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Plant Physiol, October 2000, Vol. 124, pp. 553-562
Hormonal Interactions in the Control of Arabidopsis Hypocotyl
Elongation1
Clare E.
Collett,
Nicholas P.
Harberd, and
Ottoline
Leyser*
Department of Biology, The Plant Laboratory, University of York,
York YO10 5YW, United Kingdom (C.E.C., O.L.); and The John Innes
Centre, Norwich Research Park, Norwich NR4 7UH, United Kingdom
(N.P.H.)
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ABSTRACT |
The Arabidopsis hypocotyl, together with hormone mutants and
chemical inhibitors, was used to study the role of auxin in cell elongation and its possible interactions with ethylene and gibberellin. When wild-type Arabidopsis seedlings were grown on media containing a
range of auxin concentrations, hypocotyl growth was inhibited. However,
when axr1-12 and 35S-iaaL
(which have reduced auxin response and levels, respectively) were grown
in the same conditions, auxin was able to promote hypocotyl growth. In
contrast, auxin does not promote hypocotyl growth of
axr3-1, which has phenotypes that suggest
an enhanced auxin response. These results are consistent with the
hypothesis that auxin levels in the wild-type hypocotyl are optimal for
elongation and that additional auxin is inhibitory. When ethylene
responses were reduced using either the ethylene-resistant mutant
etr1 or aminoethoxyvinylglycine, an inhibitor of
ethylene synthesis, auxin responses were unchanged, indicating that
auxin does not inhibit hypocotyl elongation through ethylene. To test for interactions between auxin and gibberellin, auxin mutants were
grown on media containing gibberellin and gibberellin mutants were
grown on media containing auxin. The responses were found to be the
same as wild-type Arabidopsis seedlings in all cases. In addition, 1 µM of the auxin transport inhibitor 1-naphthylphthalmic acid does not alter the response of wild-type seedlings to gibberellin. Double mutants were made between gibberellin and auxin mutants and the
phenotypes of these appear additive. These results indicate that auxin
and gibberellin are acting independently in hypocotyl elongation. Thus
auxin, ethylene, and gibberellin each regulate hypocotyl elongation independently.
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INTRODUCTION |
Plant morphogenesis is governed by
coordinated cell division and cell expansion. A large body of evidence
suggests that plant hormones are involved in regulating these events
but little is known about how they interact to bring about
environmentally and developmentally regulated growth. The Arabidopsis
hypocotyl is a convenient system in which to study the interaction of
plant hormones in cell expansion. The Arabidopsis hypocotyl has a
simple structure: From apex to base there are only approximately 20 cells and during its development, although the hypocotyl may increase more than 10-fold in length, there are no significant cortical or
epidermal cell divisions (Gendreau et al., 1997 ). Hypocotyl elongation is very plastic and is influenced strongly by factors that
regulate cell elongation in the adult plant such as light, plant
hormones, temperature, and touch. There are mutants in Arabidopsis with
altered hormone biosynthesis or signaling and many of these mutations
affect hypocotyl elongation. With the combination of this simple
structure and the availability of hormone mutants, it is possible to
use this system to discover more about the interactions between
hormones in the regulation of cell elongation.
The plant hormone auxin is involved in diverse developmental processes
including cell enlargement, vascular tissue differentiation, root
initiation, gravitropic and phototropic responses, and apical dominance. Auxin has long been thought of as important in cell elongation. When added to isolated stem segments and coleoptiles, auxin
is able to induce elongation. The response begins within 10 min and can
result in a 5- to 10-fold increase in growth rate that can persist for
days (Evans, 1985). Genetic approaches have identified many genes that
are needed for a wild-type auxin response. The phenotypes of some of
these mutants are consistent with a role for auxin in hypocotyl
elongation. For example, mutations in axr1 result in reduced
responses to auxin (Lincoln et al., 1990; Leyser et al., 1993) and
mutations in axr3 have phenotypes consistent with an
enhanced auxin response (Leyser et al., 1996; Rouse et al., 1998). Both
of these mutants have shorter hypocotyls than wild-type seedlings. In
transgenic 35S-iaaL plants, in which a bacterial enzyme is
expressed that conjugates auxin to Lys, free auxin levels are reduced.
Plants expressing this gene show reduced plant size, leaf size, apical
dominance, fertility, and hypocotyl length in the light (Romano et al.,
1991; Jensen et al., 1998).
In the hypocotyl, auxin appears to promote growth in some circumstances
and to inhibit it in others. When intact seedlings are grown on media
containing auxin, the usual response is an inhibition of hypocotyl
elongation. This response suggests that the levels of auxin in the
seedling are already optimal for elongation and addition of any more
auxin makes the levels supra-optimal. There is one example of auxin
promoting growth of intact seedlings. When seedlings are grown on very
low-nutrient medium, exogenous auxin is able to promote hypocotyl
elongation (Smalle et al., 1997). This elongation could happen because
in such low-nutrient conditions, the seedling is not able to synthesize
auxin at optimal levels. The role of auxin in hypocotyl elongation
appears to be different in the light compared with the dark, with polar
auxin transport being more important for hypocotyl elongation in
light-grown seedlings (Jensen et al., 1998). It has been suggested that
auxin could be inhibiting elongation through ethylene (Smalle et al., 1997) since auxin is known to be able to promote ethylene synthesis and
ethylene is known to inhibit hypocotyl elongation (McKeon and Yang,
1995).
Like auxin, gibberellins are involved in the regulation of diverse
developmental processes. Gibberellins can stimulate both cell division
and stem elongation as well as induce germination and fruit setting.
Many mutants in gibberellin biosynthesis and signaling have been
identified. ga1 and ga4 are both mutants in gibberellin biosynthesis (Koorneef and van der Veen, 1980; Sun et al.,
1992; Chiang et al., 1995) and have reduced levels of gibberellins.
Both mutants have shorter hypocotyls than in the wild-type seedlings.
gai and spy are both mutants in gibberellin signaling (Koorneef et al., 1985; Jacobsen and Olszewski, 1993; Jacobsen et al., 1996; Peng et al., 1997 ). Both GAI and SPY are thought to be negative regulators of gibberellin signal transduction that act early in the gibberellin signal transduction pathway. The
phenotypes of the mutants are opposite because gai is a
gain-of-function mutation, resulting in constitutive inhibition of the
gibberellin response, and spy is a loss-of-function
mutation, resulting in a constitutive gibberellin response.
gai plants have short hypocotyls, are dwarfed, flower late,
and are dark green, whereas spy plants show more stem
elongation than wild-type plants, flower early, and are pale green. In
the hypocotyl, it can be shown by using gibberellin-deficient and
altered gibberellin response mutants that gibberellin regulates
elongation in both the light and the dark. Exogenous gibberellin,
however, promotes hypocotyl elongation only in light-grown hypocotyls;
in the dark, the gibberellin response is close to saturation and
gibberellin has little effect (Cowling and Harberd, 1999).
Both auxin and gibberellin are clearly important in hypocotyl
elongation but it is unclear whether they act independently. Previous
studies in pea have suggested that auxin and gibberellin may not be
acting independently in the control of stem elongation. One study
suggested that gibberellin may act, in part, by enhancing auxin action:
The response to applied gibberellin was small in plants with low-auxin
content (Yang et al., 1996). Another study, also in peas, obtained the
opposite result: When auxin transport inhibitors were applied to
elongating internodes of intact wild-type plants, the level of
endogenous gibberellins was decreased below the application site (Ross,
1998). This response suggests that auxin could act by modulating
gibberellin levels. In the pea stem, elongation is a result of both
cell elongation and cell division, whereas in the hypocotyl there is
only cell elongation.
We have used the Arabidopsis hypocotyl as a model system, together with
hormone mutants, to investigate the role of auxin in hypocotyl
elongation and its possible interactions with ethylene and gibberellin.
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RESULTS |
The Role of Auxin
The response of wild-type and mutant Arabidopsis hypocotyls to
exogenous auxin was tested by germinating seedlings on a range of
indole-3-acetic acid (IAA) concentrations. In our conditions, IAA does
not promote the growth of wild-type hypocotyls at any concentration
(Fig. 1). In contrast, IAA promotes the
growth of both axr1-12 hypocotyls and the
hypocotyls of the transgenic plant 35S-iaaL (Fig. 1). This
promotion in growth is likely to be cell elongation rather than cell
division. axr1-12 seedlings have the same number
of cells in an epidermal cell file as wild type (17.06 ± 0.19 for
wild type; 17.12 ± 0.20 for axr1-12;
counted at 3 d old); therefore, the short hypocotyl is not a
result of a reduced number of cells, and previous workers have
demonstrated that there are no significant cortical or epidermal cell
divisions during the postembryonic growth of wild-type hypocotyls
(Gendreau et al., 1997). These data are consistent with the
hypothesis that in the wild-type hypocotyl, auxin levels are optimal
and additional auxin is inhibitory, but in plants with reduced auxin
levels or auxin responses, exogenous auxin can promote growth. This
hypothesis is further supported by the auxin response of the
axr3-1 hypocotyl. Exogenous IAA is unable to
promote the growth of axr3-1 hypocotyls, consistent with their increased response to auxin (Fig. 1). As previously reported, the hypocotyls of axr1 and
axr3 are resistant to inhibition by high levels of auxin
(Lincoln et al., 1990; Leyser et al., 1996). The short final length of
the axr3-1 hypocotyl suggests that a
supra-optimal auxin response inhibits elongation. In this context it is
interesting that the growth pattern of the axr3-1
hypocotyl is complex, with elongation rates above those of the wild
type in the first 3 d followed by very slow rates below those of
the wild type thereafter (Fig. 2). It is
possible that the increased auxin response in this mutant leads to a
greater rate of growth initially but that the auxin growth response
then becomes saturated.
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Figure 1.
Dose responses of wild type,
axr1-12, axr3-1, and
35S-iaaL to IAA. Seeds were germinated on media containing
various concentrations of auxins, in the light (40 µM m 2
s1) at 26°C. Hypocotyl length was measured at
5 d. Data represent the mean hypocotyl length of at least 20 seedlings expressed as a percentage of hypocotyl length on no auxin.
The mean hypocotyl lengths (in mm) on no auxin were as follows:
3.7 (Col), 2.4 (axr1), 3.3 (axr3-1),
and 3.1 (35S-iaaL). Error bars represent the
SE.
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Figure 2.
Growth curve of wild type (Col) and
axr3-1. Seedlings were grown in the light (40 µM m2
s1) at 26°C. Data represent the mean
hypocotyl length of at least 20 seedlings. Error bars represent the
SE.
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Auxin Does Not Act through Ethylene
Hypocotyl elongation is inhibited by the ethylene precursor
1-aminocyclopropane-1-carboxylic acid (ACC) (Fig.
3). To investigate whether auxin acts
through ethylene to inhibit hypocotyl elongation, the response of
hypocotyls to exogenous auxin was tested by germinating seedlings on a
range of IAA concentrations in conditions where ethylene responses were
blocked or reduced. Ethylene responses were blocked by using the
etr1 ethylene-resistant mutant (Chang et al., 1993), and it
was found that the elongation of the etr1 mutant hypocotyl
was inhibited by auxin to the same extent as the wild type (Fig.
4). Ethylene synthesis was blocked using
AVG, a known inhibitor of ethylene synthesis (Yang and Hoffman, 1984). When AVG was added to the growth media, the response to auxin was also
unchanged (Fig. 4).
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Figure 3.
Dose response of wild type to ACC. Seedlings
were grown in the light (40 µM m2
s1) at 26°C. Hypocotyl length was measured at
5 d. Data represent the mean hypocotyl length of at least 20 seedlings. Error bars represent the SE.
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Figure 4.
Dose responses of wild type (Col),
etr1, and wild type with aminoethoxyvinylglycine (AVG) to
IAA. Seeds were germinated on media containing various
concentrations of auxin with or without 5 µM
AVG. Seedlings were grown in the light (40 µM
m2 s1) at 26°C.
Hypocotyl length was measured at 5 d. Data represent the mean
hypocotyl length of at least 15 seedlings expressed as a percentage of
hypocotyl length on no auxin. The mean hypocotyl lengths (mm) on
no auxin were as follows: 2.3 (Col), 2.4 (etr1), and 1.7 (Col with AVG). Error bars represent the
SE.
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Auxin and Gibberellin Act Independently
Next we investigated the interaction of auxin and gibberellin.
When wild-type Arabidopsis seedlings are germinated on a range of
gibberellic acid (GA3) concentrations,
concentrations above 0.1 µM stimulate hypocotyl
elongation (Fig. 5). If gibberellin were
acting by modulating auxin action, then a mutant with a reduced auxin response should show reduced responses to exogenous gibberellin. The AXR1 gene is required for an early stage of auxin signal
transduction and axr1 mutants have reduced auxin sensitivity
in all tissues tested and all assays used (Lincoln et al., 1990). When
axr1 seedlings were grown on a range of
GA3 concentrations, their response was not
obviously different from wild-type seedlings (Fig. 5). If gibberellin
acted by altering auxin transport, one would expect that the addition
of an auxin transport inhibitor would reduce the hypocotyl response to
gibberellin. However, the addition of 1 µM
1-naphthylphthalmic acid (NPA) does not alter the response of the
hypocotyl to GA3 (Fig.
6). These data suggest that exogenous gibberellin can act even if auxin response and auxin transport are
reduced.
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Figure 5.
Dose responses of wild type (Col) and
axr1-12 to GA3. Seeds were
germinated on media containing various concentrations of gibberellin.
Seedlings were grown in the light (40 µM
m2 s1) at 26°C.
Hypocotyl length was measured at 5 d. Data represent the mean
hypocotyl length of at least 20 seedlings. Error bars represent the
SE.
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Figure 6.
Dose responses of wild type, in the presence or
absence of 1 µM NPA, to GA3. Seeds
were germinated on media containing various concentrations of
gibberellin with or without NPA. Seedlings were grown in the light (40 µM m2 s1)
at 26°C. Hypocotyl length was measured at 5 d. Data represent
the mean hypocotyl length of at least 20 seedlings. Error bars
represent the SE.
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If auxin were acting by changing the gibberellin response, then
gibberellin mutants would respond differently to exogenously applied
auxin compared with wild type. To test this hypothesis, the gibberellin
response mutants spy and gai and the gibberellin biosynthesis mutant ga4 were germinated on a range of IAA
concentrations. All showed wild-type IAA responses (Fig.
7). These mutants are in the Landsberg
erecta background, so Landsberg erecta seedlings were used as the control.
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Figure 7.
Dose responses of wild type (Landsberg
erecta), ga4, spy-5, and
gai to IAA. Seeds were germinated on media containing
various concentrations of auxin. Seedlings were grown in the light (40 µM m2
s1) at 26°C. Hypocotyl length was measured at
5 d. Data represent the mean hypocotyl length of at least 20 seedlings expressed as a percentage of hypocotyl length on no auxin.
The mean hypocotyl lengths (in mm) on no auxin were as follows: 2.9 (Ler), 3.0 (ga4), 3.1 (spy-5), and 1.4 (gai). Error bars represent the
SE.
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To test genetically for gibberellin-auxin interactions, crosses were
carried out between the auxin mutants axr3-1 and
axr1-3 and the gibberellin mutants
spy-5 and ga1-3 to obtain double
mutants. The auxin mutants were in the Columbia background and the
gibberellin mutants were in the Landsberg erecta background.
All of the resulting double mutants had poor fertility and phenotypes
characteristic of both parents (Fig. 8).
Although the segregation of the erecta gene had a
significant effect in adult plants, the seedling phenotypes appeared
less affected. All single mutants were shorter than both Columbia and
Landsberg erecta wild-type controls at d 7 (Fig. 9). spy-5 has little effect on
the hypocotyl length and, as expected, the hypocotyls of double mutants
with axr1-3 and axr3-1 are
similar in length to axr1-3 and
axr3-1 hypocotyls, respectively (Fig. 9A). The
hypocotyls of the ga1-3 axr1-3 double
mutant were shorter than either parent, suggesting that the phenotypes
are additive. However, the hypocotyl of the ga1-3
axr3-1 double mutant is longer than
ga1-3 but shorter than
axr3-1 at d 7 (Fig. 9b). To investigate this
result further, earlier time points in hypocotyl elongation were
examined. In the first few days of growth, axr3-1
hypocotyls are longer than wild-type hypocotyls. The presence of the
axr3-1 mutation also promotes growth in a
ga1-3 background at this time, resulting in
hypocotyls that are longer than the ga1-3 single mutant (Fig. 10).
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Figure 8.
Top (from left to right): Columbia,
axr1-3, axr3-1, Landsberg erecta,
spy-5, and ga1-3. Bottom (from left to
right): axr3-1 ga1-3, axr3-1
spy-5, axr1-3 ga1-3, and
axr1-3 spy-5. Plants were grown in 16 h of
light and 8 h of dark and were 5 weeks old. Scale bars = 3 cm.
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Figure 9.
Hypocotyl length of Columbia (Col), Landsberg
erecta (Ler), axr1-3, axr3-1,
spy-5, spy-5axr1-3, spy-5axr3-1 (A), and
Columbia, Landsberg erecta, axr1-3, axr3-1,
ga1-3, ga1-3axr1-3,
ga1-3axr3-1 (B). Seedlings were grown in the
light (130 µM m2
s1) at 23°C. All hypocotyls were measured at
7 d old. Seedlings in B were vernalized in 100 µM GA3 to germinate. Two
sets of data for each double mutant have been included to show that
there is little variation in double mutant hypocotyl length, even
though Landsberg erecta and Columbia genes are
segregating differently.
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Figure 10.
Growth curve of Columbia (Col), Landsberg
erecta (Ler), axr3-1,
ga1-3, and double mutants. Seedlings were grown in the
light (130 µM m2
s1) at 23°C. Data represent the mean
hypocotyl length of at least 20 seedlings. Error bars represent the
SE.
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DISCUSSION |
We have investigated the interactions between auxin and ethylene
and auxin and gibberellin during the control of cell elongation in the
Arabidopsis hypocotyl. This method is a convenient system in
which to study the regulation of cell elongation. Hypocotyl growth
occurs largely in the absence of cell division. The effects of
exogenous hormones can be tested by adding them to the growth medium.
Many hormone signaling and biosynthetic mutants are available to test
possible interactions between the hormones.
The Level of Auxin in Wild-Type Seedlings Is Optimal for
Hypocotyl Elongation
Under our conditions, when wild-type Arabidopsis seedlings are
grown on media containing auxin, elongation of the hypocotyl is
inhibited even though auxin is known to promote cell enlargement in
stem and coleoptile segments (Evans, 1985). However, auxin is
able to promote elongation in plants in which auxin levels or auxin
sensitivity are reduced. axr1 (Lincoln et al., 1990) has
lowered auxin responses (Leyser et al., 1993), and the transgenic line
35S-iaaL conjugates IAA to Lys, giving reduced levels of free auxin (Jensen et al., 1998). Both have shorter hypocotyls than
wild-type seedlings and in both cases adding auxin to the growth medium
stimulates hypocotyl elongation, suggesting that auxin levels in the
seedling are optimal for hypocotyl elongation and that a supra-optimal
level of auxin will inhibit elongation.
Other groups have shown that under certain conditions auxin can
stimulate elongation of hypocotyls of intact seedlings. For example, on
nutrient-poor media, auxin can stimulate hypocotyl elongation (Smalle
et al., 1997). Transgenic seedlings overexpressing the bacterial enzyme
Trp monooxygenase (iaaM) have up to 4-fold higher IAA levels
(Romano et al., 1995). These seedlings have longer hypocotyls than
wild-type seedlings in white light. However, seedlings are
indistinguishable from wild-type seedlings in red, far-red, and blue
light, and shorter than wild-type seedlings in the dark. The superroot
mutant, sur1, which also has increased levels of IAA, has a
longer hypocotyl than wild type in the light and a shorter hypocotyl
than wild type in the dark (Boerjan et al., 1995). These results
contradict our conclusion that the levels of auxin in the wild-type
hypocotyl are optimal for elongation. However, it is likely that the
auxin levels are influenced by factors such as environmental conditions
and the different results obtained by these workers could reflect this
variation. For example, a reduction in auxin synthesis could explain
why the hypocotyls of plants grown on nutrient-poor media can be
stimulated to elongate by the addition of auxin (Smalle et al., 1997).
The 35S-iaaM transgenic line produced by Romano et al.
(1995) is in the RLD background whereas our work is in the
Columbia background. There may be a difference in endogenous auxin
levels or levels of response between ecotypes.
Auxin-induced growth is also observed at higher temperatures (Gray et
al., 1998). The observation that growth at 29°C stimulates auxin
biosynthesis and auxin-dependent elongation in Arabidopsis hypocotyls
suggests that additional auxin-induced elongation is possible over and
above the elongation observed at 20°C. It is possible that the
hypothetical optimal auxin level is higher at higher temperatures.
These results illustrate how environmentally and genetically sensitive
the effect of auxin on elongation is. In some cases, increased auxin
can promote hypocotyl elongation and in others it can inhibit it,
consistent with a dual role for auxin in hypocotyl elongation. A
similar situation exists in roots with auxin promoting elongation in
some conditions and inhibiting it in others. At very low-auxin
concentrations root elongation rates are increased and at higher
concentrations they are reduced, suggesting that levels of auxin in
roots are suboptimal for elongation (Evans et al., 1994).
The response of the dominant gain of function
axr3-1 mutant is more complex. Overall the
phenotype of the mutant suggests an enhanced auxin response (Leyser et
al., 1996). This enhanced response is reflected in the observation that
axr3-1 seedlings have longer hypocotyls than
wild-type seedlings during the first 3 d of growth. However, after
this time elongation in the mutant stops, suggesting that the response
has reached a supra-optimal level and further growth is inhibited.
Consistent with this idea, the data presented here demonstrate that
exogenous auxin is unable to promote the growth of
axr3-1 hypocotyls. The AXR3 gene is a member of the Aux/IAA gene family (Rouse et al., 1998).
Aux/IAA genes are auxin-inducible and encode transcriptional
regulators with characteristically short half-lives (Abel et al.,
1994). The axr3-1 mutation results in a
stabilization of the AXR3 protein (Worley et al., 2000) and it is this
increased longevity that most likely gives rise to the enhanced
response to auxin found in axr3-1 mutant plants.
During seedling development, AXR3 expression declines after
d 4 (D. Rouse and O. Leyser, unpublished data). The
persistence of axr3-1 protein later into seedling development may
block further elongation.
The results obtained here can be compared with those obtained by
Barratt and Davies (1996) who examined the response to exogenous auxin
of pea stem segments at two different developmental stages. They showed
that the growth of early-expansion stages, which have higher levels of
endogenous auxin, was inhibited by exogenous auxin, whereas the growth
of mid-expansion segments, which have lower levels of endogenous auxin,
was promoted by exogenous auxin. Here again, when the levels of auxin
in the plant are optimal for elongation, the addition of more auxin
results in an inhibition of expansion. Moreover, the growth of early
expansion segments of dwarf and severe dwarf pea plants can be promoted
by auxin, just as the growth of axr1-12 and
35S-iaaL hypocotyls can be promoted by auxin.
All of the experiments described above were carried out in the light.
It is important to note the role of auxin in hypocotyl elongation
appears to be very different in the light versus the dark, with polar
auxin transport being more important for hypocotyl elongation in
light-grown seedlings (Jensen et al., 1998).
Auxin and Ethylene Act Independently
Our results show that auxin and ethylene act independently in the
control of hypocotyl elongation. When ethylene responses were blocked,
either using an ethylene-resistant mutant or using AVG to inhibit
ethylene biosynthesis, the effect of auxin on hypocotyl elongation was
unaltered. These data concur with those of Smalle et al. (1997) who
also found that AVG did not alter the effect of auxin on hypocotyl
elongation. In their system, auxin promoted hypocotyl elongation
whereas in our system, auxin inhibits hypocotyl elongation.
Furthermore, they found that silver ions, which interfere with ethylene
perception, reduced the response to auxin. Results with inhibitors need
to be interpreted with caution, since it is difficult to distinguish
primary from secondary effects. However, here the result with AVG is
consistent with the result using the etr1 mutant and
therefore cannot be dismissed as non-specific. In any case, it would be
unlikely that the auxin-induced inhibition of hypocotyl elongation was
mediated by ethylene since auxin can inhibit hypocotyl elongation by
over 80% yet ACC inhibits hypocotyl elongation by only 30% (Figs. 3
and 4). We conclude that auxin does not inhibit hypocotyl elongation by
acting through ethylene but that it acts by a separate mechanism. In
dark-grown seedlings, Thomine et al. (1997) looked at the effect of
anion-channel blockers on auxin and other hormone responses. These
blockers were able to counteract the inhibition of hypocotyl elongation
induced by auxin but not by ethylene or cytokinins, supporting our
results that auxin and ethylene act independently.
Gibberellin and Auxin Act Independently
Our results show that auxin and gibberellin act independently in
the control of hypocotyl elongation. The response of the auxin-resistant mutant axr1-12 to gibberellin is
very similar to the wild-type response; if anything, it responds
slightly more to gibberellin than wild type, which is the opposite of
what one would predict if a normal auxin response was necessary for a
normal gibberellin response. Also, adding NPA, an inhibitor of auxin transport, makes no difference to the gibberellin response, which again
suggests that auxin and gibberellin act independently. The auxin
responses of the gibberellin mutants spy-5, ga4, and
gai are no different from the wild type. Therefore, a normal
gibberellin response is not necessary for a normal response to auxin in
the hypocotyl.
Double-mutant analysis is consistent with the independence of auxin and
gibberellin. The hypocotyl of the ga1-3 (reduced
gibberellin biosynthesis), axr1-3 (reduced auxin
response) double mutant is shorter than that of either parent,
suggesting that the mutations are acting independently in the control
of hypocotyl elongation. The caveat here is that
axr1-3 is not a complete loss-of-function allele.
The hypocotyl of the double mutant between ga1-3
and axr3-1 (a gain-of-function mutant with
increased auxin responses) is shorter than the hypocotyl of
axr3-1 but longer than the hypocotyl of
ga1-3. Although the axr3-1
hypocotyl is shorter than the wild-type mutant at d 7, in the first
3 d of growth, the axr-1 mutant is longer
than the wild type. In Figure 9, we see that at 2 d, the double-mutant hypocotyl is intermediate in length between
axr3-1 and ga1-3, as would be expected if the
phenotypes were additive. By d 4, the axr3-1
hypocotyl has stopped elongating and the ga1-3 hypocotyl is elongating slowly. The rate of elongation of the double
mutants is slower than that of ga1-3 but faster
than the zero rate of axr3-1, again indicating
that the phenotypes are additive. spy-5 hypocotyls are
similar in length to wild-type hypocotyls and, as expected, the
hypocotyls of double mutants with axr1-3 and
axr3-1 are similar in length to
axr1-3 and axr3-1 hypocotyls, respectively. In conclusion, the phenotypes of all double
mutants between auxin and gibberellin mutants seem to be additive,
suggesting that gibberellin and auxin are acting independently in
hypocotyl elongation.
In pea internodes, it has been concluded that the effect of gibberellin
might be mediated, in part, by auxin (Yang et al., 1996): The response
of internodes to applied gibberellin was small in plants with low-IAA
content. However, in contrast to the Arabidopsis hypocotyl, in pea
internodes, elongation depends on both cell expansion and cell
division. It is possible that the interaction of gibberellin and auxin
is in cell division and not cell elongation.
Another study using pea stem segments found evidence that the mode of
action of gibberellin is different at different stages of growth
(Barratt and Davies, 1997). In early-expansion stages, the action of
gibberellin is independent of endogenous IAA concentration whereas in
mid-expansion segments, the magnitude of the response to gibberellin
depends on endogenous IAA content. Therefore, although in the hypocotyl
it appears that auxin and gibberellin act independently to regulate
elongation, further studies are needed to discover whether they
interact at other stages of Arabidopsis development. However, the adult
phenotypes of the double mutants between the auxin and gibberellin
mutants seem to be additive, suggesting that auxin and gibberellin are
acting independently at this stage. A more detailed study of these
plants would be needed to confirm this hypothesis. It is worth
noting that the auxin in the experiments described here is taken up
from the agar, whereas in nature, polar auxin transport is important.
We are currently developing a system to allow auxin to be applied apically.
| |
MATERIALS AND METHODS |
The following mutants and transgenic lines are in the Columbia
ecotype of Arabidopsis and have been described elsewhere:
axr1-3 and
axr1-12 (Lincoln et al., 1990),
axr3-1 (Leyser et al., 1996), etr1-3 (Chang et al., 1993), and 35S-iaaL
(Jensen et al., 1998). The following mutants are in the Landsberg
erecta ecotype of Arabidopsis and have been described
elsewhere: ga1-3 (Koorneef and van der Veen, 1980), ga4 (Koorneef and van der Veen, 1980),
gai (Koorneef et al., 1985), and spy-5
(Wilson and Somerville, 1995).
Arabidopsis seeds were surface sterilized for 15 min in 10%
(v/v) bleach and 0.1% (v/v) Triton, then placed in 70%
(v/v) ethanol and rinsed five times with sterile, distilled
water. Sterile seeds were placed in round 9-cm Petri dishes containing
20 mL of Arabidopsis thaliana salts growth medium
(Wilson et al., 1990). All hormone and inhibitor stocks
were dissolved in 70% (v/v) ethanol at a concentration 1,000 times greater than needed. Twenty microliters of hormone was added to
the Petri dishes prior to the addition of media. After seed sowing,
Petri dishes were chilled for 3 d at 4°C before being placed
vertically in a 16-h-light, 8-h-dark growth room. Experiments for
Figures 1 through 7 were carried out in a growth chamber at 26°C with
a light intensity of 40 µM m2
s1, and the experiments for Figures 9 and 10 were carried
out in a growth chamber at 23°C with a light intensity of 130 µM m2 s1. These
conditions account for the variability in hypocotyl length observed.
etr1-3 seed was provided by the
Nottingham Arabidopsis Stock Centre (Nottinghamshire, UK).
35S-iaaL was kindly provided by C. Romano (Monsanto, St.
Louis). IAA, GA3 (gibberellin), ACC, NPA, and AVG
were obtained from Sigma (St. Louis, MO). All gibberellin used in these
experiments was GA3.
Measurements were made using LUCIA G software (version 3.52a,
1991, Laboratory Imaging, Nikon UK Limited, Kingston, UK).
| |
ACKNOWLEDGMENTS |
We would like to thank the horticultural technicians for
excellent plant care and Stephen Day for useful comments on this manuscript.
| |
FOOTNOTES |
Received February 25, 2000; accepted May 30, 2000.
1
This work was supported by the Biotechnology and
Biological Sciences Research Council.
*
Corresponding author; e-mail hmol1{at}york.ac.uk; fax
44-1904-434312.
| |
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TOP
ABSTRACT
INTRODUCTION