Department of Chemistry and Biochemistry,
Utah State University, Logan, Utah 84322-0300
The metabolism of aliphatic epoxides (epoxyalkanes) by the
alkene-utilizing actinomycete Nocardia corallina B276 was
investigated. Suspensions of N. corallina cells grown with
propylene as the carbon source readily degraded propylene and
epoxypropane, while suspensions of glucose-grown cells did not. The
addition of propylene and epoxypropane to glucose-grown cells resulted
in a time-dependent increase in propylene- and epoxypropane-degrading
activities that was prevented by the addition of rifampin and
chloramphenicol. The expression of alkene- and epoxide-degrading
activities was correlated with the high-level expression of several
polypeptides not present in extracts of glucose-grown cells.
Epoxypropane and epoxybutane degradation by propylene-grown cell
suspensions of N. corallina was stimulated by the addition
of CO2 and inhibited by the depletion of CO2.
Cell extracts catalyzed the carboxylation of epoxypropane to form
acetoacetate in a reaction that was dependent on the addition of
CO2, NAD+, and a reductant (NADPH or
dithiothreitol). In the absence of CO2, epoxypropane was
isomerized by cell extracts to form acetone at a rate approximately
10-fold lower than the rate of epoxypropane carboxylation.
Methylepoxypropane was found to be a time-dependent, irreversible
inactivator of epoxyalkane-degrading activity. These properties
demonstrate that epoxyalkane metabolism in N. corallina occurs by a carboxylation reaction forming 
-keto acids as products and provide evidence for the involvement in this reaction of an epoxide
carboxylase with properties and cofactor requirements similar to those
of the four-component epoxide carboxylase enzyme system of the
gram-negative bacterium Xanthobacter strain Py2 (J. R. Allen and S. A. Ensign, J. Biol. Chem. 272:32121-32128, 1997). The addition of epoxide carboxylase component I from
Xanthobacter strain Py2 to methylepoxypropane-inactivated
N. corallina extracts restored epoxide carboxylase
activity, and the addition of epoxide carboxylase component II from
Xanthobacter Py2 to active N. corallina extracts stimulated epoxide isomerase rates to the same levels observed
with the purified Xanthobacter system. Antibodies raised against Xanthobacter strain Py2 epoxide carboxylase
component I cross-reacted with a polypeptide in propylene-grown
N. corallina extracts with the same molecular weight as
component I but did not cross-react with glucose-grown extracts.
Together, these results suggest a common pathway of epoxyalkane
metabolism for phylogenetically distinct bacteria that involves
CO2 fixation and the activity of a multicomponent epoxide
carboxylase enzyme system.
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INTRODUCTION |
Several bacteria, including some
strains of Mycobacterium, Xanthobacter, and
Nocardia species, are capable of growth with aliphatic
alkenes as carbon and energy sources (8, 9, 20). The pathway
for alkene metabolism in these organisms involves an initial
monooxygenase-catalyzed reaction producing epoxide intermediates, as
illustrated for the substrate propylene and the product epoxypropane in
equation 1:
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(1)
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While the monooxygenase-catalyzed epoxidation of aliphatic alkenes
is a well-characterized reaction (13, 17), less is known
about the subsequent metabolism of the epoxide intermediates thus
formed. The only characterized pathway for an
aliphatic-alkene-utilizing bacterium is that of Xanthobacter
strain Py2. In this bacterium, epoxides are further metabolized via a
novel ring-opening and carboxylation reaction that requires
CO2 as a cosubstrate and forms -keto acids as products
(1, 18). Epoxide carboxylase, the enzyme catalyzing this
reaction, requires an oxidant (NAD+) and a reductant (NADPH
or a dithiol) (21), which are reduced and oxidized in the
course of epoxide carboxylation as illustrated in equation 2 (3):
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(2)
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The epoxide carboxylase complex from Xanthobacter
strain Py2 has recently been purified and found to consist of four
separate proteins (3): component I, a homohexameric protein
(41.7-kDa subunits) that is believed to contain the epoxide binding
and/or activation site(s); component II, a dimeric flavoprotein (57-kDa subunits) identified as an NADPH:disulfide oxidoreductase which is
proposed to generate a reduced thiol(s) essential for catalysis (19); component III, a dimeric protein (26- and 26.2-kDa
subunits) with an unidentified catalytic role; and component IV, a
homodimeric protein (25.4-kDa subunits) which also has an unidentified
catalytic role (3). The mechanistic details involving the
interplay of the above-mentioned protein components and cofactors of
this complex enzyme have not been elucidated. A preliminary mechanism
involving a reductive epoxide ring-opening step, which is followed by
an NAD+-dependent oxidation step prior to product release,
has been proposed (21). Interestingly, in the absence of
CO2, epoxide carboxylase catalyzes the isomerization of
aliphatic epoxides to form ketones, although this reaction is
apparently of no physiological significance (15, 16). This
isomerase activity is, however, relevant to the catalytic mechanism
since it demonstrates that a reaction intermediate can alternatively
undergo carboxylation to form a -keto acid or protonation to form a
ketone.
Epoxide carboxylation represents a new and novel strategy for
biological epoxide activation and transformations. To date, it is the
only strategy that has been identified for aliphatic epoxide metabolism
by the class of bacteria that grow with short-chain aliphatic alkenes
as carbon and energy sources. The question of whether epoxide
carboxylation is the predominant strategy used to metabolize epoxides
in aliphatic-alkene-utilizing bacteria or whether other characterized
transformations (i.e., isomerization [10, 14] or
hydration [5, 11]) are utilized as well has been
raised. One organism that may aid in addressing this question is the
gram-positive bacterium Nocardia corallina B276. This
bacterium, isolated with propylene as the source of carbon and energy
(8), has been reported to convert 1-alkenes ranging from
C2 to C18 in chain length to 1-epoxides, as
well as to convert styrene to styrene oxide (7). The alkene
monooxygenase which catalyzes these reactions has recently been
isolated and shown to be a multiprotein enzyme system (13).
However, the pathway(s) by which epoxides are further metabolized in
N. corallina B276 has not been studied.
In the present paper, evidence that epoxides are metabolized in a
CO2-dependent manner in N. corallina, similar to
that described for Xanthobacter strain Py2, is presented.
The reaction requirements and enzymes involved in epoxide carboxylation
in N. corallina B276 are described and compared to those of
the epoxide carboxylase reaction of Xanthobacter strain Py2.
The similarities and differences between these two epoxide
carboxylation systems are of interest in the ongoing effort to gain
insight into microbial strategies for the metabolism of epoxides.
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MATERIALS AND METHODS |
Chemicals.
Tris(hydroxymethyl)aminomethane (Tris) buffer was
purchased from Sigma Chemical Co. Horseradish peroxidase color
development reagent and a goat anti-rabbit immunoglobulin G-horseradish
peroxidase conjugate were purchased from Bio-Rad. Epoxypropane (99%
minimum) and 1,2-epoxybutane (99% minimum) were purchased from Aldrich Chemical Co. Methylepoxypropane was purchased from Lancaster
Laboratories.
Growth of bacteria and preparation of cell suspensions.
Cultures of N. corallina B276 (ATCC 31338) were grown in
sealed 4-liter shake flasks containing 0.8 liter of mineral salts medium (1) with propylene (10% [vol/vol] gas phase) or
glucose (10 g/liter) as the carbon source. Cultures were harvested at an A600 of between 1.0 and 3.0 by centrifugation
and washed in buffer (50 mM potassium phosphate, pH 7.2) as described
previously (1). Cultures of Xanthobacter strain
Py2 were grown on propylene (10% [vol/vol] gas phase) or glucose (10 g/liter) as the carbon source and harvested as previously described
(1). Cell pastes were stored at 
80°C.
Assay of epoxide degradation activity in whole-cell
suspensions.
Assays of epoxyalkane degradation by whole-cell
suspensions of N. corallina were performed with shaking at
30°C in sealed 9-ml serum vials containing cells, substrate (2 µmol), and buffer (50 mM potassium phosphate, pH 7.2) in a total
volume of 1 ml (18). For whole-cell assays performed in the
absence of CO2, residual CO2 was removed by
sparging buffers and flushing sealed vials with CO2-free
nitrogen and including a KOH-saturated filter trap in each of the
vials.
Preparation of cell extracts and purified epoxide carboxylase
components.
Frozen cell paste (15 to 30 g) of N. corallina or Xanthobacter strain Py2 was thawed and
resuspended in 2 volumes of buffer (50 mM Tris-HCl [pH 8.2]
containing 1 mM dithiothreitol [DTT], 10% [vol/vol] glycerol,
DNase I [0.2 mg/ml], and lysozyme [0.3 mg/ml]). The cell suspension
was passed four times through a French pressure cell at 110,000 kDa,
and the lysate was clarified by centrifugation at 137,000 × g for 30 min at 4°C. After removal of cell debris, the
supernatant was dialyzed for 16 h at 4°C against buffer (50 mM
Tris-HCl [pH 8.2] containing 10% [vol/vol] glycerol). The
dialysate was stored at 80°C and used as the source of enzyme. Methylepoxypropane-treated cell extracts of N. corallina and
Xanthobacter strain Py2 were prepared by a method described
previously (2). Purified epoxide carboxylase components I to
IV from Xanthobacter strain Py2 were prepared as previously
described (2, 3).
Assay of epoxide carboxylase activity in cell extracts.
Epoxide carboxylase activity was measured by monitoring the
time-dependent depletion of epoxypropane by gas chromatography as
described previously (1). Assays were performed in sealed 9-ml serum vials containing a source of enzyme (cell extract alone or
cell extract plus purified epoxide carboxylase components), in 50 mM
Tris-HCl (pH 8.2) containing 10% glycerol, using reagents and reaction
conditions described previously (1, 2). For assays performed
in the absence of CO2, CO2 was removed as
described above. Acetoacetate, acetone, and 1,2-epoxybutane were
quantified by gas chromatography as previously described
(1). Products of epoxyalkane carboxylation were also
identified by using 13C-enriched NaHCO3 in the
assay mix and analyzing the reaction products by proton-decoupled
13C nuclear magnetic resonance spectrometry (NMR) as
described previously (1).
Induction of epoxypropane-degrading activity in batch cultures.
N. corallina cells which had been grown for several
generations with either glucose or propylene as the carbon source were used for induction experiments as previously described (6).
SDS-PAGE and immunoblotting procedures.
Sodium dodecyl
sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) (12% total
gel; 2.7% cross-linker running gel) was performed in a Mini-Protean II
apparatus (Bio-Rad) by the Laemmli procedure (12).
Electrophoresed proteins were visualized by Coomassie blue staining.
Apparent molecular masses of polypeptides were determined by comparison
with the Rf values for molecular mass standard
proteins. The standards were bovine serum albumin (66.2 kDa), ovalbumin
(45 kDa), carbonic anhydrase (31 kDa), and cytochrome c
(12.3 kDa). Immunoblot analysis was conducted as described previously, using a polyclonal antiserum raised against Xanthobacter
strain Py2 epoxide carboxylase component I or epoxide carboxylase
component II (2).
Protein determination.
Protein concentrations were
determined by a modified biuret assay with bovine serum albumin as the
standard (4). The protein concentration of epoxide
carboxylase component II from Xanthobacter strain Py2 was
routinely determined by using its reported extinction coefficient
(2).
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RESULTS |
CO2-dependent epoxide degradation in whole-cell
suspensions of N. corallina B276.
While the oxidation
of aliphatic alkenes to epoxides is a well-characterized reaction in
N. corallina (8, 13), the pathway by which
epoxides are further converted to central metabolites has not been
investigated. As an initial step in characterizing the
epoxide-converting reaction, the degradation of two aliphatic epoxides,
epoxypropane and 1,2-epoxybutane, was investigated using whole-cell
suspensions of propylene-grown N. corallina. As shown in
Fig. 1, both epoxides were degraded in
the presence of CO2 and bicarbonate but not in their
absence. These results suggest a role for CO2 as a
cosubstrate in epoxide degradation similar to that identified in
Xanthobacter strain Py2; i.e., aliphatic epoxides are
carboxylated to form the corresponding -keto acids. Interestingly,
in the absence of CO2, cell suspensions and cell extracts
of propylene-grown Xanthobacter cells catalyze the
isomerization of aliphatic epoxides to form the corresponding ketones
(acetone in the case of epoxypropane isomerization; methyl ethyl ketone in the case of 1,2-epoxybutane isomerization) at rates approximately 40% lower than those observed for epoxide carboxylation (1, 18). This epoxide isomerization has been proposed to be a
fortuitous reaction of no physiological importance (16). To
determine whether a similar CO2-dependent isomerization of
epoxides occurs in N. corallina, the rates of epoxypropane
and 1,2-epoxybutane degradation were measured in the absence of
CO2. As shown in Fig. 1, no significant degradation of
either substrate was observed during the time frame of these assays.
These results suggest either that the epoxide-converting enzyme of
N. corallina does not catalyze epoxide to ketone
isomerization or that the rate of isomerization, relative to that of
carboxylation, is much lower than that in the corresponding
Xanthobacter enzyme system.
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FIG. 1.
Requirement of CO2 for epoxyalkane
degradation by propylene-grown N. corallina. Assays were
performed with whole-cell suspensions (0.5 mg of protein). Closed
symbols, assays performed with CO2 and NaHCO3
(50 mM combined concentration); open symbols, assays performed without
CO2 and NaHCO3; squares, epoxypropane
remaining; circles, 1,2-epoxybutane remaining.
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Carboxylation of epoxides to -keto acids in cell extracts of
N. corallina.
As mentioned in the introduction and shown in
equation 2, epoxide carboxylase from Xanthobacter strain Py2
couples the carboxylation of epoxyalkanes to the transhydrogenation of
NAD+ and NADPH. While NADPH is believed to be the
physiological reductant for the reaction, dithiols (e.g., DTT) are
capable of substituting for NADPH. With these requirements in mind, the
in vitro degradation of epoxypropane and epoxybutane in cell extracts
of N. corallina was investigated. As observed for extracts
of Xanthobacter strain Py2 (1, 21), a
time-dependent consumption of epoxypropane or 1,2-epoxybutane was
observed in assay mixtures that contained CO2,
NAD+, and either NADPH or DTT. In the absence of both NADPH
(or DTT) and NAD+, or in the individual absence of either
reductant or oxidant, the rates of epoxyalkane degradation were
approximately five- to sevenfold lower at the outset of the assays and
decreased during the course of the assays. These results suggest that
epoxide degradation in N. corallina is coupled to the
transhydrogenation of NAD+ and NADPH, as has been
previously shown to occur for the epoxide carboxylase system of
Xanthobacter strain Py2 (3). To identify the
products of epoxyalkane degradation, assays were performed with cell
extract in the presence of NaH13CO3 and the
reaction products were analyzed by 13C NMR. The
13C NMR spectrum of the reaction products formed on
complete consumption of epoxypropane and 1,2-epoxybutane showed
resonance peaks with chemical shifts identical to the C-1 (carboxyl)
carbon atoms of acetoacetate and 3-keto-pentanoic acid, respectively
(data not shown).
As mentioned above, in the absence of CO2, cell suspensions
and extracts of propylene-grown Xanthobacter strain Py2
catalyze the isomerization of epoxides to form ketones at rates
approximately 1.5- to 2-fold lower than those observed for
carboxylation (1, 18). Epoxide isomerization requires the
same cofactors (NAD+ and either NADPH or DTT) as epoxide
carboxylation. The effect of CO2 on epoxide degradation was
investigated in cell extracts of N. corallina to determine
whether any isomerase activity could be detected in vitro and, if so,
how the rate of isomerization compared to the rate of carboxylation. As
shown in Fig. 2, in the presence of
CO2, the time course of epoxypropane consumption was
stoichiometric with the time course of acetoacetate formation. In the
absence of CO2, a 10-fold-lower rate of epoxypropane
degradation was observed, and epoxypropane consumption correlated with
the stoichiometric formation of acetone (Fig. 2). Similar results were
obtained when NADPH, rather than DTT, was used as the reductant in the
assays. These results demonstrate that the epoxide carboxylase of
N. corallina is capable of catalyzing epoxide to ketone
isomerization, albeit at a much slower rate, relative to epoxide
carboxylation, than the epoxide carboxylase from
Xanthobacter strain Py2.
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FIG. 2.
Effect of CO2 on the time courses of
epoxypropane degradation and acetoacetate formation catalyzed by cell
extracts of N. corallina. Assays were performed with 7.5 mg
of cell extract. Closed symbols, assays performed with CO2
and NaHCO3 (60 mM); open symbols, assays performed without
CO2 and NaHCO3; squares, epoxypropane
remaining; circles, acetoacetate formed; triangles, acetone formed.
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Induction of epoxide-degrading activity in N. corallina
and identification of inducible polypeptides.
The alkene
monooxygenase and epoxide carboxylase enzymes in
Xanthobacter strain Py2 are inducible proteins that are not
expressed in cultures grown on other carbon sources, such as glucose or acetone (6, 16, 18). Induction of alkene monooxygenase and
epoxide carboxylase activities by the addition of alkenes or epoxides
to glucose-grown Xanthobacter strain Py2 results in the de
novo synthesis of new polypeptides, several of which are expressed at
high levels and are hence readily visible on SDS-PAGE gels of cell
extracts (6). Several of these polypeptides represent components of the alkene monooxygenase and epoxide carboxylase enzymes.
For example, the polypeptides constituting epoxide carboxylase components I (42 kDa) and II (57 kDa) and two subunits of the three-subunit alkene monooxygenase (the 43- and 53-kDa subunits) are
readily visible in gels of cell extracts (2, 6, 17). To
obtain more information about similarities and possible differences between the Xanthobacter and N. corallina epoxide
carboxylases, we investigated whether the alkene- and epoxide-degrading
enzymes of N. corallina were similarly induced and, if so,
whether similar patterns of polypeptides could be observed in induced
cells.
To investigate the inducible nature of the N. corallina
system, batch cultures were grown with either glucose or propylene as
the carbon source and then transferred to serum bottles to which
propylene or epoxypropane was added. The time courses of substrate
disappearance in the bottles were used as a measure of the presence
and/or induction of alkene- and epoxide-degrading activities. As shown
in Fig. 3, the bacterial cells from
cultures grown with propylene as the carbon source rapidly degraded
propylene (Fig. 3A) or epoxypropane (Fig. 3B) from the outset of the
assays. The rates of propylene and epoxypropane degradation by these
cells were not affected by the addition of rifampin and
chloramphenicol. In contrast, the cells from cultures grown on glucose
did not degrade propylene or epoxypropane to any noticeable degree
within the first 100 min of incubation, during which time
propylene-grown cells had consumed nearly all of the propylene or
epoxypropane added to these assay mixtures (Fig. 3). After this initial
lag period, the propylene and epoxypropane began to disappear, and the
rates of propylene and epoxypropane depletion increased over time. In
contrast, no significant propylene or epoxypropane degradation was
observed when rifampin and chloramphenicol were added to the glucose-grown cells (Fig. 3). These data demonstrate that the alkene
monooxygenase and epoxide carboxylase enzymes in N. corallina are repressed in cultures grown on glucose as the carbon
source and induced by the addition of propylene or epoxypropane.
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FIG. 3.
Requirement of new protein synthesis for the degradation
of propylene and epoxypropane by N. corallina grown with
glucose as the carbon source. Assays were conducted in 150-ml serum
bottles containing 15 ml of glucose-grown cells
(A600 = 1.47) or propylene-grown cells
(A600 = 0.93) that had been transferred from
200-ml cultures grown in shake flasks. Closed symbols, assay bottles
containing chloramphenicol (10 mg) and rifampin (5 mg); open symbols,
assay bottles without chloramphenicol or rifampin present; circles,
propylene-grown cells; squares, glucose-grown cells. (A) Propylene
remaining; (B) epoxypropane remaining.
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The polypeptide banding patterns of cell extracts prepared from
glucose-grown (noninduced) and propylene-grown (induced) cultures of
Xanthobacter strain Py2 and N. corallina are
presented in Fig. 4. As observed for
Xanthobacter strain Py2, unique polypeptides not visible in
glucose-grown cells are readily visible in propylene-grown N. corallina cells. Presumably, some or all of these polypeptides represent subunits of the alkene monooxygenase and epoxide carboxylase enzymes. The alkene monooxygenase from N. corallina was
recently purified and found to consist of three separate components: a monomeric reductase (40 kDa), a monomeric small effector protein (14 kDa), and a heterodimeric oxygenase (35- and 53-kDa subunits) (13). Based on the purification schemes for the three
proteins, it can be concluded that the reductase and small protein are
expressed at relatively low levels and would not be easily visualized
in extracts run on SDS-PAGE gels (13). In contrast, the
oxygenase would be expected to constitute approximately 3% of the
soluble cell protein (13). Inducible polypeptides with
apparent molecular masses of 35 and 53 kDa are present in the cell
extract of propylene-grown N. corallina (Fig. 4); these
polypeptides could conceivably represent the two oxygenase subunits.
The most highly induced proteins in propylene-grown N. corallina extracts have apparent molecular masses of 42 and 59 kDa
on SDS-PAGE (Fig. 4). Clearly, these polypeptides are not associated
with the alkene monooxygenase and may be components of the epoxide
carboxylase. The relative abundance and apparent molecular masses of
these polypeptides are similar to those of components I (42 kDa on
SDS-PAGE) and II (57 kDa on SDS-PAGE) of the epoxide carboxylase
complex from Xanthobacter strain Py2 (Fig. 4).
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FIG. 4.
Gel electrophoretic analysis of propylene-induced
polypeptides in N. corallina and comparison to purified
epoxide carboxylase components (comp.) I and II from
Xanthobacter strain Py2. Lane 1, molecular mass standards (2 µg each); lane 2, epoxide carboxylase component I from
Xanthobacter strain Py2 (3 µg); lane 3, epoxide
carboxylase component II from Xanthobacter strain Py2 (3 µg); lane 4, glucose-grown cell extract from Xanthobacter
strain Py2 (25 µg); lane 5, propylene-grown cell extract from
Xanthobacter strain Py2 (25 µg); lane 6, glucose-grown
cell extract from N. corallina (25 µg); lane 7, propylene-grown cell extract from N. corallina (25 µg);
lane 8, epoxide carboxylase components I (3 µg) and II (3 µg) from
Xanthobacter strain Py2.
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Immunoblot analysis of glucose- and propylene-grown N. corallina cell extracts.
The polypeptides in glucose- and
propylene-grown N. corallina cell extracts were analyzed by
immunoblotting with polyclonal antibodies raised against purified
epoxide carboxylase components I and II from Xanthobacter
strain Py2 to determine whether there is any cross-antigenicity between
these proteins. Antibodies raised against epoxide carboxylase component
I from Xanthobacter strain Py2 cross-reacted weakly with a
protein, present in cell extracts of propylene-grown N. corallina B276 cells, that migrated on SDS-PAGE with the same
apparent molecular mass as the 42-kDa inducible polypeptide (Fig.
5A). Cross-reaction to a lesser degree
was observed at this same position in cell extracts of glucose-grown
N. corallina. Antibodies raised against purified epoxide
carboxylase component II from Xanthobacter strain Py2
cross-reacted with a protein, present in both glucose- and
propylene-grown N. corallina cell extracts, that migrated on
SDS-PAGE with an apparent molecular mass of 37 kDa but did not
cross-react with the 59-kDa inducible polypeptide (Fig. 5B).
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FIG. 5.
Immunoblot analysis of glucose- and propylene-grown cell
extracts of N. corallina. (A) Immunoblot prepared using
antibodies raised against epoxide carboxylase component I from
Xanthobacter strain Py2 as the probe. The arrow indicates
the position of component I. Lanes 1 and 6, epoxide carboxylase
component I from Xanthobacter strain Py2 (0.5 µg); lane 2, glucose-grown cell extract from Xanthobacter strain Py2 (15 µg); lane 3, propylene-grown cell extract from
Xanthobacter strain Py2 (15 µg); lane 4, glucose-grown
cell extract from N. corallina (15 µg); lane 5, propylene-grown cell extract from N. corallina (15 µg).
(B) Immunoblot prepared using antibodies raised against epoxide
carboxylase component II from Xanthobacter strain Py2 as the
probe. The arrow indicates the position of component II. Lane 1, glucose-grown cell extract from N. corallina (15 µg); lane
2, propylene-grown cell extract from N. corallina (15 µg);
lane 3, epoxide carboxylase component II from Xanthobacter
strain Py2 (0.5 µg).
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Inhibition of epoxide carboxylase activity in N. corallina by methylepoxypropane.
As mentioned in the
introduction, epoxide carboxylase from Xanthobacter Py2 is a
multiprotein enzyme complex consisting of four separate proteins that
are required for epoxide carboxylation or isomerization (3).
Since epoxide carboxylation in cell extracts of N. corallina
has cofactor requirements identical to those of the
Xanthobacter strain Py2 epoxide carboxylase, it would be
reasonable to speculate that N. corallina epoxide
carboxylase functions as a multiprotein complex as well. One
mechanistic probe that might prove useful in addressing this question
is the substrate analog methylepoxypropane, which has previously been
characterized as a time-dependent, irreversible inactivator of epoxide
carboxylase from Xanthobacter strain Py2 (2).
Methylepoxypropane differs from epoxypropane in the presence of a
methyl group rather than a hydrogen substituent on the C-2 carbon atom.
Epoxide carboxylation (or isomerization) requires the abstraction of
hydrogen, possibly as a hydride, from the C-2 carbon and the formation
of a carbonyl carbon at this center (21). Methylepoxypropane
is proposed to undergo a covalent reaction with the catalytic,
active-site-containing component of epoxide carboxylase but, due to the
lack of an abstractable hydride, not to react further to form a product
(2). The addition of epoxide carboxylase component I, but
not that of component II, III, or IV, to methylepoxypropane-inactivated
cell extracts of Xanthobacter strain Py2 restored epoxide
carboxylase activity, demonstrating that component I is the specific
target of inactivation and suggesting that it contains the epoxide
binding and/or activation site(s) (3).
The possibility that methylepoxypropane would serve as an inactivator
of epoxide carboxylase activity in N. corallina was investigated by monitoring the degradation of epoxypropane in assay
mixtures that contained various concentrations of methylepoxypropane. As shown in Fig. 6, the presence of
methylepoxypropane resulted in the concentration- and time-dependent
inhibition of epoxide carboxylase activity in N. corallina
cell suspensions. No recovery of epoxide carboxylase activity was
observed after removal of methylepoxypropane (data not shown),
demonstrating that the inhibition is essentially irreversible.
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FIG. 6.
Concentration- and time-dependent inactivation of
epoxide carboxylase in whole-cell suspensions of N. corallina by methylepoxypropane. Each assay mixture contained cell
suspension (0.35 mg of protein) and CO2 and
NaHCO3 (50 mM total). Assays were initiated by the addition
of 2 µmol of epoxypropane. Symbols:  , no methylepoxypropane;  ,
0.5 mM methylepoxypropane;  , 1 mM methylepoxypropane;  , 2 mM
methylepoxypropane;  , 4 mM methylepoxypropane.
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Restoration of epoxide carboxylase activity in
methylepoxypropane-treated N. corallina cell extract by
Xanthobacter strain Py2 component I.
As shown in Fig.
7A, the addition of
Xanthobacter epoxide carboxylase component I to
methylepoxypropane-inactivated N. corallina cell extract
restored epoxide carboxylase activity in a concentration-dependent fashion. The addition of Xanthobacter epoxide carboxylase
component II, III, or IV up to the highest amount of component I added
(1.1 mg) had no effect on activity (data not shown). Importantly,
purified component I did not display epoxide carboxylase activity alone (in the absence of methylepoxypropane-inactivated N. corallina cell extract) or in the presence of N. corallina glucose-grown cell extracts (data not shown). These
results demonstrate that the combination of Xanthobacter
epoxide carboxylase component I with active N. corallina
epoxide carboxylase components provides a heterologous system capable
of catalyzing epoxide carboxylation. These results also demonstrate
that an N. corallina protein with functions similar to that
of Xanthobacter component I is the specific target of
methylepoxypropane inactivation.
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FIG. 7.
Restoration of epoxide carboxylase activity in
methylepoxypropane-treated cell extracts of N. corallina by
addition of epoxide carboxylase component I from
Xanthobacter strain Py2. Symbols: , assays performed with
CO2 and NaHCO3 (60 mM);  , assays performed
without CO2 and NaHCO3. (A) Assays of cell
extract (4.8 mg) prepared from methylepoxypropane-treated N. corallina; (B) assays of cell extract (5.4 mg) prepared from
methylepoxypropane-treated Xanthobacter strain Py2.
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|
As mentioned earlier, there is a significant difference in the relative
rates of epoxide carboxylation and isomerization catalyzed by the
Xanthobacter (1.5- to 2-fold-lower isomerase rate) and N. corallina (10-fold-lower isomerase rate) epoxide
carboxylases. Possibly, component I in Xanthobacter strain
Py2 and the analogous methylepoxypropane-sensitive protein in N. corallina are the determinants in this rate difference. To
investigate this, the rates of epoxypropane degradation in
methylepoxypropane-treated N. corallina cell extracts complemented with Xanthobacter component I were measured in
the absence of CO2. As shown in Fig. 7A, the addition of
component I did not stimulate the rate of CO2-independent
epoxide degradation (indicative of isomerase activity). As a control,
the rate of epoxypropane degradation in assay mixtures containing the
homologous combination of Xanthobacter component I and
methylepoxypropane-inactivated Xanthobacter cell extract was
measured in the absence and presence of CO2, and the
expected relative ratio of isomerase activity to carboxylase activity
was found (Fig. 7B). These results suggest that Xanthobacter
component I is not the sole determinant in the ratio of isomerase and
carboxylase activities catalyzed by the multiprotein enzyme.
Xanthobacter strain Py2 component II confers epoxide
isomerase activity in cell extracts of N. corallina.
The
difference in the relative ratios of epoxide isomerization and
carboxylation catalyzed by the Xanthobacter and N. corallina epoxide carboxylase systems was further investigated by
individually adding each of the four purified Xanthobacter
components to active N. corallina extracts and measuring the
resultant rates of epoxide isomerase activity observed in the absence
of CO2. As shown in Fig. 8,
the addition of component II resulted in a significantly higher rate of
isomerase activity in the N. corallina cell extract. In
contrast, the addition of component I, III, or IV did not stimulate isomerization to any noticeable degree.
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FIG. 8.
Epoxide carboxylase component II from
Xanthobacter strain Py2 confers epoxide isomerase activity
in cell extracts of N. corallina. Assays were performed with
cell extracts of propylene-grown N. corallina (7.5 mg) in
the absence of CO2. Closed symbols, epoxypropane remaining;
open symbols, acetone produced; inverted triangles, addition of epoxide
carboxylase component I (0.8 mg); squares, addition of epoxide
carboxylase component II (0.6 mg); circles, addition of epoxide
carboxylase component III (0.5 mg); triangles, addition of epoxide
carboxylase component IV (0.6 mg).
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DISCUSSION |
The results of the studies presented in this paper demonstrate
that epoxide metabolism in N. corallina B276 proceeds by a CO2-dependent reaction that forms -keto acids as
products. This represents only the second example of biological epoxide
carboxylation, the other being that of Xanthobacter strain
Py2 (1, 18). These results demonstrate that epoxide
carboxylation is not an isolated phenomenon and that it may, in fact,
be the sole or predominant strategy for epoxide metabolism by the class
of bacteria that grow with aliphatic alkenes as carbon and energy
sources. N. corallina and Xanthobacter strain Py2
are phylogenetically distinct bacteria; N. corallina is a
gram-positive actinomycete, while Xanthobacter strain Py2 is
a gram-negative rod. The fact that two unrelated bacteria utilize the
same pathway of aliphatic alkene and epoxide metabolism provides
support for the idea that this is a fundamental microbial strategy for
the utilization of these compounds.
The initial characterization of epoxide carboxylase from N. corallina suggests that it, like epoxide carboxylase from
Xanthobacter strain Py2, functions as a multiprotein complex
and requires an oxidant (NAD+) and a reductant (NADPH or
DTT) as cofactors. In the purified epoxide carboxylase system from
Xanthobacter strain Py2, the carboxylation of epoxides is
coupled to the transhydrogenation of NAD+ and NADPH
(equation 2). Presumably, epoxide carboxylation in N. corallina has the same reaction stoichiometry. These cofactor requirements, and the associated transhydrogenation, are unprecedented among the known carboxylases. The mechanism of epoxide carboxylation and the roles that the individual components play in the reaction are
not well understood. Epoxide carboxylase component I from Xanthobacter strain Py2 has been proposed to play a key role
in epoxide binding and activation, based on the specific inactivation of this component by the irreversible inactivator methylepoxypropane (2). Epoxide carboxylase component II has been proposed to function as an NADPH:disulfide oxidoreductase which generates a reduced
thiol, possibly on component I, that serves as a nucleophile for attack
on and ring opening of the epoxide substrate (19). It is
unclear what role(s) epoxide carboxylase components III and IV play in
the carboxylation reaction, but they may be involved in the reduction
of NAD+ and/or the formation of the protein-protein
complexes necessary for catalysis (3).
By analogy, proteins with functions similar to those of
Xanthobacter epoxide carboxylase components I to IV are
likely to be involved in epoxide carboxylation in N. corallina. Evidence for the involvement of a protein with
component I activity was provided by the demonstration that
Xanthobacter strain Py2 component I restored epoxide
carboxylase activity when added to cell extracts of N. corallina that had been inactivated by methylepoxypropane (Fig.
7). Furthermore, induction of epoxide carboxylase activity in N. corallina led to the high-level expression of a polypeptide that
migrated on SDS-PAGE with a molecular mass nearly identical to that of
component I from Xanthobacter strain Py2 (Fig. 4) and that
cross-reacts with polyclonal antibodies raised against component I. Together, these results suggest that a protein homologous to component
I is required for epoxide carboxylation in N. corallina. A
polypeptide with a molecular weight and level of expression similar to
those of component II is present in cell extracts of propylene-grown
N. corallina as well (Fig. 4), suggesting that this
polypeptide may function in a role analogous to that of component II,
i.e., in the oxidation of NADPH and the reduction of a disulfide. This
polypeptide did not, however, cross-react to any detectable degree with
polyclonal antibodies raised against Xanthobacter strain Py2
component II. At present, we have not obtained evidence that proteins
analogous to components III and IV are present in N. corallina, although we suspect that such proteins are required. In
Xanthobacter strain Py2, the levels of expression of
components III and IV are significantly lower than those of components
I and II, and they cannot be distinguished from the protein background on one-dimensional SDS-PAGE gels of cell extracts (3).
Additional experiments, culminating with the purification and
characterization of the necessary components from N. corallina, will be required to definitively define the proteins
required by this multiprotein enzyme system.
While there are many apparent similarities between the epoxide
carboxylase systems of Xanthobacter strain Py2 and N. corallina, there is one striking difference: the lower level of
isomerase activity exhibited by N. corallina epoxide
carboxylase when CO2 is excluded from the assays. While
epoxide isomerase activity was detected in cell extracts of N. corallina, the rate of isomerization was significantly lower
(approximately five- to sevenfold) than that observed with cell
extracts or purified components from Xanthobacter strain
Py2. In Xanthobacter strain Py2, epoxide-to-ketone
isomerization is apparently a fortuitous reaction of no physiological
importance (16). The observation that isomerization can
occur is, however, significant since it demonstrates that a reaction
intermediate that can alternatively undergo carboxylation (with
CO2 present) or protonation (without CO2
present) is generated. Since component I has been implicated in epoxide
binding and activation in the Xanthobacter system (2,
3), and since the addition of purified component I from
Xanthobacter strain Py2 restored epoxide carboxylase activity to methylepoxypropane-inactivated N. corallina
extracts (Fig. 7A), it seemed reasonable to predict that differences in the respective component I proteins might be the determinant in the
observed differences in epoxide carboxylation and isomerization in the
two systems. It was therefore surprising to find that the addition of
purified component II (the NADPH:disulfide oxidoreductase) from
Xanthobacter strain Py2 to N. corallina extracts
conferred an increase in epoxide isomerase activity to the level
observed for the Xanthobacter system while components I,
III, and IV had no stimulatory effect (Fig. 8). At present we have no
clear explanation for these observations. Possibly, component II, as
well as component I, contains a portion of the epoxide binding and
activation sites or accepts an intermediate formed at some point during
the reaction from another protein component. Differences in the
properties of the respective component II proteins could thus result in
increased or decreased rates of protonation when CO2 is not
present. The binding of component II to component I may also confer
conformational changes that make the active site more or less
accessible for proton abstraction from water or a general base. Once
purified sources of the N. corallina epoxide carboxylase
proteins are available, it will be interesting to compare their
molecular properties to those of the Xanthobacter proteins
and to investigate the ratios of carboxylase and isomerase activities
when heterologous mixtures of the various components are combined.
These studies should provide further insight into microbial strategies
for the metabolism of xenobiotic compounds generated as intermediates
in unsaturated-hydrocarbon metabolism.
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Abstract
Introduction
