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Applied and Environmental Microbiology, March 2001, p. 1076-1084, Vol. 67, No. 3
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.3.1076-1084.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Chromate Reduction by a Pseudomonad Isolated from a
Site Contaminated with Chromated Copper Arsenate
Jeff
McLean
and
Terry J.
Beveridge*
Department of Microbiology, College of
Biological Science, University of Guelph, Guelph, Ontario, Canada
N1G 2W1
Received 28 August 2000/Accepted 15 December 2000
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ABSTRACT |
A pseudomonad (CRB5) isolated from a decommissioned wood
preservation site reduced toxic chromate [Cr(VI)] to an insoluble Cr(III) precipitate under aerobic and anaerobic conditions. CRB5 tolerated up to 520 mg of Cr(VI) liter
1 and reduced
chromate in the presence of copper and arsenate. Under anaerobic
conditions it also reduced Co(III) and U(VI), partially internalizing
each metal. Metal precipitates were also found on the surface of the
outer membrane and (sometimes) on a capsule. The results showed that
chromate reduction by CRB5 was mediated by a soluble enzyme that was
largely contained in the cytoplasm but also found outside of the cells.
The crude reductase activity in the soluble fraction showed a
Km of 23 mg liter1 (437 µM) and
a Vmax of 0.98 mg of Cr h1 mg of
protein1 (317 nmol min1 mg of
protein1). Minor membrane-associated Cr(VI) reduction
under anaerobiosis may account for anaerobic reduction of chromate
under nongrowth conditions with an organic electron donor present.
Chromate reduction under both aerobic and anaerobic conditions may be a
detoxification strategy for the bacterium which could be exploited to
bioremediate chromate-contaminated or other toxic heavy
metal-contaminated environments.
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INTRODUCTION |
Soluble hexavalent chromium species
[Cr(VI)] are extremely toxic and exhibit mutagenic and
carcinogenic effects on biological systems due to their strong
oxidizing nature (40). Chromate (CrO42) is the dominant Cr(VI) species in
aqueous environments at pH 6.5 to 9. Cr(III) is less toxic
and bioavailable than Cr(VI), as it readily forms insoluble oxides
and hydroxides above pH 5 (31). Previous research into
microbe-mediated Cr(VI) reduction has identified two enzymatic
mechanisms (12). Aerobic reduction is thought to be a
detoxification where cells use a soluble enzyme to reduce Cr(VI) to
Cr(III) internal or external to the plasma membrane. Reduction may
also proceed through the use of CrO42 as a
terminal electron acceptor during anaerobic respiration (22,
38). As such, this activity is associated with the membrane where cytochromes have been implicated (38). It is
possible that not enough energy is generated from anaerobic chromate
reduction to sustain cell growth (22, 23, 32). However, a
sulfate-reducing anaerobe that can reduce Cr(VI) and other
metals to support growth has been isolated (35).
A soluble enzyme from Pseudomonas putida MK1 has been
characterized for genetic engineering to enhance the aerobic chromate remediation potential of this strain (30).
Pseudomonas ambigua G-1 (18) and P. putida PRS2000 (19) also possess a soluble reductase which can reduce chromate both aerobically and anaerobically, with higher reduction rates under aerobic conditions. In
contrast, the reduction activity of Pseudomonas
fluorescens LB300 is membrane associated (9).
However, this strain could not reduce chromate anaerobically on solid
media unless acetate was added as an electron donor. Accordingly, two
separate reduction systems (one membrane-bound and the other soluble)
and mechanisms (one aerobic and one anaerobic) must exist within the
Pseudomonas genus. It is not clear how bacteria such as
P. ambigua and P. putida PRS2000 can reduce
chromate under both aerobic and anaerobic conditions. The fact that a
soluble enzyme is responsible for the catalytic reduction of Cr(VI)
in these two species suggests that it is a detoxification and that no
energy is generated from reduction. It has also been suggested that the
soluble chromate reductases found in chromate-reducing bacteria may
have different primary roles (19, 30).
Our Cr(VI)-reducing pseudomonad, designated CRB5, was recently
isolated from a decommissioned wood preservation site. It can reduce
chromate under both aerobic and anaerobic conditions and accumulates
Cr(III) internal and external to its plasma membrane (25). We have identified a soluble chromate reductase and
a complex strategy for chromate resistance. Using both intact cells and
their extracts, we located most reductase activity in the cytoplasm and
determined the enzyme's kinetics. Since there is an interest in the
bioremediation potential of such bacteria (37), we have
also characterized CRB5 for its ability to tolerate and reduce
Cr(VI) as well as additional toxic metal species under various
conditions through batch bioreactor experiments.
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MATERIALS AND METHODS |
Media.
Vogel-Bonner (VB) broth was modified as described by
Bopp et al. (8) and was used in most of the experiments as
a minimal salts medium. VB broth was chosen because it did not contain
Fe, which can reduce Cr(VI), and to ensure that our results would be comparable to those of Bopp et al. (8). VB broth was
prepared by aseptically mixing 10 ml of VB concentrate, 10 ml of 25%
(wt/vol) D-glucose solution, and 480 ml of deionized
water (all previously sterilized). VB contained the following (in
grams per liter of deionized water): K2HPO4,
10.0; Na(NH4)HPO4 · 4H2O,
3.5; citric acid, 2.0; and MgSO4, 0.2. The medium
designated VBA had additions of amino acids (MEM 50×, an amino acid
supplement; Sigma product no. M5550), which were added in the
bioreactor experiments to stimulate growth, and CaCl2 (0.08 g liter1), which was added to simulate the high Ca
concentration in the groundwater at the contaminated field site.
Batch reactors.
In order to monitor the chemical changes
that occurred during chromate reduction in the growth media, 3-liter
batch reactor systems were used. VB medium was added to the reactor and
autoclaved, followed by the addition of filter-sterilized MEM 50×,
CaCl2, and Cr(VI) to a total of 3 liters. Cells were
first grown in Trypticase soy broth (TSB) (Sigma) without chromate at
30°C, harvested after 18 h, and washed three times with 0.01 M
HEPES. The reactor was inoculated with CRB5 to approximately 6 × 108 cells ml1, and samples were immediately
taken for measurement of initial parameters. Optical density at 600 nm
(OD600), pH, Cr(VI), total Cr and Eh were
monitored over the experimental time course in the unstirred vessel at
20°C. The values obtained for the OD600 measurements
include the light-scattering capacity of cell-sized precipitates formed
during the experiments in addition to the increasing cell numbers.
Eh was a measure of the relative reduction potential of the
bulk solution, which can be due to a combination of several redox
couples. Samples for metal, chemical, and transmission electron
microscopy (TEM) analyses were withdrawn aseptically through a tube
inserted to a depth of 15 cm (the total medium depth was 35 cm) into
the reactor, and an Eh probe was immersed at a depth of 5 cm. For more exact sampling details, see reference 26.
Reduction experiments.
Since CRB5 was isolated from a site
containing copper and arsenate in addition to chromium, the effect of
Cu and As on Cr(VI) reduction was determined under growth
conditions. Aerobic reduction tests were conducted in crimp-sealed or
screw-cap Balch tubes (Bellco Glass, Inc.), leaving a headspace filled
with air, and these were sampled using sterile needles and syringes.
Cell suspensions were prepared as described above and were added to a
final concentration of 7 × 107 cells
ml1 to Balch tubes containing VB media and glucose with
various concentrations of chromate, copper and arsenic. Cultures were
incubated at 30°C without shaking. Samples were taken for Cr(VI)
analyses and TEM preparations at various times during chromate
reduction. Aliquots were plated on Trypticase soy agar (Sigma) without
Cr(VI) for cell viability testing. Chromate reduction in the tubes
containing Cu and As was monitored over time by measuring the
disappearance of Cr(VI). For each treatment, cell-free controls
were prepared to monitor whether abiotic chromate reduction occurred.
All experiments, including abiotic controls, were done in duplicate.
Chromate tolerance was assessed by incubating CRB5 for 24 h at
~7 × 107 cells ml1 in VB broth at
chromate concentrations of 52, 520, 2,600, and 5,200 mg
liter1, and the cells were spread by plating 100 µl of
the culture on Trypticase soy agar.
Metal reduction by resting cells.
Tests were conducted to
determine if CRB5 could reduce several toxic metals under nongrowth or
resting conditions. Anaerobic conditions were obtained by bubbling
bicarbonate medium (2.5 g of NaHCO3, 0.1 g of KCl) for
15 min in Balch tubes with CO2 and N2 (20:80),
which lowered the dissolved oxygen concentration and gave a pH of 6.8. The headspace was purged for 5 min with the gas mixture before being
crimp sealed. Anaerobic additions of 100 µl of 1 M lactate (as an
electron donor) to a final concentration of 10 mM plus 200 µl of
metal solution [either K2CrO4, Fe(III)NTA, Co(III)EDTA, or U(VI) acetate] to a final concentration of 15 mg
liter1 were combined with 8.7 ml of the anaerobic medium.
Harvested cells were washed three times with the anaerobic bicarbonate
buffer solution before resuspension in 25 ml of the same buffer. Balch tubes containing 9 ml of medium were subsequently anaerobically inoculated with 1 ml of culture to a concentration of ~1.5 × 107 cells ml1. Cultures were incubated at
30°C with shaking. Each treatment was conducted in duplicate, with
the initial sample taken anaerobically after the cells were inoculated.
Cell-free controls were not included due to the known stability of
these metals under the conditions of this experiment. Samples were
taken using disposable syringes, which were purged with N2
to avoid introducing any O2 into the culture tube.
Cell fractionation.
Cells were grown in TSB at 22°C and
harvested at mid-exponential phase by centrifugation at 4°C and
4,000 × g. They were washed three times by
centrifugation in HEPES buffer (pH 7), resuspended in 10 ml of the same
buffer, and kept in an ice bath. Cells were mechanically ruptured using
a French pressure cell at 17,000 lb/in2. After cell
breakage, the suspension was centrifuged at 12,000 × g
for 15 min to pellet unbroken cells. Five milliliters of the supernatant (S12) was then set aside and diluted to 10 ml
for further assay. The supernatant was then spun at 150,000 × g for 2 h at 4°C. This high-speed supernatant
(S150) was retained, and the pellet obtained from this step
was used as the membrane fraction, which was resuspended in 10 ml of
buffer for analysis. Soluble fractions (S12 and
S150) were filtered using a 0.2-µm-pore-size filter, and
the fractions were stored at 4°C for less than 1 h before use.
Cr(VI) reduction assays using these fractions were conducted for
each cell fraction at 22°C in shaken, sealed 50-ml serum vials
(anaerobic) and screw-capped bottles with rubber seals (aerobic). Each
treatment was done in duplicate, with the initial sample taken
immediately after Cr(VI) was added.
Extraction of periplasmic components was accomplished using the osmotic
shock procedure (29). Harvested cells from a 2-liter TSB
culture were washed twice with cold 10 mM Tris-HCl (pH 7.1) with 30 mM
NaCl and resuspended in 33 mM Tris-HCl (pH 7.1). Cells were rapidly
mixed into 40% (wt/vol) sucrose in 33 mM Tris-HCl, followed by the
addition of 0.1 M EDTA to a concentration of 0.1 mM EDTA. The
suspension was placed on a rotary shaker at 180 rpm for 10 min before
centrifugation to recover whole cells. The cell pellet was rapidly
dispersed in cold 0.5 mM MgCl2 for 10 min. After
centrifugation, the supernatant containing the osmotic shock proteins
(periplasmic contents) was assayed for Cr(VI) reduction activity.
Total protein in the supernatant fraction was measured before and after
treatment with EDTA to ensure that the outer membrane was permeabilized.
Analytical methods.
Cell concentrations were determined by
microscopic counting of acridine orange-stained cells. Chromate
[Cr(VI)] analyses of the liquid fraction of each treatment were
performed at various time points by aseptic removal of liquid followed
by centrifugation at 16,000 × g for 5 min in 1.5-ml
metal-free microcentrifuge tubes. Cr(VI) in the supernatant was
then measured colorimetrically at 542 nm using the diphenylcarbazide
method (2), which had a detection limit of 0.05 mg of
Cr(VI) liter1. Total Cr in solution after filtration
(0.22-µm-pore-size filter) was analyzed using graphite furnace- or
flame-atomic absorption spectroscopy after acidification. Fe(II)
production was assayed by colorimentric reaction with ferrozine
(33). Co(II) was determined on a Dionex LC-50 liquid
chromatograph (20). Uranium concentrations were determined
by kinetic phosphorescence analysis (36). An increase in
total cellular protein was used as an indication of cell growth, and
these samples were solubilized in 1 M NaOH before analysis. Protein was
measured using the Bio-Rad (Richmond, Calif.) protein assay kit.
Eh was measured using a Corning redox electrode. Where
possible, all materials (glassware, plasticware, and centrifuge tubes,
etc.) were acid leached in 50% HNO3 for at least 24 h
to remove residual metals and rinsed using deionized water.
TEM.
Whole cells and fractions from reduction experiments
were collected and processed for TEM observation without fixation and staining. Since no TEM stains were used, the contrast seen in the
micrographs is due to the binding of metals during treatments. Thin
sections were prepared on cells enrobed in Noble agar, passed through
an ethanol dehydration series, and infiltrated with LR White resin.
Electron micrographs were taken using a Philips EM400T instrument
operating at 100 kV. Energy dispersive X-ray spectroscopy (EDS) and
selected-area electron diffraction (SAED) were carried out using the
EM400T, which was coupled to a Link X-ray detector. Spectra were
collected over 100 s (live count time) using a spot size of 400 nm and
a beam current of 0.1 µA. SAED used a camera length of 640 mm.
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RESULTS |
Batch bioreactor experiments.
In order to monitor changes in
chemistry during Cr(VI) reduction, measurements of Eh,
pH, Cr(VI), total Cr (in solution), and OD600 were
taken over time in unstirred batch reactors containing 3 liters of VB
medium. Samples were also taken for TEM to monitor CRB5 cells for the
accumulation of reduced Cr precipitates. In VB medium with amino acids
and CaCl2, as the initial biomass increased (as monitored
by OD600), several changes in chromate concentration and
chemistry were observed (Fig. 1).
Although the Cr(VI) was reduced over time, the total chromium in
solution fluctuated but did not decrease significantly. The pH dropped
(6.9 to 6.3), and the Eh decreased to below 
470 mV from
initial oxic conditions. Similar changes in solution chemistry were
observed in the control bioreactor with no Cr(VI) present (Fig.
2). There was no increase in cell number
(OD600 = 0.45), however, until the Eh was
below 400 mV, at which point the pH decreased. The Eh
values reflect relative decreases in redox potential and should not be
taken as absolute values.
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FIG. 1.
Batch bioreactor results in VBA medium (VB with amino
acids and CaCl2) at an initial cell density of 6 × 108 cells ml1. Cr(VI) reduction, total Cr
[Cr(III)] plus Cr(VI)] in solution after filtration (Crtot),
pH, Eh, and OD600 are shown.
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As the culture in the Cr-containing reactors grew, its yellow color
[due to soluble Cr(VI)] was replaced by a turbid milky
white to
gray color. Whole mounts of bacteria for TEM were prepared
to determine
if this turbidity was in part due to the precipitation
of reduced
Cr(III) and not just because of increased cell numbers.
Even though
these cells were not conventionally stained for TEM,
they possessed
higher electron density than control cells. Elemental
analysis of the
cells by EDS revealed that Cr was uniformly bound
to bacterial
surfaces, allowing them to be readily imaged by TEM.
The absorbed
chromium was assumed to be Cr(III), since chromate
anions should
not bind to electronegative surface functional groups
found on
gram-negative envelopes. Figure
3 reveals
that Cr(III)
precipitates of various sizes were bound to the cell
as well as
distributed throughout the bulk solution. The
largest precipitates
were slightly rounded, did not produce
regular SAED patterns,
and were therefore amorphous mineral
phases. Given the chemistry
of the solution at sampling time (i.e.,
pH = ~6.8 and E
h =
200
mV), the EDS spectra
of the precipitates, and visual information
of the electron
micrographs, the predicted mineral phase was amorphous
Cr(III)
hydroxide [i.e., Cr(OH)
3]. Formation of these
precipitates
at random sites on the cells was observed in all samples.
Figure
4 shows a cell which was incubated
in the Cr(VI)-contaminated
groundwater from the site [~20 mg of
Cr(VI) liter
1. Electron-dense cells with particulate
Cr(III) coatings similar
to those seen in Figure
3 were commonly
seen in this preparation.
Many cells also possessed polymeric capsules
(Fig.
4) when CRB5
was incubated in the groundwater, and their capsules
were uniformly
coated with Cr(III) precipitates. These precipitates
were not
as dense as those seen on the cell surface and were
(presumably)
more highly hydrated. Even the numerous flagella of CRB5
were
often visible due to the accumulation of metal ions (Fig.
4).
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FIG. 3.
Whole mounts of CRB5 from VB medium with 20 mg of
Cr(VI) liter1. (A) Cr(III) precipitates were
found as discrete particles bound to the cell surface (arrows). One
cell has pulled away from the support film after interaction with the
electron beam. An EDS spectrum from the dense particles generated a
large Cr peak and a small Fe peak, indicating that it is most likely an
amorphous Cr(III) hydroxide or mixed Fe-Cr hydroxide. (B) Amorphous
chromium precipitates (arrows) forming on cells. Bars, 500 nm.
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FIG. 4.
Unstained whole mount of the peritrichous flagellated
CRB5 with precipitates on its capsule. Cr has also accumulated on the
outer membrane of the cell, which appears dark in the electron
micrograph. Bar, 500 nm.
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Metal reduction and tolerance.
Since the potential of this
organism for bioremediation of chromated-copper arsenate-contaminated
sites (such as those found in the wood preservation industry) may also
rely on CRB5's ability to tolerate other toxic metals besides
chromium, experiments were designed to explore tolerance to Cr, Cu, and
As. At our contaminated site, Cu and As were bound to the soil
constituents and immobilized, but it is possible that an on-site
remediation process would remobilize these toxic metals. When CRB5 was
incubated with increasing Cr concentrations, no viable cells were
recovered at concentrations above 520 mg liter1
Cr(VI) reduction in cultures containing Cr(VI) alone or mixed with Cu or As was monitored. There was no significant difference in the
extent of aerobic Cr(VI) reduction after 24 h with 60 mg of As(V) liter1 or 20 and 40 mg of Cu(II)
liter1 (Table 1). Arsenic
at a concentration of 120 mg liter1 (most likely as
AsO42) had a significant effect on initial
reduction. All treatments showed complete Cr(VI) reduction after
120 h.
The high tolerance of CRB5 to copper in solution was investigated
through the use of TEM. In whole-mount preparations, a proportion
of
cells had extensive accumulations of copper bound to the extracellular
capsules seen in the groundwater experiments (cf. Fig.
4 and
5).
EDS showed high copper peaks, and the
mineral phases were not
highly hydrated. It is possible that some of
the copper tolerance
of CRB5 may be attributed to the production of
these extracellular
polymers, which can bind copper on
electronegatively charged functional
groups in their structure
(
16).
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FIG. 5.
Whole mount of a cell grown in VB medium with 40 mg of
Cu liter1. A number of cells were found to have extensive
accumulations of Cu in a matrix of capsular polymers. Bar, 500 nm. An
EDS spectrum generated from the precipitates generated a large Cu peak.
The Ni peak is from the nickel support grid.
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Anaerobic reduction of other metals.
Alternate electron
acceptors such as Fe(III), Co(III), and U(VI), which can be
present in groundwaters, were added separately to a bicarbonate
buffer containing KCl with lactate or dextrose added as the sole
electron donor. Nongrowth conditions were chosen so as to
separate metal reduction from growth-related processes. Truex et al.
(36) suggested that metal reduction under nongrowth conditions might simulate competition for limited substrates in natural
environments. CRB5 reduced Cr(VI), U(VI), and Co(III), whereas there was no significant reduction of Fe(III) (Fig.
6A). The average concentration of the
reduced form of each metal in replicate tubes was plotted in Fig. 6A,
with standard deviations of less than 5% (n = 2). The
results show that reduction of Co(III), as Co(III)EDTA, was low.
Surprisingly, U(VI) at a concentration of 13.7 mg liter1
was reduced to a higher degree than Cr(VI) under these conditions. Uranium reduction was further investigated in tubes that were not
degassed but were crimp sealed with air in the headspace and dextrose
added to the medium as the electron donor. The resulting reduction
rates compared to those for the anaerobic treatments were higher, with
complete reduction occurring after 120 h (Fig. 6B). TEM and EDS of
thin sections and whole mounts revealed that U was located internally
as well as being highly concentrated on the cell envelope (Fig.
7).
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FIG. 6.
Reduction of alternate electron acceptors. (A) Anaerobic
reduction of Cr(VI), Co(III), and U(VI) in bicarbonate buffer with
lactate as an electron donor. (B) U(VI) reduction under anaerobic and
aerobic conditions.
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FIG. 7.
Internal accumulation of uranium confirmed by thin
section. Uranium was also bound on the cell envelope (small arrow).
Bar, 500 nm. An EDS spectrum of internal uranium precipitates is also
shown. The P peak is from the polyphosphate granules; the Cu peak is
from the copper support grid.
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Cellular chromate reduction.
Washed cell suspensions incubated
anaerobically under nongrowth (resting) conditions in bicarbonate
buffer with lactate as an electron donor reduced Cr(VI) from 7 to 4 mg liter1 (standard deviation, <5%; n = 2) (Fig. 8). The initial reduction rates with no electron donor (control) were similar to those in tubes
with lactate, but reduction ceased in control tubes after 24 h.
There was significantly more reduction occurring in the presence of an
electron donor than without a donor under resting conditions.
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FIG. 8.
Anaerobic chromate reduction by washed cells in
bicarbonate buffer with and without lactate as an electron donor.
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Chromate reduction by cell extracts.
Cr(VI) reduction
activities was evident in the soluble fractions of cell extracts
S12 and S150 under aerobic and anaerobic conditions. Figure 9 shows the cell
extracts prepared from a 24-h culture grown at 22°C with no shaking
(stationary culture). Under anaerobic conditions, approximately 80% of
a solution of 10 mg of Cr(VI) liter1 was reduced
within 2.5 h by the S150 fraction. Under aerobic conditions, only 55% was reduced during the same time period. Since
reduction is associated with the soluble fraction, the enzyme responsible could be either cytoplasmic or periplasmic in origin. The
cellular distribution of the soluble enzyme was investigated by
monitoring the Cr(VI)-reducing activity in isolated periplasmic contents and cell filtrates of the culture medium. After EDTA treatment
to permeabilize the outer membrane there was a threefold increase in
the amount of protein in solution (from 0.5 to 1.5 mg
liter1) outside the cells, indicating that periplasmic
proteins were released. There was only a slight reduction of Cr(VI)
using the periplasmic fraction under anaerobic or aerobic conditions
when the total protein concentration was approximately the same as the
concentration in the S150 fraction (Fig.
10A).
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FIG. 9.
Cr(VI) reduction by cellular fractions isolated
after differential centrifugation and mechanical breakage. Cells were
harvested from a stationary (unshaken) culture incubated at
22°C. Anaerobic reduction (solid lines with closed symbols) and
aerobic reduction (dashed lines with open symbols) of cell
fractions are shown.
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FIG. 10.
(A) Cr(VI) reduction in the isolated periplasmic
fraction under aerobic and anaerobic conditions. (B) Percent chromate
reduction in cell-free culture filtrates obtained at different
incubation times. The initial Cr(VI) concentration was 20 mg
liter1.
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Cell filtrates were obtained from a culture grown in VB medium with no
Cr(VI) present to determine if active enzyme was released
from the
cell into the culture medium. This could be through secretion
or
through cell lysis. Culture medium was withdrawn at 24, 48,
and 96 h; cells were separated from the bulk solution by centrifugation,
and
the resulting supernatant was filtered (0.22-µm-pore-size
filter
before being assayed. There was slight reduction in Cr(VI)
by the
filtrate samples taken at 24 and 96 h (Fig.
10B). Approximately
20% of a solution of 20 mg of Cr(VI) liter
1 was
reduced over 72 h in the 48-h filtrate
sample.
Kinetic analysis.
Km and
Vmax values for the crude reductase from cell
extracts and whole cells were determined. The kinetic constants were calculated by fitting the initial rate data to a double-reciprocal Lineweaver-Burk plot of 1/V [milligrams of Cr(VI)
hour1 milligram of protein1] versus
1/[Cr(VI)] (milligrams liter1) derived from a
linear transformation of the Michaelis-Menten equation. This allowed
the estimation of the specific Km and
Vmax for the crude enzyme and the non-specific rate
constants for whole cell reduction.
Washed cells were added to fresh VB medium containing various
concentrations of Cr(VI), and the reaction was monitored in
replicate samples for the loss of Cr(VI) over time (Fig.
11A).
The cultures were incubated
aerobically at 30°C in sealed Balch
tubes. Initial reduction rates
were estimated from the data in
Fig.
11A. The nonspecific
half-saturation or Michaelis-Menten constant,
Km, was estimated to be 1.16 mg
liter
1 (22.3 µM) and the maximum nonspecific reduction
rate or maximum
velocity,
Vmax, was estimated to
be 0.25 mg of Cr h
1 (4.8 µM h
1). Fraction
S
150, prepared from cell extracts as described in
Materials
and Methods, was used to determine the apparent
Km and
the maximum specific reduction rate,
Vmax, of the crude reductase.
S
150
was assayed anaerobically in 0.01 M HEPES buffer (pH 7.1)
at 30°C for
the rate of reduction from 5 to 30 mg of chromate
liter
1.
No additional electron donors (other than found in this soluble
cell
extract fraction) were added to the solution. The total protein
in the
S
150 fraction was measured and then added at a
concentration
of 6.4 mg liter
1. It was assumed that with
excess substrate the reaction would
be pseudo first order and the
initial reaction rate would be independent
of the substrate
concentration. Cr(VI) reduction rates in the
S
150
fraction for 10 to 30 mg liter
1 are shown in Fig.
11B.
Anaerobic reduction by S
150 resulted in
an apparent
Km of 23 mg liter
1 (437µM) and a
maximum specific velocity,
Vmax, of 0.98 mg of
Cr h
1 mg of protein
1 (19 µM
h
1 mg of protein
1).
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FIG. 11.
(A) Cr(VI) reduction of intact cells in VB medium
at five different initial Cr(VI) concentrations. (B) Chromate
reduction in the soluble fraction of cell extracts (S150).
The supernatant fraction was assayed anaerobically at various initial
chromate concentrations in 0.1 M HEPES buffer at 30°C.
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DISCUSSION |
Chromate was readily reduced by CRB5 under aerobic and anaerobic
conditions as cell density increased, with concomitant decreases in redox potential and pH. The changes in solution chemistry were not simply a result of reactions involving chromate reduction; they
were the ultimate result of cellular metabolism as CRB5 grew. Production of acidic metabolic byproducts from aerobic or
anaerobic respiration may account for the observed pH decrease.
The Eh decrease was a result of using oxygen as a
terminal electron acceptor during aerobic respiration as
well as Cr(VI) reduction. Similar changes in chemistry were
observed with the groundwater from the site. At neutral pH, chemical
thermodynamics predict that Cr(III) will readily form insoluble
oxides and hydroxides. The low Eh generated by CRB5
actually favors the precipitation of Cr(III) hydroxides (31). TEM and EDS revealed that Cr(III) was uniformly
adsorbed to the surface of the cells and that precipitates resulted
(Fig. 3). Precipitates were also dispersed in the bulk solution.
Bacteria are excellent nucleation sites for fine-grained mineral
formation due to their high surface area-to-volume ratio
(3) and the presence of electronegative surface functional
groups (e.g., carboxyl), phosphoryl, and hydroxyl groups [6, 14,
15]). As Cr(VI) is reduced, Cr(III) is free to bind
stoichiometrically to these sites and, once bound, will act as a
template for further heterogeneous nucleation and crystal growth
(5). The presence of measurable Cr in solution also
suggests that a proportion of the reduced Cr is complexed with soluble
organic compounds, perhaps electronegative exopolymers
liberated from capsules (Fig. 4 and 5) (16). DeLeo and
Ehrlich reported that formation of Cr(III) precipitates was not
evident in batch and continuous cultures of P. fluorescens LB300 (13), whereas
Pseudomonas chromatophilia, P. ambigua, and
Pseodomonas maltophilia all induce the formation of
precipitates (7, 18, 21).
The toxic effect of Cu (40 mg liter1) and As (20 mg
liter1) on the rate of reduction of Cr(VI) was
insignificant compared to that for controls containing Cr(VI) only.
At high As levels, the low reduction rate may be due to the toxicity of
As(V) on CRB5, which would decrease the number of viable cells. It is
also possible that arsenate could compete as an electron acceptor.
Using TEM and EDS, copper was adsorbed on extracellular polymeric
fibers produced by the cells (Fig. 5), which should lower the metal's toxicity. The potential bioremediation use of CRB5 at site is enhanced
by its ability to tolerate high levels of Cr(VI), Cu(II), and
As(V); these metals will not inhibit reduction.
Resting cells were able to anaerobically reduce Cr(VI),
Co(III), and U(VI) but not Fe(III) with lactate as an electron donor. Slightly higher U(VI) reduction rates were observed under aerobic conditions with glucose rather than lactate as the electron donor. Complete reduction of 170 mg of U(VI) liter1 was observed
after 125 h, with cells accumulating the reduced uranium both on
the surface and internally (Fig. 7). We believe surface precipitation
was via exposed reactive groups (5, 6), although it could
also be due to surface phosphatase activity (24). The
internalization of U was not predicted, as it is most likely toxic to
the cell once in the cytoplasm. CRB5, however, contains large
polyphosphate granules (26) which bind metals (4). Uranium forms strong complexes with phosphate and
could be bound to these internal granules as well as to other
components within the cytoplasm (Fig. 7). Although CRB5 can reduce
Cr(VI), Co(III), and U(VI), it is not clear if the metal ions are
reduced so as to derive energy (as terminal electron acceptors) during anaerobic respiration or to detoxify them.
CRB5, although closely related to P. fluorescens
(26), uses a soluble reductase to reduce chromate. After
separation of the cell membranes from soluble cellular components,
aerobic and anaerobic chromate reduction activity was found in the
soluble fractions (S12 and S150). The membrane
fraction showed no activity; the location of the enzyme is restricted
to the cytoplasm or, possibly, the periplasm. All soluble fractions,
including periplasmic and cell-free filtrates, were obtained from
cultures grown without Cr(VI), therefore, the presence of
Cr(VI) is not required for enzyme production. Although some
reductase may be present in the periplasm, there was not a significant
amount of reduction by this periplasmic fraction over 72 h
compared to that observed in the S150 fraction. Total
protein concentrations in the S150 and periplasmic
fractions were 1.4 and 1.5 mg liter1, respectively. Since
reductase activity was also observed in cell filtrates from 48-h
cultures, the enzyme could be secreted or its presence could be due to
cell lysis. There are obvious advantages to the bacterium if it
transports the enzyme into its environment, such as our toxic
metal-contaminated site, since it would act as a detoxifying agent.
And, since a proportion of reductase is also available in the
periplasm, it would further inhibit the entry of toxic metal into
cells. The majority of the enzyme resides in the cytoplasm.
Accordingly, we suggest that CRB5 could have three lines of defense
against Cr(VI) and other toxic heavy metals. The cytoplasm is where
the reductase is synthesized so as to develop a cellular pool [which
could detoxify Cr(VI) if necessary and be the last line of
defense]. This pool would supply the periplasm with a small but active
concentration of the enzyme so that incoming metal ions could be
detoxified (second line of defense). The pool could also act as a
resevoir for secretion or be liberated by cell lysis (first line of defense).
Other bacteria possess different resistance mechanisms. For
example, a plasmid confers Cr resistance in P. fluorescens
LB300, Pseudomonas aeruginosa, P. putida, and
Alcaligenes eutrophus via decreased uptake of the
metal (8, 11, 27, 28), whereas sensitive strains do not
contain the plasmid (10). A membrane protein, ChrA,
confers tolerance by extrusion of chromate ions in P. aeruginosa and A. eutrophus (1), but
P. ambigua G-1 has a capsule thought to inhibit
chromate from entering (18). It is interesting, then, that
in the groundwater and Cu situations, CRB5 produced an exoplymeric
capsule in which Cr(III) precipitates were found (Fig. 4 and 5).
This could be an additional line of defense.
One result, however, does not fully support the detoxification model of
chromate reduction. Anaerobic reduction by whole-cell suspensions under
resting conditions with lactate as an electron donor was significantly
greater than that by controls without lactate (Fig. 8). Chromate
reduction ceased after 70 h and was not complete over the 140 h it
was monitored. Increased reduction in lactate-containing cultures
indicated that it was an active process. Cells may be reducing chromate
by using it as a terminal electron acceptor in anaerobic respiration.
Another alternative is that the soluble reductase may be enhanced by
the addition of an electron donor, which has been reported previously
with glucose in P. fluorescens (9). If cells
are using chromate to derive energy, membrane-associated reductive
activity would be expected, since the electron transport chain is in
the plasma membrane.
Reduction by Escherichia coli ATCC 33456, under anaerobic
and aerobic conditions, has linked a soluble Cr(VI) reductase to the membrane electron transport chain (32). Although
Cr(VI) reduction was largely due to soluble reductase activity, the
results from those authors indicate that there was minor Cr(VI)
reductase activity associated with this respiratory chain. These
cytochromes required the presence of the soluble reductase for
electron transport to Cr(VI). H2-reduced cytochromes
b and d were reoxidized by Cr(VI) and oxygen
in a fraction containing both the soluble reductase and the
cytochromes, whereas the isolated cytochrome membrane fraction was not
reoxidized by Cr(VI). The authors proposed that only one enzyme was
responsible for electron transport to Cr(VI) and that an active
site in the reductase became membrane associated. They also suggested
that there was not enough energy generated from this reduction at the
cell surface by a soluble reductase to support growth. However,
fermentation with an eventual Cr(VI) electron acceptor via an
abbreviated electron transport chain is energetically favorable and may
be a possible mechanism by which cells can derive energy from chromate
reduction (32). This may also explain the minor reductive
activity of CRB5 observed during resting when an electron donor such as
glucose is present.
Characterization of the chromate reduction activity by CRB5
revealed certain similarities to the E. coli system. Both
E. coli and CRB5 can use endogenous electron donor reserves
and do not require the presence of an external electron donor
such as NADH or glucose. Furthermore, both E. coli
and CRB5 have an increased rate of reduction with increased cell
density and no significant influence on the rate of Cr(VI)
reduction with redox change. It is possible that CRB5 can reduce
Cr(VI) in the same manner as E. coli under aerobic and
anaerobic conditions. In comparison, the reduction by the soluble
fractions of both P. ambigua and P. putida
PRS2000 and MK1 required NADH or NADPH as an electron donor for
activity. Kinetic analysis of our crude reductase activity in the
soluble fraction (S150), conducted under anaerobic
conditions, resulted in a Michaelis-Menten constant
(Km) of 23 mg liter1 (437 µM)
and a maximum specific reduction rate (Vmax) of
0.98 mg of Cr h1 mg of protein1 (317 nmol
min1 mg of protein1) These
Km values are 10 times higher than those
reported for P. putida PRS2000 (19) and 34 times higher than those for P. ambigua G-1. With the
addition of NADH, the soluble reductase activity from P. putida MK1 was 374 µM and 1.72 µmol min1 mg of
protein1 (30).
CRB5 appears to have developed a highly complex set of strategies
to deal with toxic metals at high concentrations through enzymatic and nonenzymatic processes. By producing a soluble enzyme that can catalyze the reduction of Cr(VI) to Cr(III), it
can detoxify its environment. Cell envelope and capsule
exopolymer chromium complexation also inhibit the metal from
entering the cytoplasm. Once reduced, Cr(III) is then free to bind
to the electronegatively charged surface functional groups on the cell
surface, including those on the outer membrane and capsule, which serve
as nucleation sites for further precipitation (5, 6). By
employing this battery of processes, chromate can be effectively
detoxified by reduction and removed from solution. These particular
traits for Cr(VI) and other metal reductions, along with the
bacterium's ability to survive in the stressful on-site environmental
conditions from which it was isolated (25, 26), may
make CRB5 a suitable candidate for a bioremediation strategy.
| |
ACKNOWLEDGMENTS |
The assistance of R. Harris and D. Moyles with TEM and EDS is
gratefully acknowledged.
This work was funded by a Natural Sciences and Engineering Research
Council (NSERC) of Canada research grant to T.J.B. J.M. was funded
by an NSERC industrial scholarship combined with partial funding
through Total Forest Industries Ltd., Guelph, Ontario, Canada. The
electron microscopy was performed in the NSERC Guelph Regional
Scanning Transmission Electron Microscopy Facility (GRSF), which
is partially funded by an NSERC Major Facilities Access grant to T.J.B.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Microbiology, College of Biological Science, University of Guelph,
Guelph, Ontario, Canada N1G 2W1. Phone: (519) 824-4120, ext. 3366. Fax: (519) 837-1802. E-mail: tib{at}micro.uoguelph.ca.
Present address: Pacific Northwest National Laboratory,
Environmental Microbiology Section, Richland, WA 99352.
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Applied and Environmental Microbiology, March 2001, p. 1076-1084, Vol. 67, No. 3
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.3.1076-1084.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
