Effects of brassinosteroid, auxin, and cytokinin on ethylene production in Arabidopsis thaliana plants

Richard N. Arteca^* and Jeannette M. Arteca

Department of Horticulture, The Pennsylvania State University, University Park, PA 16802, USA

^* To whom correspondence should be addressed. E-mail: rna{at}psu.edu

Received 15 February 2008; Revised 2 May 2008 Accepted 8 May 2008

Abstract

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Inflorescence stalks produced the highest amount of ethylenein response to IAA as compared with other plant parts tested.Leaf age had an effect on IAA-induced ethylene with the youngestleaves showing the greatest stimulation. The highest amountof IAA-induced ethylene was produced in the root or inflorescencetip with regions below this producing less. Inflorescence stalkstreated with IAA, 2,4-D, or NAA over a range of concentrationsexhibited an increase in ethylene production starting at 1 µMwith increasingly greater responses up to 100 µM, followedby a plateau at 500 µM and a significant decline at 1000µM. Both 2,4-D and NAA elicited a greater response thanIAA at all concentrations tested in inflorescence stalks. Inflorescenceleaves treated with IAA, 2,4-D, or NAA exhibited the same trendas inflorescence stalks. However, they produced significantlyless ethylene. Inflorescence stalks and leaves treated with100 µM IAA exhibited a dramatic increase in ethylene production2 h following treatment initiation. Inflorescence stalks showeda further increase 4 h following treatment initiation and nofurther increase at 6 h. However, there was a slight declinebetween 6 h and 24 h. Inflorescence leaves exhibited similarrates of IAA-induced ethylene between 2 h and 24 h. Light andhigh temperature caused a decrease in IAA-induced ethylene inboth inflorescence stalks and leaves. Three auxin-insensitivemutants were evaluated for their inflorescence's responsivenessto IAA. aux2 did not produce ethylene in response to 100 µMIAA, while axr1-3 and axr1-12 showed reduced levels of IAA-inducedethylene as compared with Columbia wild type. Inflorescencestreated with brassinolide alone had no effect on ethylene production.However, when brassinolide was used in combination with IAAthere was a dramatic increase in ethylene production above theinduction promoted by IAA alone.

Key words: Arabidopsis, auxin, brassinolide, cytokinin, ethylene, indole-3-acetic acid

Introduction

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Ethylene is the simplest plant hormone known today. Even thoughthe structure is very simple it participates in the regulationof a variety of developmental processes in plants, from seedgermination through organ senescence and abscission (Abeles et al., 1992).In recent years there has been an explosion of ethylene research,thereby leading to enormous strides forward in this area. Thereare a number of ethylene-signalling and -response pathways,which are very complex. There are many factors that stimulatethese pathways, some of which are as follows: ethylene, cytokinins,auxins, brassinosteroids, plant development, stress pathogens,sugars, jasmonic acid, gibberellins, abscisic acid, and a varietyof others (Stepanova and Alonso, 2005). There are a number ofreports in the literature showing that auxin stimulates ethyleneproduction in a variety of plant tissues. In fact, many of theresponses that were once attributed to auxins have now beenshown to be due to ethylene (Abeles et al., 1992; Arteca and Arteca, 2001).More than 30 years ago brassinosteroid research began when JohnMitchell and co-workers at the US Department of Agriculturebegan screening pollens in search of new plant hormones. Todaybrassinosteroid (BR) has been shown to be involved in a widerange of physiological processes in plants, which have beensummarized in numerous review articles (Adam and Marquardt, 1986;Mandava, 1988; Sakurai and Fujioka, 1993; Arteca, 1995; Chory et al., 1996;Yokota, 1997; Clouse and Sasse, 1998; Haubrick and Assmann, 2006).It was nearly a decade ago when BR-deficient Arabidopsis mutantswere discovered, establishing BR as an essential plant hormone,thereby stimulating many studies on multiple mechanisms of BRsignalling (Gendron and Wang, 2007). In addition to auxin, BR,a growth-promoting compound with a similar structure to animalsteroid hormones, has been shown to induce ethylene productionalone, and acts synergistically to stimulate ethylene productionin etiolated mung-bean seedlings (Arteca et al., 1983; Yi et al., 1999;Swarup et al., 2002). More recently Joo et al. (2006) showedthat epibrassinosteroid induces AtACS4 an auxin-responsive ACCsynthase gene in Arabidopsis. Although auxins and BRs have beenshown to promote ethylene alone and, when applied in combination,act synergistically in the stimulation of ethylene production(Arteca et al., 1983, Swarup et al., 2002), most of the workhas been performed in mung bean, which has a number of disadvantagesassociated with it, one of the main ones being that geneticanalysis is difficult. To date there has been no detailed analysisof auxin and BR induction of ethylene alone or in combinationin Arabidopsis, nor has a model experimental system been establishedas to what the optimal tissue, stage of development, or otherfactors are required for maximal hormonal stimulation of ethyleneproduction. The purpose of this study was to evaluate whichtissues were most sensitive to plant hormones, the optimal conditionsfor the induction of ethylene by different plant hormones, andthe interactions between the different plant hormones on theinduction of ethylene in Arabidopsis, thereby establishing amodel experimental system. By establishing a model experimentalsystem in Arabidopsis, utilizing genetic and molecular toolscurrently available when using Arabidopsis as an experimentalorganism, it will be possible to go into more depth as to howand why auxins and BR trigger ethylene production in green plants.

Materials and methods

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Conditions for plant growth
Arabidopsis thaliana (L.) Heynh ecotype Columbia wild-type (WT)and the auxin-insensitive mutant (axr2, axr1-3, and axr1-12)plants were grown in soil or hydroponically. Plants grown insoil were as described in the Arabidopsis Biological ResourceCenter (ABRC) manual. Plants were grown hydroponically accordingto the procedure outlined by Arteca and Arteca (2000). The environmentalconditions used to grow plants were the same for those grownin both soil or hydroponically. Temperatures were maintainedat 22±2 °C for a 16 h day/8 h night period. The lightlevels were maintained between 100 and 120 µmol m^–2s^–1 with cool white fluorescent lights. Plants grown insoil were watered by sub-irrigation with tap water twice a week.

Treatments
In order to evaluate IAA-induced ethylene production in differentArabidopsis plant parts, 35- to 45-d-old plants grown hydroponicallywere divided into different plant parts including roots, youngrosette leaves, inflorescence leaves, terminal inflorescencebud, lateral inflorescence bud, axillary leaf bud, and primary,secondary, and lateral inflorescence stalk. The different plantparts were put into 12x75 mm test tubes containing 200 µlof 100 µM IAA or water, which served as a control, thensealed with serum caps and placed in the dark. The temperaturewas maintained at 22±2 °C and ethylene analysed after24 h unless specified otherwise. In all cases values are expressedas the mean of four replications ±standard error unlessspecified otherwise.

To determine if leaf position had an effect on IAA-induced ethyleneproduction in Arabidopsis plants, 24-d-old plants grown in soilwere divided into four groups, based on their position in therosette from the youngest to the oldest, as described by Arteca and Arteca (2001).Leaves from different positions were put into test tubes andtreated as previously described.

Root systems from 24-d-old Arabidopsis plants grown hydroponicallywere divided into four 5 cm sections in order to determine ifthe location on the root had an effect on IAA-induced ethylene.The different sections were put into test tubes and treatedas previously described.

To evaluate if the location on the inflorescence had an effecton IAA-induced ethylene production, 35-d-old Arabidopsis plantsgrown in soil, with inflorescences 10 cm long, were dividedinto five 2 cm sections. The 2 cm sections were cut into fivesections 4 mm in length. The different sections were put intotest tubes and treated as previously described.

Primary inflorescences, 4–6 cm in length with flowerspartially opened, from 35- to 45-d-old Arabidopsis plants wereused in order to determine the effects of different concentrationsof indole-3-acetic acid (IAA), 2,4-dichlorophenoxyacetic acid(2,4-D), naphthaleneacetic acid (NAA), and tryptophan (TRP)on ethylene production in inflorescence stalks and leaves. Theinflorescence tip containing the flower was removed and thetop 2 cm from the inflorescence stalk and the top two leaveswere used. The inflorescence stalk was cut into five 4 mm sections.The different plant parts were put into varying concentrations(0–1000 µM) of IAA, 2,4-D, NAA, or TRP in test tubesand treated as previously described. The tubes were then sealedwith serum caps, placed in the dark at 22±2 °C, andethylene analysed after 24 h. In order to determine the kineticsof induction, the effects of 100 µM IAA on ethylene inductionin inflorescences stalks and leaves were evaluated over a timecourse from 0 h to 26 h following treatment initiation underthe conditions previously described.

To establish if light had any effect on IAA-induced ethyleneproduction, inflorescences 4–6 cm in length with flowerspartially open were used from 35- to 45-d-old Arabidopsis plants.The inflorescence tip containing the flower was removed andthe top 2 cm from the inflorescence stalk and the top two leaveswere used. The inflorescence stalk was cut into five 4 mm sections.The different plant parts were put into 12x75 mm test tubescontaining 200 µl of 100 µM IAA or water, whichserved as a control, then sealed with serum caps, placed inthe light at 110 µmol m^–2 s^–1 with cool whitefluorescent lights or in darkness. The temperature was maintainedat 22±2 °C and ethylene analysed after 24 h.

To evaluate the effect of high temperature on IAA or wound-inducedethylene production, inflorescences 4–6 cm in length withflowers partially open were used from 35- to 45-d-old Arabidopsisplants. The inflorescence tip containing the flower was removedand the top 2 cm from the inflorescence stalk and the top twoleaves were used. The inflorescence stalk was cut into five4 mm sections. The different plant parts were put into 12x75mm test tubes containing 200 µl of 100 µM IAA orwater, which served as a control. Samples were put at 29, 37,or 43 °C in the dark for 15, 30, or 60 min, while the controlsamples were put in the dark at 22±2 °C. At the designatedtime interval, test tubes were removed from the heat chamber,allowed to cool for 10 min in the dark, and the heat-treatedsample with the appropriate control sealed with serum caps andput in the dark at 22±2 °C for a 24 h period priorto ethylene analysis.

The effects of varying concentrations of IAA alone or in combinationwith BL or BAP on ethylene production were evaluated in orderto determine the relationship between IAA and BL or BAP. Inflorescences,4–6 cm in length with flowers partially open, were usedfrom 35- to 45-d-old Arabidopsis plants. The inflorescence tipcontaining the flower was removed and the top 2 cm from theinflorescence stalk and the top two leaves were used. The inflorescencestalk was cut into five 4 mm sections. The different plant partswere put into 12x75 mm test tubes containing 200 µl ofvarying concentrations of IAA from 0 µM to 100 µMIAA alone or in combination with 2 µM BL or 10 µMBAP or water, which served as a control, then sealed with serumcaps and placed in the dark. The temperature was maintainedat 22±2 °C and ethylene analysed after 24 h.

Ethylene determinations
Ethylene was analysed with a Hewlett Packard 5890 gas chromatographequipped with a 1.83 mx3.175 mm o.d.x1.2 m stainless steel PorapakQ column. Injector port, flame ionization detector, and columntemperatures were 70, 200, and 70 °C, respectively. Headspacegases were evaluated at designated treatment times.

Results

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Different plant parts varied in IAA-induced ethylene production,inflorescence stalks showed the greatest induction, while allother plant parts tested produced significantly less (Table 1).Leaf age had an effect on IAA-induced ethylene production withthe youngest leaves showing the greatest stimulation, and, asthe age of the leaf increased, there was a reduction in theirability to produce ethylene (Table 2). When inflorescence stalksfrom Arabidopsis Columbia WT, which served as a control, andthree auxin-insensitive mutants were treated with 100 µMIAA, there was an increase in ethylene production in WT. However,reduced levels were produced in the auxin-insensitive mutants:axr1-12 produced slightly less IAA-induced ethylene than theWT control; axr1-3 produced lower levels of IAA-induced ethylenethan axr1-12; while axr2 barely produced detectable levels ofethylene (Fig. 1).

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Table 1. IAA-induced ethylene production in different Arabidopsis plant parts including root, young rosette leaves, inflorescence leaves, terminal inflorescence bud, lateral inflorescence bud, axillary leaf bud, primary inflorescence stalk, secondary inflorescence stalk, and lateral inflorescence stalk

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Table 2. Effects of leaf position on IAA-induced ethylene production in 24-d-old Arabidopsis plants

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Fig. 1. Effects of IAA on ethylene production in Arabidopsis Columbia WT and three auxin-insensitive mutants, axr1-12, axr1-3, and axr2. Inflorescences, 4–6 cm in length with flowers partially open, were taken from 35- to 45-d-old Arabidopsis plants. The inflorescence stalk was cut into five 4 mm sections and put in 12x75 mm test tubes containing 200 µl of 100 µM IAA (white columns) or water control (black columns). The tubes were then sealed, placed in the dark and ethylene analysed after 24 h. Values are expressed as the mean of four replications ±standard error.

The highest amount of IAA-induced ethylene production was producedin the root tip with regions below this producing less (Table 3).IAA-induced ethylene production was also greatest from the tipof the inflorescence stalk to 2 cm below the tip, and from thispoint down the length of the inflorescence there was a reductionin ethylene production (Table 4).

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Table 3. Ethylene production of roots of 24-d-old Arabidopsis plants grown hydroponically

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Table 4. Ethylene production of inflorescences, 10 cm in length with flowers partially open, taken from 35- to 45-d-old Arabidopsis plants

When inflorescence stalks were treated with IAA, 2,4-D, or NAAover a range of concentrations from 0 µM to 1000 µMthere was an increase in ethylene production starting at 1 µMwith increasingly greater responses up to 100 µM, followedby a plateau with the 500 µM treatment and a significantdecline at 1000 µM. Both 2,4-D and NAA elicited a greaterresponse than IAA at all concentrations tested in inflorescencestalks. Inflorescence leaves treated with IAA, 2,4-D, and NAAalso exhibited an increase in ethylene production at a 1 µMconcentration, reaching a maximum at 500 µM, and was followedby a significant decline at the 1000 µM concentration.Inflorescence leaves produced significantly less ethylene thanstalks at all concentrations of auxins tested. TRP did not induceethylene at concentrations from 1 µM to 1000 µMin inflorescence leaves or stalks (Fig. 2).

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Fig. 2. Effects of different auxins on ethylene production. Inflorescences, 4–6 cm in length with flowers partially open, were taken from 35- to 45-d-old Arabidopsis plants. The inflorescence tip containing the flower was removed and the top 2 cm from the inflorescence stalk (white columns) or the top two leaves (black columns) were used. The inflorescence stalk was cut into five 4 mm sections. The plant parts were put into varying concentrations of (A). IAA, (B) NAA, (C) 2,4-D, or (D) TRP in 12x75 mm test tubes containing 200 µl of treatment solution. The tubes were then sealed, placed in the dark, and ethylene analysed after 24 h. Values are expressed as the mean of four replications ±standard error.

Inflorescence stalks and leaves treated with 100 µM IAAexhibited a dramatic increase in ethylene production 2 h followingtreatment initiation. Inflorescence stalks showed a furtherincrease 4 h following treatment initiation with no furtherincrease at 6 h. Between 6 h and 24 h there was a decline inthe rate of ethylene production, while at the 26 h samplingthe rates of ethylene produced were the same as the 24 h readings.Inflorescence leaves exhibited similar rates of IAA-inducedethylene production between 2 h and 26 h following treatmentinitiation (Table 5).

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Table 5. Effects of IAA on ethylene production in inflorescence stalks and inflorescence leaves over a time course

When inflorescence stalks and leaves were treated with IAA andkept in the light there was a 36% reduction in IAA-induced ethyleneproduction in inflorescence stalks and a 28% reduction in theleaves as compared with plant parts kept in the dark (Table 6).When inflorescence stalks or leaves were treated at 43 °Cfor 30 min there was no effect on IAA-induced ethylene in theinflorescence stalk, while there was a 15% reduction in theleaves. After a 60 min treatment at 43 °C, IAA-induced ethyleneproduction was reduced 41% in the inflorescence stalks and 42%in the leaves (Table 7). When inflorescence stalks or leaveswere treated at 29 °C or 37 °C for 30–60 min,there was no effect on IAA-induced ethylene (data not shown).

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Table 6. Effects of light versus darkness on IAA-induced ethylene production

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Table 7. Effects of short-term exposure to high temperature on IAA-induced ethylene production

When 2 µM brassinolide (BL) or 10 µM 6-benzylaminopurine(BAP) were used alone to treat inflorescence stalks there wasno enhancement of ethylene production. However, when 2 µMBL was used in combination with 0.1, 1.0, or 10.0 µM IAAthere was a dramatic increase in ethylene production above theinduction promoted by the IAA treatment alone. At the highestconcentration of IAA (100 µM) tested there was no furtherenhancement of IAA-induced ethylene production by BL. BAP wasfound to be ineffective in the enhancement of IAA-induced ethyleneproduction (Table 8).

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Table 8. The effects of varying concentrations of IAA alone or in combination with BR or BAP on ethylene production

	Discussion

Top Abstract Introduction Materials and methods Results Discussion References

The plant can regulate ethylene internally, by non-stressfulenvironmental factors or a variety of stress factors. Internallycontrolled factors include the plants genetics, stage of development,ageing and senescence, type of organ, feedback regulation, and/orhormones. Regulation by non-stressful environmental factorsincludes temperature, light, oxygen, carbon dioxide, nutrition(both organic and inorganic), touch, gravity, and circadianrhythm. Stress factors regulating ethylene production are chillingand freezing stress, high temperature stress, excessive wateror flooding stress, drought stress, chemical stress, radiationstress, and/or mechanical stress. There are also a variety ofbiotic stresses including viral, bacterial, and fungal diseasesthat can induce ethylene production (Abeles et al., 1992). Thepurpose of this study was to evaluate which tissues were mostsensitive to plant hormones, the optimal conditions for theinduction of ethylene by different plant hormones, and the interactionsbetween the different plant hormones on the induction of ethylenein Arabidopsis, thereby establishing a model experimental system.By establishing this new and innovative model experimental systemin Arabidopsis, it will be possible to go into more depth asto how and why auxins and BR trigger ethylene production ingreen plants, utilizing genetic and molecular tools currentlyavailable when using Arabidopsis as an experimental organism.

The different plant hormones used to study ethylene productionin light-grown Arabidopsis plants were IAA, 2,4-D, NAA, BL,and BAP, each of which had been previously shown to stimulateethylene production in etiolated mung-bean segments (Abeles et al., 1992).

In this study, it has been shown that young leaves and the apicalportions of inflorescences and roots are most responsive toauxins, with inflorescences being the most responsive of thethree. These findings are in agreement with the literature whichshows that high rates of ethylene production are associatedwith actively dividing cells, as is the case in younger leaves(Abeles et al., 1992). In addition, it was shown that inflorescencestalks from auxin-insensitive mutants produced less IAA-inducedethylene than the WT controls. This is the first report, asfar as is known, that Arabidopsis inflorescence stalks are muchmore responsive to auxin treatment than any other plant part,and that inflorescence stalks from auxin-insensitive mutantsproduced less IAA-induced ethylene than the WT controls.

It has also been shown that both 2,4-D and NAA induce higherlevels of ethylene than IAA at all concentrations tested, inboth inflorescence stalks and leaves, while TRP did not promoteany stimulation. These results differ from previous work withetiolated mung-bean sprouts which showed that 100 µM IAApromoted higher levels of ethylene than either NAA or 2,4-D(Arteca et al., 1983). Also in this study it has been shownthat light causes a dramatic reduction in auxin-enhanced ethyleneproduction. This is the first report, as far as is known, onthe light inhibition of IAA-induced ethylene production in Arabidopsis.However, there are reports in the literature in other experimentalorganisms showing that light inhibits normal, and stress- andhormone-induced ethylene production in experimental systemssuch as soybean (Rodecap and Tingey, 1983), mung bean (Arteca and Bachman, 1987),tomato, sunflower, wheat and tobacco leaves (Delaat et al.,1981; Wright, 1981; Bassi and Spencer, 1983), which is in agreementwith the present findings. There are also reports which showthat light increases ethylene production in melon petioles (Toppan and Esquerre-Tugaye, 1984),bean-leaf discs (Porter et al., 1986), bromeliad plants (DeGreef et al., 1983),and sorghum seedlings (Craker et al., 1971), which does notagree with the present findings.

It has been shown that short-term heat treatments of 43.5 °Ccause a dramatic reduction in auxin-enhanced ethylene production,whereas temperatures at 29 °C and 37 °C have no effect.This is the first report, as far as is known, that short-termheat treatments inhibit auxin-induced ethylene production. Ithas been suggested that the optimal temperature for ethyleneproduction is near 30 °C and that the rate of ethylene productiondecreases beyond this point (Burg and Thimann, 1959); however,it has also been shown that heat treatment above 40 °C canstimulate ethylene production (Yang et al., 1990), which differsfrom the present results.

In this study, it has been shown that when BL or BAP were usedalone to treat Arabidopsis inflorescence stalks there was noenhancement of ethylene production. This differs from previouswork in etiolated mung beans showing that BL (Arteca et al., 1983)or BAP (Schlagnhaufer et al., 1984) alone stimulated ethyleneproduction. In this study, it was also shown that when BL wasused in combination with IAA there was a dramatic increase inethylene production above the induction promoted by the IAAtreatment alone, whereas BAP had no interactive effect. Thisis in agreement with the present findings that BL acts synergisticallywith IAA to stimulate ethylene production in etiolated mung-beansegments (Arteca et al., 1983). However, it is not in agreementwith previous results which showed that BAP interacts to stimulateethylene production in etiolated mung-bean segments (Schlagnhaufer et al., 1984).

In summary, both 2,4-D and NAA induce higher levels of ethylenethan IAA at all concentrations tested in both inflorescencestalks and leaves, while TRP did not promote any stimulation.Inflorescence stalks, including primary, secondary, and lateral,produced the greatest amount of ethylene in response to IAA,whereas all other plant parts tested produced significantlylower levels of ethylene in response to the hormone treatment.The apical portion of the inflorescence produced the highestlevels of IAA-induced ethylene with less ethylene produced assections were taken farther away from the tip. The inflorescencestalks from three auxin-insensitive mutants produced less IAA-inducedethylene than their WT control. Short-term heat treatments withhigh temperatures inhibited IAA-induced ethylene productionin both inflorescence stalks and leaves. Light also had an inhibitoryeffect on IAA-induced ethylene production. BL interacted withIAA to produce higher levels than either alone, while BAP hadno interactive effect. Future studies are now in progress tolook for changes in ethylene biosynthetic signalling genes inorder to better understand how auxins and BRs are triggeringethylene production at the molecular level. In addition, variousauxin-insensitive mutants will be studied in more depth andBR Arabidopsis mutants that are insensitive or do not producethese hormones will be evaluated for their ability to produceethylene in response to IAA or BL. With the data presented inthis paper there is now an excellent model system utilizingArabidopsis inflorescences that will enable us to explore inmore depth how and why auxins and BRs trigger ethylene productionand the signalling pathways involved.

Acknowledgements

This is contribution no. 463 of the Department of Horticulture,The Pennsylvania State University and was supported in partby the Pennsylvania Agricultural Experiment Station projectnumber 4106.

Abbreviations

BAP, 6-benzylaminopurine; BL, brassinolide; BR, brassinosteroid; 2,4-D, 2,4-dichlorophenoxyacetic acid; IAA, indole-3-acetic acid; NAA, naphthaleneacetic acid; TRP, tryptophan; WT, wild-type.

References

Top
Abstract
Introduction
Materials and methods
Results
Discussion
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Articles by Arteca, R. N.

Articles by Arteca, J. M.

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				E. W. Chehab, E. Eich, and J. Braam Thigmomorphogenesis: a complex plant response to mechano-stimulation J. Exp. Bot., January 1, 2009; 60(1): 43 - 56. [Abstract] [Full Text] [PDF]

Journal of Experimental Botany

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Effects of brassinosteroid, auxin, and cytokinin on ethylene production in Arabidopsis thaliana plants