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Plant Physiol, March 2000, Vol. 122, pp. 737-746
Regulation of Sulfate Assimilation by Nitrogen in
Arabidopsis1
Anna
Koprivova,2
Marianne
Suter,
Roel Op
den
Camp,3
Christian
Brunold, and
Stanislav
Kopriva2*
Institute of Plant Physiology, Altenbergrain 21, CH-3013 Bern,
Switzerland
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ABSTRACT |
Using
Arabidopsis, we analyzed the effect of omission of a nitrogen source
and of the addition of different nitrogen-containing compounds on the
extractable activity and the enzyme and mRNA accumulation of adenosine
5'-phosphosulfate reductase (APR). During 72 h without a nitrogen
source, the APR activity decreased to 70% and 50% of controls in
leaves and roots, respectively, while cysteine (Cys) and glutathione
contents were not affected. Northern and western analysis revealed that
the decrease of APR activity was correlated with decreased mRNA and
enzyme levels. The reduced APR activity in roots could be fully
restored within 24 h by the addition of 4 mM each of
NO3 , NH4+, or
glutamine (Gln), or 1 mM O-acetylserine
(OAS). 35SO42 feeding showed that
after addition of NH4+, Gln, or OAS to
nitrogen-starved plants, incorporation of 35S into proteins
significantly increased in roots; however, glutathione and Cys labeling
was higher only with Gln and OAS or with OAS alone, respectively. OAS
strongly increased mRNA levels of all three APR isoforms in roots and
also those of sulfite reductase, Cys synthase, and serine
acetyltransferase. Our data demonstrate that sulfate reduction is
regulated by nitrogen nutrition at the transcriptional level and that
OAS plays a major role in this regulation.
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INTRODUCTION |
Several studies have established regulatory interactions between
assimilatory sulfate and nitrate reduction in plants (Rennenberg and
Bergmann, 1979 ; Reuveny et al., 1980; Cacco et al., 1983; Brunold and
Suter, 1984; Haller et al., 1986; Takahashi and Saito, 1996).
The two assimilatory pathways are very similar and well coordinated
(Brunold, 1993). Deficiency for one element was shown to repress the
other pathway (Reuveny et al., 1980; Neuenschwander et al., 1991). The
activities of ATP sulfurylase (ATPS) and adenosine 5'-phosphosulfate
(APS) reductase (APR), which has been shown to be identical to APS
sulfotransferase (Suter et al., 2000), decreased under
nitrogen-deficient conditions in Lemna minor L. and cultured
tobacco cells (Reuveny et al., 1980; Brunold and Suter, 1984). At the
same time, the addition of nitrate or ammonia to the medium quickly
restored the activity of these two enzymes. Later, ATPS was shown to
not always be repressed by the absence of nitrogen (Haller et al.,
1986), whereas the activity of APR always rapidly decreased under these
conditions (Brunold, 1990). Activity of the last enzyme of
sulfate assimilation pathway, Cys synthase (CS), can also be critical
in varying the flux through the sulfate reduction pathway, since the
precursor of Cys, O-acetylserine (OAS), is derived from the
carbon and nitrogen assimilation pathways. Accordingly, several studies
showed that expression of different isoforms of CS is regulated
differently under both sulfur and nitrogen starvation (Takahashi and
Saito, 1996; Warrilow and Hawkesford, 1998).
ATPS and APR occupy a central control position of sulfate reduction
(Brunold, 1990). Three isoforms of ATPS were cloned from Arabidopsis
(Leustek et al., 1994; Klonus et al., 1995; Murillo and Leustek, 1995),
all possessing a putative chloroplast-targeting peptide. Also, APR
forms a small family of presumably chloroplast localized proteins.
Three cDNA clones coding for APR isoforms were obtained from
Arabidopsis (Gutierrez-Marcos et al., 1996; Setya et al., 1996). Other
enzymes involved in sulfate reduction have already been characterized
on a molecular level (Hell et al., 1994; Ruffet et al., 1995;
Brühl et al., 1996). The availability of molecular probes now
makes it possible to study the regulation of the whole pathway at a
molecular level. Takahashi et al. (1997) demonstrated that
sulfate-deficiency-induced expression of three genes of the pathway
only, the sulfate transporter AST68, APR1, and
SAT-1 (Ser acetyltransferase).
We report the effects of nitrogen deficiency and the subsequent
addition of different nitrogen sources on APR mRNA and protein accumulation and activity in Arabidopsis shoots and roots. To address
the flux through the sulfate assimilation pathway under these
conditions, we also determined the incorporation of
[35S]sulfate into Cys, glutathione (GSH), and proteins.
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MATERIALS AND METHODS |
Plant Cultivation and Treatment
Seeds of Arabidopsis var Columbia, were germinated in plastic pots
(5 cm high, 5 cm in diameter) filled with small moistened balls (2-6
mm in diameter) of burned clay (Blähton, Migros, Switzerland). The pots were placed in trays containing Hentschel nutrient solution (Hentschel, 1970). The plants (three to five per pot) were grown in a
day/night cycle of 10 h/14 h and a light intensity of 115 to 160 µmol
s1 m2. Average
temperature was 25°C to 27°C during the day and 23°C at night.
Relative humidity ranged between 40% and 60%. All experiments were
performed with 4.5-week-old plants. For establishing nitrogen deficiency, the plants were provided with modified Hentschel nutrient solution prepared by substitution of all nitrogen-containing components by the corresponding chlorides. Control plants obtained fresh nutrient
solution at the beginning of the experiment. Plants were incubated for
72 h under the same conditions, then nutrient solution with 4 mM NaNO3, 4 mM ammonium
tartrate, 4 mM Gln, and 0.4 or 1 mM OAS was
added to the nitrogen-deficient plants and they were cultivated for an
additional 24 h.
Enzyme Assays
For preparing extracts, whole shoot or root systems of three to
five plants were pooled and homogenized 1:10 and 1:20 (w/v), respectively, in 50 mM Na/K phosphate buffer, pH 8.0, supplemented with 30 mM
Na2SO3, 0.5 mM
5'-AMP, and 10 mM dithioerythritol (DTE) (Imhof, 1994)
using a glass homogenizer. The crude extracts were filtered through two
layers of Miracloth (Migros, Bern, Switzerland). APR activity in
extracts was measured as the production of
[35S]sulfite, which was assayed as
acid-volatile radioactivity formed in the presence of
[35S]APS and DTE (Brunold and Suter, 1990). CS
activity was determined by measuring the Cys produced from OAS and
S2, as described in Pieniazek et al. (1973).
The protein concentrations in the extracts were determined according to
the method of Bradford (1976) with bovine serum albumin as a standard.
Isolation of Total RNA and Northern Blotting
Plant material was pulverized with mortar and pestle in liquid
nitrogen, and RNA was isolated by phenol extraction and selective precipitation with LiCl. Electrophoresis of RNA was performed on
formaldehyde-agarose gels at 120 V. RNA was transferred onto Hybond-N
nylon membranes (Amersham-Pharmacia Biotech, Uppsala) and hybridized
with 32P-labeled cDNA probes. The membranes were
washed four times at different concentrations of SSC in 0.1%
(w/v) SDS for 20 min, with the final washing step being 0.5×
SSC, 0.1% (w/v) SDS at 65°C, and exposed to x-ray film
(medical RX, Fuji Photo Film, Tokyo) at  80°C for 3 to 8 d. The
autoradiograms were quantified with a densitometer (model GS-670,
Bio-Rad Laboratories, Hercules, CA) using the software Molecular
Analyst (Bio-Rad). Under the hybridization and washing conditions
applied there was no cross-hybridization among the APR and CS isoforms.
The cDNA probes for APR1, APR2, and APR3 were obtained from Dr. T. Leustek (the Center for Agricultural Molecular Biology, Rutgers
University, New Brunswick, NJ), and the cytosolic and chloroplastic CS
and SAT-A cDNAs from Dr. R. Hell (Institute of Plant Genetics and Crop
Plant Research, Gatersleben, Germany). The ATPS1 and SiR cDNAs
corresponding to accession numbers U05218 and Z49217, respectively,
were amplified by RT-PCR from Arabidopsis total RNA, and the identity
of the PCR fragments was verified by sequencing. Northern analysis was
performed on two independent RNA preparations with the same results.
Western-Blot Analysis
Protein extracts were prepared as described by Zavgorodnyaya et
al. (1997). Aliquots representing 10 µg of protein were subjected to
SDS-PAGE and electrotransferred to nitrocellulose filters
(0.2-µm pore size; Schleicher & Schuell, Dassel, Germany). The
blots were analyzed with antisera against APR and developed with the
SuperSignal western-blotting system (Pierce Chemical, Rockford, IL).
The antisera were produced in rabbits from purified APR2 protein
overexpressed in Escherichia coli by the pET His-Tag system
(Novagen, Madison, WI). The antisera cross-reacted with the recombinant
APR1 and APR3 proteins. The analysis was performed on two independent
protein preparations with the same results.
Feeding of 35SO42 and
Determination of 35S in Thiols and Proteins
Four pots with Arabidopsis plants were fed with Hentschel nutrient
solution containing 0.75 mM
SO42 supplemented with 4 mCi of
35SO42
and the different nitrogen sources for 4 h. Shoots and roots were
extracted with 0.1 M HCl containing 1 mM
Na2EDTA and the extracts were centrifuged for 30 min at 4°C. The thiols in the supernatant were reduced with
bis-(2-mercaptoethylsulfone) (BMS) (Bernhard et al., 1998) and labeled
by monobromobimane as described by Newton et al. (1981) and as modified
by Kranner and Grill (1996). A 100-µL aliquot of each sample was
separated by reverse-phase HPLC, as previously described
(Rüegsegger and Brunold, 1992) and fractions of 0.75 mL were
collected in scintillation vials. The 35S
radioactivity was determined in a liquid scintillation counter (Betamatic V, Kontron, Zurich). The radioactivity in the first five
fractions of the eluate corresponded to
35SO42.
Total Cys,  -EC, and GSH were analyzed by the HPLC system described by Schupp and Rennenberg (1988) and modified by Rüegsegger and Brunold (1992). For measurement of 35S
incorporation into proteins, proteins were precipitated from 200 µL of extract with 10% (w/v) TCA, washed twice with 1%
(w/v) TCA and once with 96% (v/v) ethanol, and
redissolved in 400 µL of 0.2 M NaOH. Radioactivity in an
aliquot of the protein solution was determined using a liquid
scintillation counter.
Statistical Analysis
The Student Newmann Keuls method (SigmaStat for Windows, Version
1.0, 1992-94, SPSS, Chicago) was used to determine significant differences in the enzyme activities and the contents of labeled thiols.
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RESULTS |
Effect of Nitrogen Deficiency on the Sulfate Assimilation
Pathway
As evident from Figure 1A, APR
activity was significantly decreased in both roots and leaves of
Arabidopsis after 72 h of nitrogen deficiency. Significant
(P < 0.05) differences in activity were detectable in
leaves after 48 h. Afterward, the enzyme activity further
decreased and after 72 h the extractable APR activity was reduced
to about 70% of that in control plants. In roots, however, the APR
activity was first increased and only after 24 h started to
decrease rapidly, so that after 72 h it had decreased to 50% of
the activity in control plants. The variation in activity within the
first 8 h of treatment in both control and treated plants was due
to diurnal changes (Kopriva et al., 1999). These changes were
characterized by a rapid increase in activity, protein level, and mRNA
during the morning, a decrease during the afternoon, and a slow
increase during the night both in roots and shoots, and had to be taken
into account in the analysis of the results described here. CS, the
final enzyme in the pathway, which we measured for comparison,
exhibited no diurnal changes. As shown in Figure 1B, omission of
nitrogen from the nutrient solution over 3 d did not affect this
enzymatic activity in roots or in shoots. Plant growth measured on a
fresh weight basis and extractable protein were also not significantly
affected by the omission of a nitrogen source (data not shown). The
plants could only be kept on nitrogen-deficient nutrient solution for
4 d, however, since after this time the first symptoms of
senescence were detectable.
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Figure 1.
APR and CS activity during nitrogen deficiency.
Arabidopsis plants (4.5 weeks old) were transferred onto nutrient
solution without a nitrogen source. APR (A) and CS (B) activities were
measured at the time points indicated in extracts from leaves and roots
of nitrogen-deficient plants ( ) and controls cultivated with 4 mM NO3 ( ). Mean values ± SD from five to nine measurements are shown. The
differences in APR activity between nitrogen-deficient and control
plants are significant (P < 0.05) from 48 h.
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Figure 2 shows the changes in mRNA and
protein accumulation of APR and CS during 3 d of nitrogen
deficiency. The levels of mRNA for all three APR isoforms in control
plants increased slightly during the course of the experiment (Fig.
2A), probably due to exchange of the nutrient solution. The APR mRNA
levels in leaves and roots decreased to about 60% and 50%,
respectively, of those in control plants (Fig. 2, A and B). The effect
of nitrogen deficiency was thus more pronounced in roots than in
leaves, which is in agreement with the changes in APR activity (Fig.
1). In leaves levels of mRNA for APR1 and APR2 isoforms decreased more
rapidly in response to nitrogen starvation than APR3, whereas in roots the APR3 isoform was more affected than APR1 and APR2. Despite there
being no changes in enzyme activity, the mRNA level of the chloroplastic isoform of CS decreased in leaves and roots (Fig. 2, A
and B). The level of mRNA for the cytoplasmic isoform of CS in leaves
was not significantly changed, but in roots a decrease of the mRNA
level for this isoform was detected. The discrepancy between total CS
activity and expression of the chloroplastic and cytosolic CS isoforms
might be best explained by assuming a higher expression of the
mitochondrial CS isoform, which would complement the decrease in
expression of the two other isoforms. Indeed, this expression pattern
was described for nitrogen deficiency in spinach (Takahashi and Saito,
1996).
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Figure 2.
Expression analysis of APR and CS isoforms during
nitrogen deficiency. A, Total RNA (10 µg) isolated from leaves or
roots of plants cultivated without a nitrogen source up to 72 h
and controls was analyzed with cDNA probes for APR1, APR2, and APR3,
and chloroplastic (chlCS) and cytosolic (cytCS) CS.
Ethidium-bromide-stained RNA is shown as a control of loading and RNA
intactness. B, Relative mRNA levels of APR1 (), APR2 ( ), and APR3
( ) (top panels), and chloroplastic () and cytosolic () CS
(bottom panels) in leaves (left panels) and roots (right panels) during
nitrogen deficiency. One-hundred percent represents the mRNA level in
control plants at the selected time point. C, Protein extracts (10 µg
of protein) were analyzed by western blotting with antisera against
recombinant APR2. The upper panel shows the protein accumulation in
control plants (C), the lower panel in plants cultivated without a
nitrogen source up to 72 h (N).
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Western-blot analysis revealed a decrease in the APR protein level
during nitrogen deficiency (Fig. 2C) in both leaves and roots. In
contrast, there was no significant effect on the protein accumulation
of both chloroplastic and cytoplasmic isoforms of CS (data not shown).
The Cys and GSH levels in leaves and roots did not change significantly
during 72 h of nitrogen deficiency (data not shown).
Effect of Addition of Different Nitrogen Sources on
APR and CS Activities
The ability of different nitrogen sources to restore the normal
APR activity after 72 h of nitrogen deficiency is demonstrated in
Figure 3. As in Figure 1A, the variation
in APR activity in control and treated plants within the
course of the experiment was due to diurnal rhythms. The
addition of 4 mM nitrate and ammonia restored
normal APR activity in roots within 4 h. During further treatment
with nitrate, APR activity increased to about 120% of the controls. In
leaves the effects of nitrate and ammonia only became significant after
24 h, and APR activity never reached that of controls. Gln only
partially restored APR activity in both roots and leaves (Fig. 3). The
addition of 1 mM OAS caused an increase in APR activity in
roots after 4 h, to 250% of those of nitrogen-deficient plants.
After 8 h, APR activity was four times as high as in the
nitrogen-deficient plants and twice that of controls; however, after
24 h, it dropped to a level lower then the controls. In leaves no
effect of OAS addition on the APR activity was detectable. No
significant effect of the various nitrogen sources was detected on CS
activity (data not shown).
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Figure 3.
APR activity after addition of different nitrogen
compounds. Arabidopsis plants were cultivated for 72 h without a
nitrogen source, fresh media containing different nitrogen sources were
added, and plants were cultivated for additional 24 h. APR
activity was measured in leaf and root extracts 4, 8, and 24 h
after treatment with 4 mM NO3
(), 4 mM NH4+ (), 4 mM Gln (), or 1 mM OAS ( ), as well as in
controls ( ) and plants cultivated without nitrogen (). Mean
values ± SD from five to nine measurements are shown.
Time point 0 corresponds to 72 h without nitrogen.
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The levels of the three APR transcripts in leaves were not affected by
the addition of the different nitrogen sources up to 8 h (Fig.
4). After 24 h with nitrate,
however, a strong increase in the APR3 mRNA level (+200%) and a weaker
increase in the APR1 and APR2 levels (+20% and +80%, respectively)
were detected. The addition of
NH4+ or Gln had no effects
on APR1 and APR2 mRNA during the experimental period, but the APR3 mRNA
level was increased at this time point by both compounds (Fig. 4, A and
B). OAS had no effect on APR mRNA levels in leaves at either 0.4 or 1 mM. The decrease in APR2 mRNA levels at 4 and 8 h and
the increase after 24 h in both control and treated plants is
consistent with previous experiments and is controlled by natural
diurnal rhythms (Kopriva et al., 1999). In roots, nitrate,
NH4+, and Gln did not
affect the levels of APR1 and APR2 mRNA, but those of APR3 were
slightly increased 8 h after the addition of NH4+ and Gln (Fig. 4B). OAS
rapidly induced the mRNA expression of all APR isoforms. Four hours of
treatment with 0.4 mM OAS resulted in three times higher
APR1 and APR3 mRNA levels, which dropped to the control levels after
total 8 h of treatment and increased again to 150% of the
controls after 24 h (Fig. 4B). On the other hand, APR2 transcript
levels only increased about 20% and the increased level remained
stable. The addition of higher concentrations of OAS (1 mM)
had a more prolonged and slightly stronger effect on the expression of
all three APRs than that caused by a 0.4 mM concentration,
but, again, the APR1 and APR3 mRNA levels increased much more than the
APR2 level.
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Figure 4.
Northern analysis of APR after addition of
different nitrogen sources. A, Total RNA (10 µg) isolated from leaves
(left) or roots (right) 4, 8, and 24 h after beginning of
treatment was hybridized with cDNA probes for the three APR isoforms.
Ethidium-bromide-stained RNA is shown as a control of loading and RNA
intactness (RNA). Time point 0 corresponds to 72 h without
nitrogen. B, Relative mRNA levels of the APR isoforms after addition of
different nitrogen sources. The autoradiograms (A) were quantified by
densitometry and the changes in mRNA levels of the APR isoforms after
further incubation without nitrogen () and after additions of
nitrate (), NH4+ (), Gln (),
0.4 mM OAS (), or 1 mM OAS ( ) are
presented. One-hundred percent represents the mRNA level in the
nitrogen-deficient plants at time 0, corresponding to 72 h without
nitrogen.
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Western analysis revealed that the addition of all nitrogen-containing
compounds increased APR protein accumulation in both leaves and roots
(Fig. 5). APR protein gradually increased
after the addition of nitrate,
NH4+, and Gln; the addition
of 1 mM OAS increased APR protein rapidly and transiently.
Nitrate was also the most efficient in the long-term induction of APR
protein accumulation in roots, whereas Gln and OAS induced the fastest
response.
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Figure 5.
Western-blot analysis of APR after the addition of
different nitrogen sources. Protein extracts were prepared from leaves
and roots at the time points indicated and analyzed with antisera
against recombinant APR2, as described in experimental procedures. Time
point 0 corresponds to 72 h without nitrogen.
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Regulation of Other Genes Involved in Sulfate Assimilation by OAS
in the Roots
To evaluate the effect of nitrogen-deficient conditions on other
enzymes of the sulfate assimilation pathway, we performed a northern
analysis with probes against sulfite reductase, SAT-A, a chloroplastic
isoform of ATPS (ATPS1), and chloroplastic and cytosolic CS. No
significant effects on steady-state levels of these mRNAs were observed
in leaves and roots during 3 d of nitrogen deficiency (data not
shown). However, feeding 0.4 mM OAS to the nitrogen-deficient plants led to an increase of mRNA levels of sulfite
reductase, both CS isoforms, and SAT-A in roots (Fig. 6). Only the ATPS1 mRNA was unaffected by
OAS treatment. These data demonstrate that OAS has a major role in the
regulation of sulfate assimilation.
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Figure 6.
Effect of OAS on mRNA levels of genes involved in
sulfate assimilation. Total RNA (10 µg) isolated from roots of plants
kept on nitrogen-deficient nutrition (N) and treated with 0.4 mM OAS at 4, 8, and 24 h after beginning of treatment
was hybridized with cDNA probes for ATPS1, sulfite reductase,
chloroplastic (chl.) and cytosolic (cyt.) CS, and the SAT-A isoform.
Ethidium-bromide-stained RNA is shown as a control of loading and RNA
intactness (RNA). Time point 0 corresponds to 72 h without
nitrogen.
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In Vivo Flux through the Sulfate Assimilation Pathway
For analyzing in vivo sulfate assimilation, plants were
fed with
35SO42
in the nutrient solution for 4 h after 3 d of nitrogen
deficiency and after the addition of various nitrogen sources to the
culture medium of nitrogen-starved plants. The amount of
radioactivity incorporated into thiols and proteins was
measured. The addition of nitrate did not change the
35S uptake into leaves or its incorporation into
GSH and proteins; however, it caused a significant decrease in labeling
of Cys in both leaves and roots (Fig. 7).
OAS increased the
35SO42
labeling of the leaves 2-fold, caused a similar increase of
35S incorporation into proteins, and caused three
times higher labeling of Cys and GSH than in nitrogen-deficient
controls. Although having a significant effect on APR activity and
expression of most genes of the pathway, as in leaves, nitrate did not
significantly alter the amount of
35SO42
incorporated into proteins but diminished the accumulation of radioactive Cys to 50% in roots.
NH4+ and Gln significantly
increased protein labeling; Gln had a stronger effect and also
increased the amounts of labeled GSH. Most interestingly, feeding with
1 mM OAS led to a 30-fold increase in
35S-labeled Cys, a 20-fold increase in -EC
(not shown), and six and four times higher labeling of proteins and
GSH, respectively, compared with nitrogen-deficient controls.
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Figure 7.
Incorporation of 35S from
[35S]sulfate into thiols and proteins. Arabidopsis plants
(4.5 weeks old) were fed with
35SO42 in the nutrient solution
for 4 h together with different nitrogen compounds as in Figure 3.
Radioactive sulfur in SO42, Cys, GSH, and
protein in leaves and roots was measured. Mean values ± SD from four measurements are presented. Values indicated
by different letters are different at P  0.05.
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The data demonstrate a strong positive effect of nitrogen-containing
compounds on the flux through the sulfate assimilation pathway. This
effect was increased the closer the nitrogen source was metabolically
related to OAS, and the acceptor of sulfur was reduced to the thiol level.
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DISCUSSION |
Until now, our knowledge of the regulation of sulfate
assimilation, and particularly APR, by nitrogen nutrition could be
addressed only by activity measurements. Due to the availability of
cDNA probes and antisera, the regulation of APR mRNA and protein could also be analyzed for the first time to our knowledge. During nitrogen deficiency, APR mRNA and protein accumulation decreased in correlation with APR activity. It has to be stressed that the plant growth and
protein concentration in extracts did not change during nitrogen deficiency, indicating that the Arabidopsis plants had sufficient nitrogen stored to cope with this situation. This was corroborated by
the finding that the Cys and GSH concentrations did not change.
Cys synthesis from OAS and sulfide by CS links assimilatory sulfate
reduction with carbohydrate and nitrogen metabolism (Brunold, 1993).
The availability of both substrates of CS is strongly controlled. Cys
inhibits SAT at low concentrations (Brunold and Suter, 1982; Noji et
al., 1998) and sulfate uptake and reduction is inhibited at high Cys
concentrations (Herschbach and Rennenberg, 1994). Therefore, when these
two internal control systems are circumvented by supplying plants with
either OAS or H2S, Cys synthesis is
enhanced and more Cys is synthesized than is needed for protein
synthesis (Neuenschwander et al., 1991; Buwalda et al., 1993; Saito et
al., 1994). The surplus of Cys synthesized under these conditions is used for GSH synthesis and, correspondingly, GSH levels in plants fed
with OAS or H2S were shown to be highly increased
(Neuenschwander et al., 1991; Buwalda et al., 1993). These findings
were corroborated in our experiments using OAS. In addition, they
showed that OAS not only increased APR activity, but also led to a
strong increase in APR mRNA levels and protein accumulation. The
35SO42
feeding revealed that in roots OAS is rapidly metabolized to Cys and
used further for synthesis of proteins and GSH. In leaves, however, APR
activity and the synthesis of 35S-labeled
compounds were much less enhanced by OAS compared with roots,
indicating that OAS was mostly metabolized already in roots and
transported to the shoots only in minute amounts. The increased 35S labeling of Cys and GSH in leaves of
OAS-treated plants compared with those cultivated with the other
nitrogen compounds may be based on the higher specific activity of
35SO42
(Fig. 7) transported to the leaves and/or on enhanced, OAS-driven sulfate reduction in leaf cells.
Most enzymes of the sulfate assimilation pathway are present in
multiple isoforms in plants. In Arabidopsis three organelle-specific isoforms of SAT and CS occur, and ATPS and APR also form small families
of three isoenzymes (however, these are all localized in the
chloroplast) (Murillo and Leustek, 1995; Gutierrez-Marcos et al., 1996;
Setya et al., 1996). Our results clearly showed that the APR mRNAs were
differently regulated by nitrogen compounds and differences were also
observed between roots and leaves (Fig. 4). APR1 and APR2 decreased in
a similar manner during nitrogen deficiency, while APR1 and APR3 mRNAs
responded very similarly to the different nitrogen sources. Also, the
diurnal changes in APR1 and APR3 mRNA levels were not as pronounced as
those of APR2. Interestingly, the amino acid sequence of APR1 is more
related to APR3, being 86.7% and 91.9% identical to APR2 and APR3,
respectively (Gutierrez-Marcos et al., 1996). In addition, both APR1
and APR3 are located on chromosome IV of Arabidopsis, whereas APR2
resides on chromosome I. Nevertheless, the special roles of the
different APR isoforms remain to be elucidated.
Although regulatory interactions between nitrate and sulfate
assimilation have already been described, the mechanism is not yet
clear. Previous reports (Reuveny et al., 1980; Brunold and Suter, 1984;
Haller et al., 1986) documented a strong decrease in APR and ATPS
activities upon nitrogen deficiency. These experiments were, however,
performed with cell cultures or L. minor, thus circumventing
the roots and root/shoot interactions. It is therefore significant that
by using whole Arabidopsis plants, the same effects of nitrogen
deficiency on APR activity were detected. This enzyme activity could be
quickly restored in roots, where reduced nitrogen compounds were more
effective than nitrate. In leaves, only nitrate was able to fully
restore APR activity, probably because of limited transport of the
other nitrogen compounds applied. In L. minor both nitrate
and NH4+ were very
efficient in restoring APR activity, which achieved normal values
4 h after beginning feeding (Brunold and Suter, 1984).
Our feeding experiments demonstrated that the closer the nitrogen
sources were metabolically related to OAS, the higher was their impact
on
35SO42
incorporation (Fig. 7). The lower 35S labeling of
Cys in roots after the addition of
NO3,
NH4+, or Gln compared with
nitrogen-deficient controls indicates that the newly produced
radioactive Cys is used for protein synthesis to a high degree, and
therefore does not accumulate. In addition, northern analysis revealed
that OAS feeding increased mRNA levels of a wide range of genes
involved in sulfate reduction (Figs. 4 and 6). Our data thus extend the
results of Smith et al. (1997), who showed that in barley roots OAS
induced not only sulfate uptake but also the mRNA level of a sulfate
transporter. However, the experiments with OAS were performed on plants
deficient in nitrogen and, therefore, in free amino acids, including
OAS. Cys synthesis may be thus limited by low concentrations of OAS.
The addition of this compound might thus remove this limitation,
leading to a rapid depletion of sulfide and other intermediates of the
sulfate assimilation pathway. This might result in sulfur deficiency, which is known to induce expression of several genes of the sulfate assimilation pathway (Takahashi et al., 1997). In contrast to sulfur
deficiency, however, feeding with OAS led to a high increase of mRNA
levels for sulfite reductase, chloroplastic and cytosolic CS, and SAT-A
(Fig. 6). It seems therefore likely that OAS is a direct
transcriptional regulator of genes involved in sulfate assimilation.
This view is supported by the fact that in bacteria, an isomer of OAS,
N-acetylserine, induces transcription of several genes in
the Cys regulon (Kredich, 1993).
In conclusion, the data presented here show that APR activity in plants
is controlled by nitrogen availability on a transcriptional level, and
that the three APR isoforms are differently regulated. Furthermore, our
results lead to the conclusion that OAS plays a central role in
coordinating sulfate with nitrate assimilation and in the regulation of
the whole assimilatory sulfate reduction pathway.
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ACKNOWLEDGMENTS |
We thank Dr. T. Leustek and Dr. R. Hell for cDNA probes of APR,
CS, and SAT, respectively. We would also like to acknowledge Dr. M. Hawkesford for helpful discussions.
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FOOTNOTES |
Received June 1, 1999; accepted October 28, 1999.
1
This work was supported by the Swiss National
Foundation (grant no. 3149246-96 to C.B.).
2
Present address: Institut für Forstbotanik
und Baumphysiologie, Am Flughafen 17, D-79085 Freiburg in
Breisgan, Germany.
3
Present address: Institute of Plant
Sciences, ETH-LFW D17.2, Universitätstrasse 2, CH-8092
Zürich, Switzerland.
*
Corresponding author; e-mail kopriva{at}uni-freiburg.de; fax
49-761-2038302.
| |
LITERATURE CITED |
-
Bernhard MC, Junker E, Hettinger A, Lauterburg BH
(1998)
Time course of total cysteine, glutathione and homocysteine in plasma of patients with chronic hepatitis C treated with interferon-a with and without supplementation of N-acetylcysteine.
J Hepatol
28: 751-755
[CrossRef][Web of Science][Medline]
-
Bradford MM
(1976)
A rapid and sensitive method for quantification of microgram quantities of protein utilizing the principle of protein-dye-binding.
Anal Biochem
72: 248-254
[CrossRef][Web of Science][Medline]
-
Brühl A, Haverkamp T, Gisselmann G, Schwenn JD
(1996)
A cDNA clone from Arabidopsis thaliana encoding plastidic ferredoxin: sulfite reductase.
Biochem Biophys Acta
1295: 119-124
[CrossRef][Medline]
-
Brunold C
(1990)
Reduction of sulfate to sulfide.
In
H Rennenberg, C Brunold, LJ De Kok, I Stulen, eds, Sulfur Nutrition and Sulfur Assimilation in Higher Plants. SPB Academic Publishing, The Hague, The Netherlands, pp 13-31
-
Brunold C
(1993)
Regulatory interactions between sulfate and nitrate assimilation.
In
LJ De Kok, I Stulen, H Rennenberg, C Brunold, WE Rauser, eds, Sulfur Nutrition and Sulfur Assimilation in Higher Plants. SPB Academic Publishing, The Hague, The Netherlands, pp 61-75
-
Brunold C, Suter M
(1982)
Intracellular localization of serine acetyltransferase in spinach leaves.
Planta
155: 321-327
[CrossRef]
-
Brunold C, Suter M
(1984)
Regulation of sulfate assimilation by nitrogen nutrition in the duckweed Lemna minor L.
Plant Physiol
76: 579-583
[Abstract/Free Full Text]
-
Brunold C, Suter M
(1990)
Adenosine 5'-phosphosulfate sulfotransferase.
In
P Lea, ed, Methods in Plant Biochemistry, Vol. 3. Academic Press, London, pp 339-343
-
Buwalda F, De Kok LJ, Stulen I
(1993)
Effects of atmospheric H2S on thiol composition of crop plants.
J Plant Physiol
142: 281-285
-
Cacco G, Saccomani M, Ferrari G
(1983)
Changes in the uptake and assimilation efficiency for sulfate and nitrate in maize hybrids selected during the period of 1930 through 1975.
Physiol Plant
58: 171-174
-
Gutierrez-Marcos JF, Roberts MA, Campbell EI, Wray JL
(1996)
Three members of a novel smallgene-family from Arabidopsis thaliana able to complement functionally an Escherichia coli mutant defective in PAPS reductase activity encode proteins with a thioredoxin-like domain and "APS reductase" activity.
Proc Natl Acad Sci USA
93: 13377-13382
[Abstract/Free Full Text]
-
Haller E, Suter M, Brunold C
(1986)
Regulation of ATP-sulfurylase and adenosine 5'-phosphosulfate sulfotransferase by the sulfur and the nitrogen source in heterotrophic cell suspension cultures of Paul's scarlet rose.
J Plant Physiol
125: 275-286
-
Hell R, Bork C, Bogdanova N, Frolov I, Hauschild R
(1994)
Isolation and characterization of two cDNAs encoding for compartment specific isoforms of O-acetylserine (thiol) lyase from Arabidopsis thaliana.
FEBS Lett
351: 257-262
[CrossRef][Web of Science][Medline]
-
Hentschel G
(1970)
Untersuchungen über die Aufnahme von 15N-markiertem Harnstoff bei Phaseolus vulgaris L. PhD thesis. University of Hohenheim/Stuttgart, Germany
-
Herschbach C, Rennenberg H
(1994)
Influence of glutathione (GSH) on net uptake of sulphate and sulphate transport in tobacco plants.
J Exp Bot
45: 1069-1076
[Abstract/Free Full Text]
-
Imhof M
(1994)
Die Rolle von Glutathion bei der Resistenz von Arabidopsis thaliana gegen den pathogenen Pilz Pythium paroecandrum. Diploma work. Institute for Plant Physiology of the University of Berne, Switzerland
-
Klonus D, Riesmeier JW, Willmitzer L
(1995)
A cDNA clone for an ATP-sulfurylase from Arabidopsis thaliana.
Plant Physiol
107: 653-654
[Medline]
-
Kopriva S, Muheim R, Koprivova A, Trachsel N, Catalano C, Suter M, Brunold C
(1999)
Light regulation of assimilatory sulfate reduction in Arabidopsis thaliana.
Plant J
20: 37-44
[CrossRef][Web of Science][Medline]
-
Kranner I, Grill D
(1996)
Determination of glutathione and glutathione disulfide in lichens: a comparison of frequently used methods.
Phytochem Anal
7: 24-28
-
Kredich NM
(1993)
Gene regulation of sulfur assimilation.
In
LJ De Kok, I Stulen, H Rennenberg, C Brunold, WE Rauser, eds, Sulfur Nutrition and Sulfur Assimilation in Higher Plants. SPB Academic Publishing, The Hague, The Netherlands, pp 37-47
-
Leustek T, Murillo M, Cervantes M
(1994)
Cloning of a cDNA encoding ATP sulfurylase from Arabidopsis thaliana by functional expression in Saccharomyces cerevisiae.
Plant Physiol
105: 897-902
[Abstract]
-
Murillo M, Leustek T
(1995)
Adenosine-5'-triphosphate-sulfurylase from Arabidopsis thaliana and Escherichia coli are functionally equivalent but structurally and kinetically divergent: nucleotide sequence of two adenosine-5'-triphosphate-sulfurylase cDNAs from Arabidopsis thaliana and analysis of recombinant enzyme.
Arch Biochem Biophys
323: 195-204
[CrossRef][Medline]
-
Neuenschwander U, Suter M, Brunold C
(1991)
Regulation of sulfate assimilation by light and O-acetyl-L-serine in Lemna minor L.
Plant Physiol
97: 253-258
[Abstract/Free Full Text]
-
Newton GL, Dorian R, Fahey RC
(1981)
Analysis of biological thiols: derivatisation with monobromobimane and separation by reversed-phase high performance liquid chromatography.
Anal Biochem
114: 383-387
[CrossRef][Web of Science][Medline]
-
Noji M, Inoue K, Kimura N, Gouda A, Saito K
(1998)
Isoform-dependent differences in feedback regulation and subcellular localization of serine acetyltransferase involved in cysteine biosynthesis from Arabidopsis thaliana.
J Biol Chem
273: 32739-32745
[Abstract/Free Full Text]
-
Pieniazek N, Stepien PP, Paszewski A
(1973)
An Aspergillus nidulans mutant lacking cystathionine-synthase: identity of L-serine sulfhydrylase with cystathionine-synthase and its distinctness from O-acetyl-L-serine sulfhydrylase.
Biochim Biophys Acta
297: 37-47
[Medline]
-
Rennenberg H, Bergmann L
(1979)
Influences of ammonium and sulfate on the production of glutathione in suspension cultures of Nicotiana tabacum.
Z Pflanzenphysiol
92: 133-142
-
Reuveny Z, Dougall DK, Trinity PM
(1980)
Regulatory coupling of nitrate and sulfate assimilation pathways in cultured tobacco cells.
Proc Natl Acad Sci USA
77: 6670-6672
[Abstract/Free Full Text]
-
Rüegsegger A, Brunold C
(1992)
Effect of cadmium on -glutamylcysteine synthesis in maize seedlings.
Plant Physiol
99: 428-433
[Abstract/Free Full Text]
-
Ruffet M-L, Lebrun M, Droux M, Douce R
(1995)
Subcellular distribution of serine acetyltransferase from Pisum sativum and characterization of an Arabidopsis thaliana putative cytosolic isoform.
Eur J Biochem
227: 500-509
[Web of Science][Medline]
-
Saito K, Kurosawa M, Tatsuguchi K, Takagi Y, Murakoshi I
(1994)
Modulation of cysteine biosynthesis in chloroplasts of transgenic tobacco overexpressing cysteine synthase [O-acetylserine(thiol)-lyase].
Plant Physiol
106: 887-895
[Abstract]
-
Schupp R, Rennenberg H
(1988)
Diurnal changes in glutathione content of spruce needles (Picea abies L.).
Plant Sci
57: 113-117
[CrossRef]
-
Setya A, Murillo M, Leustek T
(1996)
Sulfate reduction in higher plants: molecular evidence for a novel 5'-adenylsulfate reductase.
Proc Natl Acad Sci USA
93: 13383-13388
[Abstract/Free Full Text]
-
Smith FW, Hawkesford MJ, Ealing PM, Clarkson DT, van den Berg PJ, Belcher AR, Warrilow AG
(1997)
Regulation of expression of a cDNA from barley roots encoding a high affinity sulphate transporter.
Plant J
12: 875-884
[CrossRef][Web of Science][Medline]
-
Suter M, von Ballmoos P, Kopriva S, Op den Camp R, Schaller J, Kuhlemeier C, Schürmann P, Brunold C
(2000)
Adenosine 5'-phosphosulfate sulfotransferase and adenosine 5'-phosphosulfate reductase are identical enzymes.
J Biol Chem
275: 930-936
[Abstract/Free Full Text]
-
Takahashi H, Saito K
(1996)
Subcellular localization of spinach cysteine synthase isoforms and regulation of their gene expression by nitrogen and sulfur.
Plant Physiol
112: 273-280
[Abstract]
-
Takahashi H, Yamazaki M, Sasakura N, Watanabe A, Leustek T, de Almeida Engler J, Engler G, Van Montagu M, Saito K
(1997)
Regulation of sulfur assimilation in higher plants: a sulfate transporter induced in sulfate-starved roots plays a central role in Arabidopsis thaliana.
Proc Natl Acad Sci USA
94: 11102-11107
[Abstract/Free Full Text]
-
Warrilow AGS, Hawkesford MJ
(1998)
Separation, subcellular location and influence of sulfur nutrition on isoforms of cysteine synthase in spinach.
J Exp Bot
49: 1625-1636
[Abstract/Free Full Text]
-
Zavgorodnyaya A, Papenbrock J, Grimm B
(1997)
Yeast 5-aminolevulinate synthase provides additional chlorophyll precursor in transgenic tobacco.
Plant J
12: 169-178
[CrossRef][Medline]
© 2000 American Society of Plant Physiologists
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|
|
|
|
|
|
|
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[Full Text]
[PDF]
|
|
|
|
|
|
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|
|
|
|
|
|
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[Full Text]
[PDF]
|
|
|
|
|
|
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[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
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837 - 845.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
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Microarray analysis of E2Fa-DPa-overexpressing plants uncovers a cross-talking genetic network between DNA replication and nitrogen assimilation
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4249 - 4259.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
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1701 - 1709.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
N. Ohkama, K. Takei, H. Sakakibara, H. Hayashi, T. Yoneyama, and T. Fujiwara
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43(12):
1493 - 1501.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
S. Kopriva, M. Suter, P. von Ballmoos, H. Hesse, U. Krahenbuhl, H. Rennenberg, and C. Brunold
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November 1, 2002;
130(3):
1406 - 1413.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
O. Berkowitz, M. Wirtz, A. Wolf, J. Kuhlmann, and R. Hell
Use of Biomolecular Interaction Analysis to Elucidate the Regulatory Mechanism of the Cysteine Synthase Complex from Arabidopsis thaliana
J. Biol. Chem.,
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277(34):
30629 - 30634.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
G. Noctor, L. Novitskaya, P. J. Lea, and C. H. Foyer
Co-ordination of leaf minor amino acid contents in crop species: significance and interpretation
J. Exp. Bot.,
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53(370):
939 - 945.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
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127(2):
543 - 550.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
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Orchestrated Transcription of Key Pathways in Arabidopsis by the Circadian Clock
Science,
December 15, 2000;
290(5499):
2110 - 2113.
[Abstract]
[Full Text]
|
|
|
|
|
|
|
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Characterization of Sulfate Assimilation in Marine Algae Focusing on the Enzyme 5'-Adenylylsulfate Reductase
Plant Physiology,
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123(3):
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[Abstract]
[Full Text]
|
|
|
|
|
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