrrA was seen only in the
membrane-bound fraction of DrrA in DrrAB-containing cells (Fig. 5).
These data suggest that it is the specific interaction between DrrA and
DrrB in the membrane that introduces a conformational change in the ATP
binding site of DrrA. Hence, although DrrA is tightly associated with
the membrane in the absence of DrrB (Fig. 4), it is not in an active
conformation. Hence, the ability of DrrB to be stably maintained in the
cell and/or inserted into the membrane depends on DrrA, and the ability
of DrrA to bind and/or hydrolyze ATP depends on the presence of DrrB in
the membrane. In this respect, the DrrAB complex is a novel ABC
transporter, where two components assist each other in a stepwise
manner. Based on the data presented in this paper, we propose that DrrA
is an allosteric protein that goes through different conformations
depending on the presence or absence of DrrB and the ligand doxorubicin (Fig. 8). The DrrB protein is shown as consisting of seven
transmembrane -helices based on preliminary analysis of gene fusions
with alkaline phosphatase and
-galactosidase.2 In its
uncomplexed state, DrrA is in conformation I, which is inactive in
terms of its ability to UV-cross-link with ATP. Interaction with DrrB
results in maintenance of DrrB in the cell membrane, and this
interaction introduces a conformational change in the active site of
DrrA, which is shown as conformation II. Active conformation of DrrA,
depicted as conformation III, can be achieved via conformation II upon
the addition of doxorubicin. It is in this conformation that DrrA is
able to form the UV-activated cross-link with ATP (Figs. 2 and 5).
A better understanding of how DrrA and DrrB interact would undoubtedly lead to a better understanding of how domains within Pgp might interact and stabilize each other and how energy might be transduced between the catalytic ABC domain and the membrane-spanning domain of Pgp. This has implications for understanding the evolution of multidomain proteins found primarily in eukaryotic cells.
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ACKNOWLEDGEMENT |
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Thanks are due to P. C. Tai for helpful discussions during preparation of the manuscript.
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FOOTNOTES |
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* This work was supported by the National Institutes of Health Research Service Award R29 GM51981-02.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed: Dept. of Biology, 24 Peachtree Center Ave., Georgia State University, Atlanta, GA 30303. Tel.: 404-651-3864; Fax: 404-651-2509; E-mail:
bioppk{at}panther.gsu.edu.
1
The abbreviations used are: Pgp, P-glycoprotein;
PAGE, polyacrylamide gel electrophoresis; IPTG,
isopropyl-1-thio--D-galactopyranoside; DSP,
dithiobis(succinimidyl propionate); DTSSP,
dithiobis(sulfosuccinimidyl propionate).
2 P. Kaur and J. Levine, unpublished data.
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