The Phototropic Responses of Avena Coleoptiles

Macleod, K., Firn, R. D. and Digby, J. 1986. The phototropicresponses of Avena coleoptiles.—J. exp. Bot. 37: 542–548. A number of studies of the elongation rate changes causing phototropismhave been made but the findings of different groups have notbeen entirely Consistent. Studies of oat coleoptile phototropismin response to first-positive and second-positive doses indicatethat no single pattern of elongation rate changes causes phototropismeven in a single species. The relative effect of phototropicstimulation on the elongation rate at the shaded or the illuminatedside of coleoptiles subject to unilateral illumination dependson physiological state of the cell-for instance its positionin the elongation zone or whether it has been given red lightrecently. Models of phototropism will have to account for sucha diversity of phototropic responses. The importance of makingfull elongation rate measurements has once again been demonstrated. Key words: Phototropism, first-positive, second-positive, phytochrome, coleoptile, elongation rate     

Growth and Geotropic Responses of Avena Coleoptiles to 4-Amino-3,5,6-Trichloropicolinic Acid

The elongation and geotropic responses of coleoptile sections of Avena sativa L. to various concentrations of 4-amino-3,5,6-trichloropicolinic acid (Tordon) proved to be qualitatively similar to those previously reported for 2,3,6-trichlorobenzoic acid (TCBA). Tordon stimulated growth in a range of concentrations from 1 × 10^?6 to 1 × 10^?4M but higher concentrations were inhibitory. Geotropic curvature was extensively depressed by 1 × 10^?5 and 1 × 10^?4M Tordon, concentrations which accelerated elongation. A similar differential effect has been reported for TCBA and other auxins. Several other picolinic acids and related compounds were tested, but only very slight responses were noted.     

Effects of Electrolyte and Non-Electrolyte Solutions on the Tropic Responses of Avena Coleoptiles

Solutions of mannitol and carbowax 1540 reduced the geotropicresponse of Avena sativa coleoptiles to at least the same extentas a potassium chloride solution of equal osmotic potential.Similar results were obtained with the phototropic response.The magnitude of these decreases increased almost linearly withthe osmotic concentration of the solutions over the range 0.025–0.45J cm^–3. In contrast, the geotropic and phototropic responseswere scarcely affected by exposing the coleoptiles to solutionsof glycerol. The absence of an effect with glycerol is probably due to thepenetration of the coleoptile cells by this solute. The similaror greater reduction in tropic curvature brought about by mannitoland carbowax 1540 solutions, as compared with a potassium chloridesolution of equal osmotic potential, makes untenable a previoussuggestion attributing the inhibitory effects of electrolytesolutions to a shunting of the electro-potential differenceson the plant surface.     

The Effects of Paraffin Oil on Phototropic and Geotropic Responses in Avena Coleoptiles

Experiments are described which were designed to test the significanceof the coleoptile tip as the site of reception of light stimulusleading to negative photo-tropic response under paraffin oil.The results show clearly that the tip is of paramount importancein this respect. Further experiments in which the coleoptiletips were bisected in a plane at right angles to the light rayslend support to the hypothesis that negative phototropism underoil is related tolateral transport of material in the tip. Lastly,experiments which show that the geotropic response of coleoptilesis not reversed by immersion in oil are described. These findingsare discussed in relation to certain hypotheses concerning themechanism of negative phototropism under oil.     

DMPA and Avena Coleoptiles RNA Turn-over

Addition of α-methoxy-(3, 4-dichlorophenyl) acetic acid (DMPA) at different concentrations in the culture medium of sub-apical sections of Avena coleoptile results in an increased growth rate, which correspond to the quantitative measure of the increasing of ribosomal and soluble RNA turn-over. The relative decrease in total RNA synthesis observed for the supraoptimal DMPA concentration of 1000 μg/ml appears to be due to the specifical retardation in the 4 S RNA turn-over.     

Phytochrome-controlled Hydrogen Ion Excretion by Avena Coleoptiles

A red light-induced, far red reversible stimulation of proton efflux from apical segments of etiolated Avena sativa L. cv. Victory coleoptiles was observed. The acidification responses to red light and also to auxin were not the consequence of respired CO(2). The response to red light was strongly inhibited by cycloheximide and carbonyl cyanide, m-chlorophenyl hydrazone, but mannitol had a stimulatory effect. Red light and auxin applied together yielded a greater than additive response, in comparison to the effects of the two stimuli applied separately.     

Effects of Chlorpromazine on Gravitropism in Avena Coleoptiles

Chlorpromazine (CPZ), an inhibitor of the calcium-activatedform of calmodulin, is readily taken up by the roots of intactoat seedlings but poorly translocated from the roots to thecoleoptile of these plants. However, plants repeatedly rotatedthrough solutions containing low concentrations of CPZ (10^–8–10^–5M)are infiltrated, and under these conditions, CPZ significantlyinhibits the negative gravitropic response of the coleoptilewithout retarding elongation growth. This effect is observablein ‘decapitated’ (apical 1–2 mm removed) coleoptilesections and in intact whole coleoptiles. If exogenous auxinis supplied to the decapitated sections, both their growth ratesand gravitropic responsiveness are increased and, under theseconditions, CPZ can reduce the gravitropic curvature withoutreducing the overall growth rate. These results are discussedin relation to the possible role of calmodulin-dependent calcium-ionpumps in gravitropism. chlorpromazine, gravitropism, calmodulin, calcium, oat, Avena sativa     

Effect of Peeling on IAA-induced Growth in Avena Coleoptiles

The act of peeling removes the epidermis exclusively from Avenacoleoptiles. Peeling inhibits IAA-induced growth, by inhibitingthe growth of segments incubated in the presence of IAA, andpromoting that of those incubated in water. The magnitude ofthe inhibition of IAA-induced growth is proportional to theamount of epidermis removed. It is shown that neither lateralswelling, wounding, anaerobiosis, nor exposure to supraoptimalconcentrations of IAA cause the inhibition. It is concludedthat in Avena coleoptiles the epidermis regulates the rate ofexpansion of the underlying parenchyma cells and is the principaltarget of IAA-action. Avena sativa L., oat, coleoptile, indol-3-ylacetic acid, auxin, extension growth     

Calcium Requirement for Indoleacetic Acid-induced Acidification by Avena Coleoptiles

The ionic specificity of IAA-induced acidification by Avena coleoptiles was studied, using zwitterionic, presumably impermeant buffers. The acidification was almost totally dependent on divalent cations with an order of effectiveness of Ca(2+) >/= Sr(2+) > Mn(2+), Mg(2+); whereas other polyvalent cations tested were ineffective. The Ca(2+) response was IAA-dependent. The CaCl(2) concentration was optimal at 0.3 to 1 mm and inhibitory at higher concentrations. Sr(2+) inhibited Ca(2+)-dependent acidification and monovalent cations such as K(+) did not induce additional acidification in the presence of optimal CaCl(2). These data are consistent with a mechanism for IAA-induced acidification involving a Ca(2+) -H(+) exchange.     

Metabolism of Indole-3-acetaldehyde. III. Some Characteristics of the Aldehyde Oxidase of Avena Coleoptiles

Coleoptiles of Avena contain a soluble enzyme system, capable of oxidizing indoleacetaldehyde (lAAld) to indoleacetic acid (IAA). There is a gradient in the concentration of the enzyme along the length of the coleoptile and the first inter-node. The top 5 mm segment of each organ is relatively richer in this enzyme than the rest of the tissue. The enzyme was purified 17.7-fold by fractional precipitation with ammonium sulphate followed by gel filtration on Sephadex. Optimal pH for lAAld oxidation is ca. 4.4. Activity of the enzyme is normally oxygen obligatory. But, in the absence of oxygen, phenazine methosulphate (PMS) serves as hydrogen acceptor for aldehyde oxidation, but not some other dyes tried. Approximately one mole of oxygen was consumed for each mole of IAA formed. Formation of H₂O₂ could not be detected. Added H₂O₂ inhibited the reaction. Prolonged dialysis progressively inactivated the enzyme. Added NAD, NADP, FMN, FAD, cytochrome c, cyanoco-balamin, folic acid and ascorbic acid did not restore the lost activity. But 10^?3M cysteine restored about 60 % of the lost activity. The enzyme is an acidic protein, isoelectric at pH 4.05. For lAAld, under the conditions of experimentation, a Km of 3.45 × 10^?4M was calculated. Besides lAAld, indole-3-aldehyde and phenylacetaldehyde served as substrates, but not acetaldehyde, propionaldehyde, salicylaldehyde, xanthine, hypoxanthine or catechol. Cyanide, dithionite and mercapto-ethanol totally inactivated the enzyme depending upon the concentration and duration of treatment. X-ray irradiation up to a dosage of 2900 r promoted the lAAld oxidizing activity of cell-free preparations made from irradiated coleoptiles. As yet, no cofactor requirements have been found for the activity. The enzyme is unlikely to be a pyridino- or a flavoprotein.     

Ethylene Responses in Rice Roots and Coleoptiles Are Differentially Regulated by a Carotenoid Isomerase-Mediated Abscisic Acid Pathway

Ethylene and abscisic acid (ABA) act synergistically or antagonistically to regulate plant growth and development. ABA is derived from the carotenoid biosynthesis pathway. Here, we analyzed the interplay among ethylene, carotenoid biogenesis, and ABA in rice (Oryza sativa) using the rice ethylene response mutant mhz5, which displays a reduced ethylene response in roots but an enhanced ethylene response in coleoptiles. We found that MHZ5 encodes a carotenoid isomerase and that the mutation in mhz5 blocks carotenoid biosynthesis, reduces ABA accumulation, and promotes ethylene production in etiolated seedlings. ABA can largely rescue the ethylene response of the mhz5 mutant. Ethylene induces MHZ5 expression, the production of neoxanthin, an ABA biosynthesis precursor, and ABA accumulation in roots. MHZ5 overexpression results in enhanced ethylene sensitivity in roots and reduced ethylene sensitivity in coleoptiles. Mutation or overexpression of MHZ5 also alters the expression of ethylene-responsive genes. Genetic studies revealed that the MHZ5-mediated ABA pathway acts downstream of ethylene signaling to inhibit root growth. The MHZ5-mediated ABA pathway likely acts upstream but negatively regulates ethylene signaling to control coleoptile growth. Our study reveals novel interactions among ethylene, carotenogenesis, and ABA and provides insight into improvements in agronomic traits and adaptive growth through the manipulation of these pathways in rice.     

Isolation and Purification of an alpha-Mannosidase from Coleoptiles of Avena sativa

An alpha-mannosidase has been purified from the coleoptiles of Avena sativa L. var. Segrehavre. The enzyme, which is tightly associated with the cell wall, was solubilized with 3 m LiCl. The purification involves precipitation with (NH(4))(2)SO(4), gel filtration, ion exchange chromatography, and isoelectric focusing. The enzyme appears homogeneous when chromatographed on disc gels and on isoelectric focusing gels. The enzyme runs as a single protein of constant specific activity when chromatographed on Sephadex G-200. The estimated molecular weight of the enzyme is 630,000. The enzyme appears to have no metal ion cofactor requirement and is insensitive to p-chloromercuribenzoate. The pH optimum for the enzyme with p-nitrophenyl-alpha-d-mannoside as the substrate is 4.5 and the K(m) is 3.2 mm. The enzyme may have some carbohydrate associated with it as indicated by a positive periodate-Schiff reaction on disc gels.     

Inhibition of Low pH-induced Elongation in Avena Coleoptiles by Abscisic Acid

An angular position-sensing transducer was used to make continuous measurements of acid-induced elongation of Avena sativa coleoptile segments. Elongation rates at pH 4.5 (5 mm succinate buffer) were about 5-fold greater than those at pH 6.0. Buffered 0.1 mm abscisic acid produced a partial decrease of the growth rate. Pretreatments with abscisic acid buffered at pH 6.0 usually caused a further reduction of the elongation response when the coleoptile segments were subsequently placed in buffer at pH 4.5 containing abscisic acid. Abscisic acid did not completely prevent the pH effect in any of these experiments, and the brief latent period of the pH response was not affected by abscisic acid treatments. At pH 4.5, where the inhibitory effect of ABA was maximum, low pH-induced elongation was also inhibited by KCN and HgCl₂. These results suggest that pH-(4.5) induced elongation in this system may be dependent on some metabolic processes and that abscisic acid-induced inhibition of this elongation may involve an interaction with these processes.     

The Phototropic Response of Avena Coleoptiles following Localized Continuous Unilateral Illumination

When only part of the elongating zone on an Avena coleoptileis subject to continuous unilateral illumination, the majorphototropic response is restricted to the illuminated area.It is argued that previous studies have greatly exaggeratedthe contribution of any differential growth in non-illuminatedzones to the development of second positive phototropic curvature. Key words: Phototropism, Avena, Blue light, Growth rate