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First published online September 11, 2003; 10.1104/pp.103.022665 Plant Physiology 133:517-527 (2003) © 2003 American Society of Plant Biologists Ethylene and Auxin Control the Arabidopsis Response to Decreased Light Intensity1Department of Molecular Genetics, University of Ghent, Belgium (F.V., W.H.V., J.S., D.V.D.S.); and Department of Molecular and Laser Physics, University of Nijmegen, The Netherlands (L.J.J.L., F.J.M.H.)
Morphological responses of plants to shading have long been studied as a function of light quality, in particular the ratio of red to far red light that affects phytochrome activity. However, changes in light quantity are also expected to be important for the shading response because plants have to adapt to the reduction in overall energy input. Here, we present data on the involvement of auxin and ethylene in the response to low light intensities. Decreased light intensities coincided with increased ethylene production in Arabidopsis rosettes. This response was rapid because the plants reacted within minutes. In addition, ethylene- and auxin-insensitive mutants are impaired in their reaction to shading, which is reflected by a defect in leaf elevation and an aberrant leaf biomass allocation. On the molecular level, several auxin-inducible genes are up-regulated in wild-type Arabidopsis in response to a reduction in light intensity, including the primary auxin response gene IAA3 and a protein with similarity to AUX22 and the 1-aminocyclopropane-1-carboxylic acid synthase genes ACS6, ACS8, and ACS9 that are involved in ethylene biosynthesis. Taken together, the data show that ethylene and auxin signaling are required for the response to low light intensities.
One of the more important environmental factors for plants is the availability of sufficient light. Shading in nature consists of distinguishable features. First, there are the changes in light quality, most often an increase in far red (FR) light due to neighboring vegetation or end of day effects. Within canopies, other spectral changes are also observed (Holmes, 1983  ). Second, there is a diminishment of light intensity or photosynthetic photon flux density (PPFD), including blue and red (R) light, which has direct effects on photosynthesis and photomorphogenesis. Although a large amount of data is available on the influence of light intensity on general biomass production and root to shoot partitioning (Blackman and Wilson, 1951; McConnaughay and Coleman, 1999), relatively little is known about more subtle effects of light quantity on plant architecture and morphogenesis. The latter effects include biomass allocation within organs and leaf form.
Many plant species try to avoid shading and adapt their phenotype to reach out for light (Holmes, 1983
GAs, ethylene, or auxins can induce reorientation of leaves (Brock et al., 1994
PhyB (Phytochrome B) mutants have elevated petioles even in non-shaded conditions (Somers et al., 1991
A first indication for a correlation between ethylene action and hyponasty was presented in a study of the submergence response of Rumex palustris. In this flooding-tolerant species, ethylene induces hyponasty and extension of petioles, allowing the leaf blades to reach the water surface (Cox et al., 2003
On the other hand, there is also a relation between light signaling and ethylene. Sorghum (Sorghum bicolor) wild-type plants subjected to dim FR-enriched light, and phyB mutants produced more ethylene than wild-type plants under white light (Finlayson et al., 1998
Data on ethylene and light interactions in vegetative development are rather scarce. It is generally accepted that light inhibits ethylene synthesis by reducing 1-aminocyclopropane-1-carboxylic acid (ACC) oxidase (ACO) activity (Kao and Yang, 1982
Considering the phenotypic overlaps of shade, auxin, and ethylene responses, we decided to investigate to which extent these factors work together to determine plant architecture. In the majority of previous studies on shading, the emphasis was put on qualitative differences, i.e. changes in the R to FR ratio. Nevertheless, reacting to mere changes in light intensity can be of considerable importance in pioneer plants such as Epilobium species and Arabidopsis (Chapin et al., 1994
Low Light Intensity Is Correlated with an Increase in Ethylene Production
Ethylene production of intact 2-week-old Arabidopsis seedlings was measured using laser-based photo-acoustic detection, able to detect levels as low as 1 nL L–1 (Bijnen et al., 1996
Plants grown on medium containing the ethylene precursor ACC produced sufficient amounts of ethylene for continuous flow detection. To measure changes in ethylene production in Arabidopsis upon a switch in light intensity, seedlings were grown on a saturating concentration of ACC (50 µM; Smalle et al., 1997
Auxin-insensitive mutants are affected in numerous developmental processes (for review, see Tian and Reed, 2001
We further investigated the role of ethylene and auxin on leaf angle, induced by low light intensity. Elevation angle was defined by Herbert (1983
Similar to ethylene-insensitive mutants, the effect of light intensities on the elevation angle in auxin mutants was also less pronounced than in the wild type (Fig. 3). Axr1-3 and axr2 and did not respond. Hls1-1, which is disturbed in differential growth for apical hook formation in dark grown seedlings, had a wild type-like response (Lehman et al., 1996 To investigate the relation between ethylene and auxin in this process in more detail, we treated auxin mutants with ethylene for 6 d. The effect was severely attenuated in axr2 and was still very obvious in axr1-3 (Fig. 4). Thus, intact auxin signaling is needed for the ethylene-induced phenotype to occur.
Together, these data suggest that low light-induced leaf elevation is dependent of both ethylene and auxin signals and that the ethylene response requires a functional auxin signaling pathway.
Another characteristic typical of wild-type Arabidopsis plants grown in low R to FR ratios is the increase in elongation of petioles and a reduction of leaf blade surface (Robson et al., 1993
The auxin-insensitive mutants (axr2 and axr1-3) were also impaired in the redistribution of biomass (Fig. 6B). In comparison with wild type, they had short petioles, especially in low light (Table I; Fig. 5). Axr2 had the most severe phenotype. In this mutant, no change was observed. This confirms the necessity for a normal auxin response in the reaction to shading. Continuous supply of 50 µM ACC could not revert the phenotype of the auxin-insensitive mutant axr2 (Fig. 6C).
To investigate to what degree changes in gene expression are involved in the above-described responses, we used a modified cDNA-AFLP method to analyze part of the transcriptome (Breyne et al., 2002
To assess the effect on the final step in ethylene biosynthesis, the expression of six ACO genes was studied. Transcript regulation was similar to that of the ACS genes. A number of ACO genes, with At1g5010 (ACO1), At1g62380 (ACO2), and At1g04350 among them, were rather constitutively expressed. In contrast, the putative ACOs, At2g19590 and At5g63600, were clearly induced in leaf blades in low light intensities. This was also the case for At5g43450, albeit to a lesser extent. ACO mRNA levels were never down-regulated in low light intensity.
Quality versus Quantity Shading. Can They Be Uncoupled?
Plants react to shading of canopies by detecting changes in light quality, i.e. R to FR ratio (Smith and Whitelam, 1997
At4g32285 is a homolog of the auxin inducible AUX22 genes of mung bean hypocotyls (Yamamoto et al., 1992 Moreover, auxin-inducible ethylene biosynthesis genes had a higher transcript level in phyB-9 mutants (Fig. 7). These plants have a constitutive shade avoidance phenotype, typical for plants grown under low R to FR ratios. Therefore, it is likely that the responses to quantity shading have a similar underlying auxin-dependent mechanism as those upon growth in quality shading, i.e. low R to FR ratios. However, as to the ethylene production rates, quantity and quality shading can be uncoupled. Upon FR enrichment without altering PPFD levels, the ethylene signal is of minor importance because ethylene-insensitive mutants do react to the addition of FR. Moreover, we could not detect any increase in ethylene production. In contrast, lowering light intensity coincided with increased ethylene production, and ethylene-insensitive mutants have a defect in leaf hyponasty.
In Arabidopsis, elevation of leaves has been described as a function of gravity and is influenced by R to FR ratio and light intensity (Fig. 3; Hangarter, 1997
One of the best known ethylene responses is the inhibition of cell expansion and consequent dwarfism. This has been shown for roots, dark-grown hypocotyls, and light-grown mature plants. Previous work indicated that as leaves expand, ACS1 mRNA levels decrease (Rodrigues-Pousada et al., 1993 The respective partial and complete failure of ethylene- and auxin-insensitive mutants to react to shading suggests that both hormones may be involved in the same cascade. However, auxin-insensitive mutants could not be rescued by continuously applying exogenous ACC or ethylene. This may not reflect the natural conditions, in which diurnal fluctuations of ethylene production can occur (F. Vandenbussche and D. Van Der Straeten, unpublished data). Thus, timing of the signals may be important. Nonetheless, it is also possible that light intensity exerts its regulation of ethylene synthesis independent of the auxin signal.
Transcription of putative ACO genes, although shade induced, appeared independent of phytochrome B signaling with the exception of At2g19590, which had a lower expression level in phyB-9. However, it remains to be determined whether At2g19590 is a true ACO. Other factors probably exert an effect on expression of ACOs upon shading. One possibility is regulation by other stable phytochromes (Clack et al., 1994
Apart from regulation of ethylene biosynthesis genes on the transcriptional level, light also has an influence on ethylene production by the modification of ACO. The fast decrease in ethylene production, which we measured during the change from low to high light intensities, might indicate a rapid change of enzyme activity due to a depletion of catalytic CO2 caused by an increase in photosynthetic activity. This confirms previous reports in which light was found to have an inhibitory effect on ethylene biosynthesis in green tissues (Yang and Hoffman, 1984
PhyB mutants have a higher ethylene production (Fig. 1A; Finlayson et al., 1998 The reaction of Arabidopsis plants to shading, caused by spectral changes (i.e. FR enrichment) or low light intensity, probably relies to some extent on the same mechanism. This involves a precise control of auxin and ethylene signals and determines the architecture of the leaves.
Plant Material and Biometrics
Col-0, phyB-9, axr1-3, axr2-1, hls1-1, eto2, ein2-1, and etr1-3 seeds were obtained from the Arabidopsis Biological Resource Center (Columbus, OH). All mutants are of the Col-0 background. Seeds were sown and plants were grown under sterile conditions as described (Smalle et al., 1997 For the leaf biomass distribution experiments, plants were grown on a medium containing one-half-strength Murashige and Skoog salts and 1% (w/v) Suc in cool-white light (Lumilux Plus, Osram, Germany) under a photoperiod of 16 h of light/8 h of dark at 22°C. Three days after the emergence of leaves 5 and 6, corresponding to approximately 2.5 weeks at midday, leaves 3 and 4 were harvested and stuck to paper with tape. An image was acquired using a flatbed scanner. Analysis of the petiole length and leaf blade surfaces was done with ScionImage software (Scion Corp., Frederick, MD). For the study of leaf angles, plants were grown on soil in cool-white light (Lumilux Plus) under the same photoperiod as above. When the fourth leaf pair emerged, plants were taken from the soil at midday and meticulously dissected such that only the hypocotyl, the apical meristem, the petiole, and the midvein of leaf 6 were left. These were very carefully stuck onto paper without disturbing the original inclination. An image was acquired using a flatbed scanner. Analysis of the elevation angles (this is the angle between petiole and the horizontal) was done with ScionImage software (Scion Corp.).
Plants were grown on Murashige and Skoog/2 medium containing 1% (w/v) Suc and 50 µM ACC in 16 h of light/8 h of dark at 22°C and 60% relative humidity. To compare the effect of low light and higher light intensities on ethylene biosynthesis, 2-week-old Col-0 and phyB-9 plants were grown in 120 or 30 µmol m–2 s–1 PPFD, respectively, for 3 d to minimize effects of circadian rhythms. After that, 12 plants were put in air-tight 100-mL glass vials while remaining on the same medium. Ethylene production of wild-type Arabidopsis plants was too low for continuous flow measurements. Therefore, we measured ethylene after accumulation in a closed vial. Every 2 h, the vials were flushed at a flow rate of 1 L h–1, and ethylene was measured.
For the light switch experiment, plants were essentially in the same conditions as mentioned above. Variety in light intensity was achieved by adding or removing cool-white light tubes. Changes in R to FR ratio were obtained by adding filtered incandescent light from a 60-W bulb. The R to FR and PPFD values were determined using an Li-1800 (LI-COR) portable spectroradiometer. After 2 weeks, they were put in glass jars for gas measurements while still on the same medium. The jars were fit into a continuous flow system, connected to a photo-acoustic detector for measuring ethylene (Bijnen et al., 1996
Leaf blades and petioles of 2.5-week-old plants, grown on Murashige and Skoog/2 + 1% (w/v) Suc in 16 h of light/8 h of dark at 22°C, were harvested at midday and frozen in liquid nitrogen. RNA was prepared using QIAGEN RNeasy (QIAGEN GmbH, Hilden, Germany). RNA was treated with Dnase amplification grade (Life Technologies/Gibco-BRL, Cleveland).
To get an overview of gene expression, we used a modified cDNA-AFLP technique (Breyne et al., 2002 RT-PCR with gene-specific primers was also performed. For ACS4, ACS6, ACS8, all ACO genes, and UBQ 14, the pre-amplification reactions of the cDNA-AFLP were used as template material for the gene-specific PCR. For all other genes, the gene-specific PCRs were done directly on cDNA that was obtained by a classical RT reaction according to protocol (Invitrogen, Carlsbad, CA). All PCRs were done in a Mastercycler (Eppendorf, Hamburg, Germany). Cycles had 30 sec at 95°C, 35 sec at hybridization temperature, and 30"at 72°C. A list of gene-specific primers and reaction conditions is given in Table II. Separation was done on a 1% (w/v) agarose gel. DNA was stained with ethidium bromide in the gel.
The authors wish to thank Mira Haegman for technical assistance and the sequencing group at the Plant Systems Biology lab of Ghent university for all their good work. Received February 26, 2003; returned for revision April 14, 2003; accepted June 30, 2003.
Article, publication date, and citation information can be found at www.plantphysiol.org/cgi/doi/10.1104/pp.103.022665.
1 This work was supported by the Fund for Scientific Research (Flanders; grants no. G.0281.98, WO.004.99, and G.0345.02 to D.V.D.S.), by the Flanders Interuniversity Institute of Biotechnology, and by the European Union (grant nos. EU–RTN–INTEGA and HPRN–CT–2000–00090).
2 Present address: College of Agricultural and Life Sciences, University of Wisconsin, Madison, WI 53706. * Corresponding author; e-mail dominique.vanderstraeten{at}ugent.be; fax 32–9–2645333.
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