Relationship between endogenous ethylene production and natural
					defoliation traits during the maturation of sugarcane

Gao, Xin Xin; Fan, Xian; Dao, Jing Mei; Deng, Jun; Li, Ru Dan; Zhang, Yue Bin; Guo, Jia Wen; Liu, Shao Chun

doi:10.1590/1678-4499.0366

Abstract

The relationship between endogenous ethylene production and natural defoliation rate was examined in sugarcane cultivars with different natural defoliation traits. Ethylene production was examined at different positions on leaf sheaths and leaf scars at various sugarcane maturation stages using gas chromatography as an external standard method. During the sugarcane maturation process, ethylene production was greatest in the 2nd leaf sheath scar, followed by the 5th and 10th, in that order. It was also greatest during the early maturation stage, followed by the mid-maturation and harvest stages. Ethylene production of the leaf sheaths and leaf scars differed significantly among the sugarcane cultivars. Cultivars that defoliate easily produced significantly more ethylene than those that do not defoliate easily. The natural defoliation rates was greatest in the harvest stage, followed by mid-maturation and early maturation stage. Correlation analysis indicated that ethylene production was positively correlated with natural defoliation rates, particularly during early- and mid-maturation stages.

sugarcane maturity period; sheath and leaf scars; endogenous ethylene production; natural defoliation rate

1 INTRODUCTION

Sugarcane (Saccharum spp.) is the most important global sugar crop, accounting for 65% of the world’s sugar production. China is one of the world’s major sugar producers. In 2010, 166.7 million hectares were planted to sugarcane in China, and the annual national sugar production was 10.08 million tons. The sugarcane planting areas in China are located mainly in the tropics and subtropics south of 24 degree. In raw sugar production, natural defoliation at the maturation stage affects the efficiency of the sugarcane harvesting process, especially in countries growing mountain sugarcane. Few machines can be used for harvesting sugarcane in China because this crop is planted mainly on hillsides. In manual sugarcane processing, manual peeling of the leaves accounts for 65% of the entire labor involved in the harvest process (Shukla et al., 1991Shukla, L. N., Irvinder, S., & Sandhar, N. S. (1991). Design development and testing of sugarcane cleaner. Agricultural Mechanization in Asia, 22, 55-58.; Singh et al., 2011Singh, J., Singh, A. K., Sharma, M. P., Singh, P. R., & Srivastava, A. C (2011). Mechanization of Sugarcane cultivation in India. Sugar Tech, 13, 310-314. http://dx.doi.org/10.1007/s12355-011-0101-5.
http://dx.doi.org/10.1007/s12355-011-010... ; Srivastava & Kishan, 1990Srivastava, A. C., & Kishan, S. (1990). Development of a power-driven sugarcane detrasher. Agricultural Mechanization in Asia, 21, 49-52.).

Sugarcane leaves are composed of a leaf blade and leaf sheath. During the maturation period, mature leaf sheaths naturally pull away from sugarcane stems and defoliate; however, different sugarcane cultivars have shown considerable variation in the rate of natural defoliation. Some high-yielding sugarcane clones are often eliminated from agriculture practice due to their poor natural defoliation traits. In recent years, in part because of rising labor costs, the breeding of cultivars with improved defoliation traits and research into agronomic technology for the regulation of defoliation have gained increasing interest.

International and domestic studies have indicated that ethylene plays an important role in the shedding process of plant organs and as a natural regulator of plant organ defoliation (Patterson, 2001Patterson, S. E. (2001). Cutting loose. Abscission and dehiscence in Arabidopsis. Plant Physiology, 126, 494-500. http://dx.doi.org/10.1104/pp.126.2.494. PMid:11402180
http://dx.doi.org/10.1104/pp.126.2.494... ; Taylor & Whitelaw, 2001Taylor, J. E., & Whitelaw, C. A. (2001). Signals in abscission. The New Phytologist, 151, 323-340. http://dx.doi.org/10.1046/j.0028-646x.2001.00194.x.
http://dx.doi.org/10.1046/j.0028-646x.20... ). The abscission layer cells in the leaf sheath can regulate endogenous ethylene production to induce the expression of genes related to shedding by sensing signals of defoliation (Goto et al., 1980Goto, M., Yaguchi, Y., & Hyodo, H. (1980). Ethylene production in citrus leaves infected with Xanthomonas citri and its relation to defoliation. Physiological Plant Pathology, 16, 343-350. http://dx.doi.org/10.1016/S0048-4059(80)80006-3.
http://dx.doi.org/10.1016/S0048-4059(80)... ; Lu et al., 1997Lu, D. Z., Fu, J. R., & Song, S. Q. (1997). Plant senescence and Its regulation. Beijing: China Agriculture Press, p. 65-92.; Schupp & Greene, 2004Schupp, J. R., & Greene, D. W. (2004). Effect of aminoethoxyvinylglycine (AVG) on preharvest drop, fruit quality, and maturation of ‘McIntosh’ apples. I. Concentration and timing of dilute applications of AVG. HortScience, 39, 1030-1035.; Uthaichay et al., 2007Uthaichay, N., Ketsa, S., & van Doorn, W. G. (2007). G.1-MCP pretreatment prevents bud and flower abscission in Dendrobium orchids. Postharvest Biology and Technology, 43, 374-380. http://dx.doi.org/10.1016/j.postharvbio.2006.09.015.
http://dx.doi.org/10.1016/j.postharvbio.... ). Ethylene can improve enzyme degradation activity in plant cell walls in the organ abscission layer, and the degrading enzymes accumulate in the cell wall, promoting degradation of the cell wall and middle lamella, which causes abscission (Campillo & Bennett 1996Campillo, E., & Bennett, A. B. (1996). Pedicel breakstrength and cellulase gene expression during tomato flower abscission. Plant Physiology, 111, 813-820. http://dx.doi.org/10.1104/pp.111.3.813. PMid:8754682
http://dx.doi.org/10.1104/pp.111.3.813... ; González-Carranza et al., 1998González-Carranza, Z. H., Lozoya-Gloria, E., & Roberts, J. A. (1998). Recent development s in abscission: shedding light on the shedding process. Trends in Plant Science, 3, 10-14. http://dx.doi.org/10.1016/S1360-1385(97)01132-1.
http://dx.doi.org/10.1016/S1360-1385(97)... ; Mishra et al., 2008Mishra, A., Khare, S., Trivedi, P. K., & Nath, P. (2008). Effect of ethylene, 1-MCP, ABA and IAA on break strength, cellulase and polygalacturonase activities during cotton leaf abscission. South African Journal of Botany, 74, 282-287. http://dx.doi.org/10.1016/j.sajb.2007.12.001.
http://dx.doi.org/10.1016/j.sajb.2007.12... ). The production of ethylene significantly affects plant organ shedding. In citrus fruits during the early stage of abscission, ethylene promotes organ shedding at low concentrations but inhibits it at high concentrations (Abeles et al., 1992Abeles, F. B., Morgan, P. W., & Saltveit, M. E. (1992). Ethylene in plant biology. (p. 135-159). New York: Academic Press. ; Plummer et al., 1991Plummer, J. A., Mullins, M. G., & Vine, J. H. (1991). Seasonal changes in endogenous ABA and IAA and the influence of applied ABA and auxin in relation to shoot growth and abscission in Valencia Orange. Plant Growth Regulation, 10, 139-151. http://dx.doi.org/10.1007/BF00024960.
http://dx.doi.org/10.1007/BF00024960... ). Spraying low concentrations of ethylene on bean leaves can artificially induce bean leaf shedding (Jackson & Osborne, 1970Jackson, M. B., & Osborne, D. J. (1970). Ethylene, the natural regulator of leaf abscission. Nature, 225, 1019-1022. http://dx.doi.org/10.1038/2251019a0. PMid:16056901
http://dx.doi.org/10.1038/2251019a0... ). In addition, the application of appropriate concentrations of the ethylene biosynthesis inhibitor AVG (Aminoethoxyvinylglycin) to apple trees caused a reduction in fruit ethylene production and a significant delay in fruit shedding (Schupp & Greene, 2004Schupp, J. R., & Greene, D. W. (2004). Effect of aminoethoxyvinylglycine (AVG) on preharvest drop, fruit quality, and maturation of ‘McIntosh’ apples. I. Concentration and timing of dilute applications of AVG. HortScience, 39, 1030-1035.). However, the spraying of high quantities of ethylene onto citrus fruits has little effect on fruit stalk abscission (Patterson & Bleecker, 2004Patterson, S. E., & Bleecker, A. B. (2004). Ethylene-dependent and -independent processes associated with floral organ abscission in Arabidopsis. Plant Physiology, 134, 194-203. http://dx.doi.org/10.1104/pp.103.028027. PMid:14701913
http://dx.doi.org/10.1104/pp.103.028027... ). The effect of exogenous ethylene has been studied on sugarcane tillering (Mishra et al., 2014Mishra, S., Nailwal, T. K., & Pant, R. C. (2014). In vitro study of role of ethylene during tillering in sugarcane. Sugar Tech, 16, 255-263. http://dx.doi.org/10.1007/s12355-013-0251-8.
http://dx.doi.org/10.1007/s12355-013-025... ), sugar accumulation (Fong Chong et al., 2010Fong Chong, B., Mills, E., Bonnett, G. D., & Gnanasambandam, A. (2010). Early exposure to ethylene modifies shoot development and increases sucrose accumulation rate in sugarcane. Journal of Plant Growth Regulation, 29, 149-163. http://dx.doi.org/10.1007/s00344-009-9118-3.
http://dx.doi.org/10.1007/s00344-009-911... ; Wang et al., 2008Wang, A. Q., Fan, Y. G., Zhao, X. Y., He, L. F., Yang, L. T., & Li, Y. R. (2008). The relationship between Ethylene induced three members of ACC synthase gene family to express in the stem and ethylene production as well as sugar accumulation in sugarcane. Crop Science, 34, 418-422.), and drought resistance (Ye et al., 2005Ye, Y. P., Li, Y. R., Luo, T., Pang, G. Y., & Yang, L. T. (2005). Influence of ethylene pretreatment with seeds on drought resistance. Chinese Agricultural Science Bulletin, 6, 387-389.), but no previous studies on the regulation of sugarcane defoliation have been reported. Information on the relationship between endogenous ethylene production and intrinsic natural defoliation traits relevant to sugarcane maturation is of great significance.

Here, we studied the relationship between the amount of ethylene released by different leaf sheaths and leaf scars and the natural leaf defoliation rate during the maturation process of different sugarcane cultivars. The objective of this study was to determine the physiological index, which influences the defoliation traits of sugarcane and may provide information that will facilitate the development of agronomic techniques for promoting natural defoliation.

2 MATERIAL AND METHOD

Sugarcane cultivars

The easy-to-defoliate sugarcane cultivars CYZ03-194 and CMT69-421, and difficult-to-defoliate cultivars GT02-467 and CYZ99-91 were used in this study. Their leaf sheaths are of similar size and they reach maturity at the same time (maturity lasts from November to January). As shown in figure 1, the leaf sheaths and leaf scars of the easy-to-defoliate sugarcane cultivars cracked easily, but those of the difficult-to-defoliate cultivars did not. The characteristics of the experimental soil are as follows: 20.5 g kg^–1 organic matter, 1.64 g kg^–1 total nitrogen, 0.67 g kg^–1 total phosphorus, 13.7 g kg^–1 total potassium, 80.79 mg kg^–1 available nitrogen, 9.81 mg kg^–1 available phosphorus, 112.78 mg kg^-1 available potassium, and pH 6.0. The number of sugarcane buds was 120000/hm² and rows were spaced 1 m apart. Fertilizer was applied at the following rates: 345 kg N/hm², 108 kg P₂O₅/hm² and 110 kg K₂O/hm². The sugarcane was irrigated six times at a rate of 225 m³/hm² each time. Sugarcane samples were collected during the early maturation stage (November 30, 2012), mid-maturation stage (December 30, 2012), and harvest stage (January 30, 2013). Ten plants were selected from each variety and the leaf scar tissues of each plant at the 2^nd, 5^th, and 10^th leaves from the top visible hypertrophy ring were cut 1 cm above the leaf scar, and 2 cm of the leaf sheath was cut below the leaf scar. Samples were collected between 8–9:00 a.m. and were immediately placed into ethylene bottles and sealed. Ethylene was collected for 4 h and the amount of ethylene released was measured. The measurements were repeated three times. Total expanded leaves of each plant and abscised leaves were surveyed to calculate the defoliation rate for all sample plants. Defoliation rate = natural defoliation/total number of leaves × 100.

Figure 1
Abscission zone at the 10^th leaf in four different cultivars.

Determination of ethylene production

A Shimadzu 2014 gas chromatograph was used to determine ethylene production. The GC chromatographic conditions were as follows: RT-Q-BOND (30 m × 0.53 mm × 20 μm); inlet temperature: 100 °C; detector temperature: 200 °C; carrier gas (N₂) flow rate: 1.8 mL/min; aid gas flow: air, 400 mL/min, hydrogen, 30 mL/min; makeup gas (N₂): 30 mL/min; split ratio: 5:1; oven temperature: 50 °C for 4 min. The external standard method was used; the retention time of the standard sample was used to assess quality, and the peak area was calculated to assess quantity and therefore overall ethylene production.

Data analysis

Test results were analyzed using Excel 2003 and SPSS 19.0 statistical software. The statistical method used was a single-factor analysis of variance (ANOVA), and LSD was used to test significance at a p<0.01 level.

3 RESULTS

Validation of ethylene GC detection methods

Ethylene gas chromatography measurements were conducted on a standard ethylene sample (>99.95%) and fresh sugarcane test samples. As shown in figure 2, the ethylene peak retention time was 3.350 min, the peak shape was good, there was no interference from other substances, and the time of the peak appearance was short and highly precise. The standard curve of ethylene concentration vs. the peak area is described using the following equation: Y = 0.0068X-3.2119 (Y, concentration; X, peak area), R² = 0.9998, with an 88% recovery rate. The fresh sugarcane test tissue samples were measured six times in parallel to calculate the standard deviation (SD) and relative standard deviation (RSD). The average concentration of the six test samples was 0.0184 μl/L, with an SD of 0.00052 and an RSD of 2.24%. The data indicated a high ethylene correlation coefficient, high sample recovery, and considerable reproducibility, which meets the test requirements and indicates that this method is suitable for the quantitative analysis of sugarcane ethylene production.

Figure 2
Electropherogram of ethylene.

Natural defoliation rate

During the maturity process, the natural defoliation rates of four sugarcane cultivars was greatest in the harvest stage, followed by mid-maturation and early maturation stage. As shown in figure 3, the natural defoliation rates differed significantly between the cultivars at different stages of maturation, It was greatest for the cultivar of GT02-467, followed by CYZ99-91, CMT69-421 and CYZ03-194. The natural defoliation rates increased as the maturation process progressed, and the high rates of defoliation differed significantly between stages. Specifically, the defoliation rate of CYZ03-194 at the harvest stage was 13.32% and 6.59% higher than the mid-maturation and early maturation stages, respectively; the defoliation rate of CMT69-421 at the harvest stage was 16.16% and 7.52% higher than the mid-maturation and early maturation stages, respectively; the defoliation rate of GT02-467 was 8.26% and 2.91% higher than the mid-maturation and early maturation stages, respectively; the defoliation rate of CYZ99-91 was 5.84% and 0.47% higher than the mid-maturation and early maturation stages, respectively. The magnitude of increase in defoliation rate from highest to lowest was CYZ03-194 > CMT69-421 > CYZ99-91 > GT02-467.

Figure 3
Leaf defoliation rate of four sugarcane cultivars during different periods. Upper- and lowercase letters within a column indicate significance levels of 0.01 and 0.05, respectively

Ethylene production by leaf sheaths at the mature stage

During the process of maturation, ethylene production at the same leaf positions differed significantly between the four cultivars (Table 1). There was higher ethylene production in young leaves than in mature leaves. It was greatest in the 2nd leaf sheath scar, followed by the 5th and 10th. With respect to different cultivars and leaf locations, ethylene production of CYZ03-194 was greatest, followed by CMT69-421, GT02-467 and CYZ99-91, for the 2^nd, 5^th, and 10^th leaves at the early maturation stage and for the 2^nd and 5^th leaves at the mid-maturation and harvest stages. Ethylene production was significantly higher in the easy-to-defoliate cultivars CYZ03-194 and CMT69-421 than in the difficult-to-defoliate cultivars GT02-467 and CYZ99-91 in the 2^nd, 5^th, and 10^th leaves during the early maturation stage, in the 5^th leaves during the mid-maturation stage, and in the 2^nd and 5^th leaves during the harvest stage. At the mid-maturation and harvest stages, ethylene production of the 10^th leaves was below the detection limits for all four cultivars. At this stage, the sugarcane continued to mature, and the 10^th leaf sheath tissues showed accelerated aging and became yellowish, which may have caused ethylene production to fall below the detection values. During the cane maturation process, less ethylene was released by the sheath at harvest stage than other times for all leaves except the 10^th leaf.

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Table 1
Ethylene production by leaf sheaths of different sugarcane cultivars

Ethylene production by leaf scars at the mature stage

During the cane maturation process, the release of ethylene by leaf scars followed the same trend as the leaf sheaths, i.e., there was a decline in the amount of ethylene released as the canes matured (Table 2). Ethylene production was significantly different between all four cultivars at the same leaf positions. Ethylene production of CYZ03-194 was greatest, followed by CMT69-421, GT02-467 and CYZ99-91 for all leaf scar positions and maturation stages, and the differences were significant. Ethylene production by the easy-to-defoliate cultivars CYZ03-194 and CMT69-421 was significantly higher than that of the difficult-to-defoliate cultivars GT02-467 and CYZ99-91. Young leaves produced significantly more ethylene compared with mature leaves. The results were similar to those recorded for leaf sheaths, which might be related to the degree of maturity and aging status of the leaf scar tissue.

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Table 2
Ethylene production by leaf scars of different sugarcane cultivars

Correlation analysis between ethylene production by leaf sheaths and leaf scars and defoliation rate during maturation

Ethylene production was evaluated in four sugarcane cultivars during the same period in the maturation process. The corresponding natural defoliation rate was used for correlation analysis, which showed that ethylene production of different leaf sheaths and leaf scars were positively correlated with the natural defoliation rate. During the early maturation and mid-maturation stages, ethylene produced by leaf sheaths and leaf scars was significantly positively correlated with the natural defoliation rate (Table 3). At the harvest stage, ethylene production from the leaf sheath and leaf scars was not significantly related to the defoliation rates. This may be because both sheaths and scars mature during the harvest stage when ethylene production declines.

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Table 3
Correlation analysis of ethylene produced by leaf sheaths and leaf scars and defoliation rates

4 DISCUSSION

The shedding of plant organs is a complex physiological process. During abscission, an abscission zone is formed at the base area and hormones, enzymes, and other regulatory substances complete the process of leaf shedding (Hadfield & Bennett, 1998Hadfield, K. A., & Bennett, A. B. (1998). Polygalacturonases: many genes in search of a function. Plant Physiology, 117, 337-343. http://dx.doi.org/10.1104/pp.117.2.337. PMid:9625687
http://dx.doi.org/10.1104/pp.117.2.337... ; Kalaitzis et al., 1997Kalaitzis, P., Solomos, T., & Tucker, M. L. (1997). Three different polygalacturonases are expressed in tomato leaf and flower abscission, each with a different temporal expression pattern. Plant Physiology, 113, 1303-1308. http://dx.doi.org/10.1104/pp.113.4.1303. PMid:9112778
http://dx.doi.org/10.1104/pp.113.4.1303... ; McManus, 2008McManus, M. T. (2008). Further examination of abscission zone cells as ethylene target cells in higher plants. Annals of Botany, 101, 285-292. http://dx.doi.org/10.1093/aob/mcm269. PMid:17965027
http://dx.doi.org/10.1093/aob/mcm269... ; Tabuchi et al., 2000Tabuchi, T., Ito, S., & Arai, N. (2000). Development of the abscission zones in pedicels of galapagos wild tomatoes. CAB Direct, 69, 443-445.). Ethylene is one of the most important hormones involved in the regulation of plant organ shedding. This hormone acts directly on the genes encoding cellulase and polygalacturonase, which are closely related to shedding. In addition, ethylene can regulate and control the genes encoding glutathione S-transferase, actin-related proteins, and the light-harvesting complex, which are closely correlated with resistance in sugarcane plants.

Numerous studies have shown that ethylene is an important regulatory hormone affecting the shedding of plant organs. In previous work, spraying 20 μL/L ethylene on tomato pedicellariae significantly improved the abscission rate (Wei et al., 2011Wei, Y. W., Deng, Z. N., Hung, C. M., & Li, Y. R. (2011). Ethephon regulated differential gene expression in sugarcane. Journal of Southern Agriculture, 1, 6-10.). At all levels of maturity in the current study, more ethylene was produced by the leaf sheaths and leaf scars of easy-to-defoliate cultivars than by those of difficult-to-defoliate cultivars. During maturation, ethylene production by leaf sheaths and leaf scars of different cultivars was positively correlated with the defoliation rate; these correlations were significant during the early maturation and mid-maturation stages (Table 3). This finding is consistent with results reported for tomatoes, mung beans, and apples (Decoteau & Craker, 1987Decoteau, D. R., & Craker, L. E. (1987). Abscission: ethylene and light control. Plant Physiology, 83, 970-972. http://dx.doi.org/10.1104/pp.83.4.970. PMid:16665373
http://dx.doi.org/10.1104/pp.83.4.970... ; Michael, 1985Michael, S. R. (1985). Ethylene and abscission. HortScience, 20, 45-50.; Wang et al., 2003Wang, Y. C., Li, T. L., & Hou, J. P. (2003). The impact of Ethylene processing on Tomato Pedicel shedding. Gardening Journal, 5, 554-558.) and suggests that increased endogenous ethylene production of leaf sheaths and leaf scars helps to regulate and control the defoliation rate. Previous studies in citrus fruits have shown ethylene promotes shedding at low concentrations but inhibits it at high concentrations (Abeles et al., 1992Abeles, F. B., Morgan, P. W., & Saltveit, M. E. (1992). Ethylene in plant biology. (p. 135-159). New York: Academic Press. ; Plummer et al., 1991Plummer, J. A., Mullins, M. G., & Vine, J. H. (1991). Seasonal changes in endogenous ABA and IAA and the influence of applied ABA and auxin in relation to shoot growth and abscission in Valencia Orange. Plant Growth Regulation, 10, 139-151. http://dx.doi.org/10.1007/BF00024960.
http://dx.doi.org/10.1007/BF00024960... ). Ethylene production by mature leaf sheaths and leaf scars showed a gradual declining trend. Similarly, natural defoliation only occurred at relatively low leaf positions with low ethylene production and did not occur at all at the high leaf positions where there was greater ethylene production. This suggests that high concentrations of ethylene have no effect on defoliation, but these results are limited to endogenous ethylene. It is necessary to conduct experiments to validate the role of exogenous ethylene and to clearly quantify the role of ethylene in the regulation of cane defoliation traits.

Previous studies have shown that ethylene is produced in all living plant cells (Uheda & Nakamura, 2000Uheda, E., & Nakamura, S. (2000). Abscission of Azolla branches induced by ethylene and sodium azide. Plant & Cell Physiology, 41, 1365-1372. http://dx.doi.org/10.1093/pcp/pcd071. PMid:11134422
http://dx.doi.org/10.1093/pcp/pcd071... ). More ethylene was produced by cucumber leaves at higher positions compared with lower positions (Zheng et al., 2003Zheng, Z. Y., Sun, X. L., Liu, S. Q., & Gao, J. F. (2003). Preliminary study on ethylene distribution and dynamic annual variations in cucumber. Shandong Agricultural Sciences, 4, 15-17.). In the current study, more ethylene was emitted by young leaf sheaths and scars than by mature leaf sheaths. Later, during the mid-maturation stage, ethylene production by the 10^th leaf sheath was below the detection limit. This may be because the upper leaf sheath tissues are younger and contain more living cells. Auxins can inhibit the shedding of plant organs (Abebie et al., 2008Abebie, B., Lers, A., Philosoph-Hadas, S., Goren, R., Riov, J., & Meir, S. (2008). Differential effects of NAA and 2,4-D in reducing floret abscission in cestrum (Cestrum elegans) cut flowers are associated with their differential activation of Aux/IAA homologous genes homologousgenes. Annals of Botany, 101, 249-259.), and there is antagonism between auxin and ethylene. Young leaves have a higher auxin content than mature leaves, which is why the abscission layer cells of young leaves are not as sensitive to ethylene compared with mature leaves (Meir et al., 2010Meir, S., Philosoph-Hadas, S., Sundaresan, S., Selvaraj, K. S., Burd, S., Ophir, R., Kochanek, B., Reid, M. S., Jiang, C. Z., & Lers, A. (2010). Microarray analysis of the abscission-related transcriptome in the tomato flower abscission zone in response to auxin depletion. Plant Physiology, 154, 1929-1956. http://dx.doi.org/10.1104/pp.110.160697. PMid:20947671
http://dx.doi.org/10.1104/pp.110.160697... ). During the maturation process in the current study, natural cane defoliation always occurred in mature leaves, and there was significantly more ethylene production by young leaves than mature leaves; however, no defoliation was observed in the young leaf sheaths. It is possible that the auxin content of the upper young leaves was higher than the mature leaves.

5 CONCLUSION

There was a close correlation between the natural defoliation rate and endogenous ethylene production by leaf sheaths and leaf scars of mature sugarcane. An appropriate level of endogenous ethylene production was the physiological basis for the increased rate of natural defoliation, and the natural cane defoliation always occurred at the early stages of maturation. With the use of agronomic technology, exogenous ethylene may be suitable for regulating defoliation in sugarcane. Promoting endogenous ethylene production in an appropriate range during the early- and mid-stages of maturation can improve the natural defoliation rate of sugarcane. This may help solve the problem of defoliation in sugarcane harvesting.

ACKNOWLEDGEMENTS

This study was supported by the Earmarked Fund for National Natural Science Foundation of China (31160257).

REFERENCES

Abebie, B., Lers, A., Philosoph-Hadas, S., Goren, R., Riov, J., & Meir, S. (2008). Differential effects of NAA and 2,4-D in reducing floret abscission in cestrum (Cestrum elegans) cut flowers are associated with their differential activation of Aux/IAA homologous genes homologousgenes. Annals of Botany, 101, 249-259.
Abeles, F. B., Morgan, P. W., & Saltveit, M. E. (1992). Ethylene in plant biology. (p. 135-159). New York: Academic Press.
Campillo, E., & Bennett, A. B. (1996). Pedicel breakstrength and cellulase gene expression during tomato flower abscission. Plant Physiology, 111, 813-820. http://dx.doi.org/10.1104/pp.111.3.813. PMid:8754682
» http://dx.doi.org/10.1104/pp.111.3.813
Decoteau, D. R., & Craker, L. E. (1987). Abscission: ethylene and light control. Plant Physiology, 83, 970-972. http://dx.doi.org/10.1104/pp.83.4.970. PMid:16665373
» http://dx.doi.org/10.1104/pp.83.4.970
Fong Chong, B., Mills, E., Bonnett, G. D., & Gnanasambandam, A. (2010). Early exposure to ethylene modifies shoot development and increases sucrose accumulation rate in sugarcane. Journal of Plant Growth Regulation, 29, 149-163. http://dx.doi.org/10.1007/s00344-009-9118-3.
» http://dx.doi.org/10.1007/s00344-009-9118-3
González-Carranza, Z. H., Lozoya-Gloria, E., & Roberts, J. A. (1998). Recent development s in abscission: shedding light on the shedding process. Trends in Plant Science, 3, 10-14. http://dx.doi.org/10.1016/S1360-1385(97)01132-1.
» http://dx.doi.org/10.1016/S1360-1385(97)01132-1
Goto, M., Yaguchi, Y., & Hyodo, H. (1980). Ethylene production in citrus leaves infected with Xanthomonas citri and its relation to defoliation. Physiological Plant Pathology, 16, 343-350. http://dx.doi.org/10.1016/S0048-4059(80)80006-3.
» http://dx.doi.org/10.1016/S0048-4059(80)80006-3
Hadfield, K. A., & Bennett, A. B. (1998). Polygalacturonases: many genes in search of a function. Plant Physiology, 117, 337-343. http://dx.doi.org/10.1104/pp.117.2.337. PMid:9625687
» http://dx.doi.org/10.1104/pp.117.2.337
Jackson, M. B., & Osborne, D. J. (1970). Ethylene, the natural regulator of leaf abscission. Nature, 225, 1019-1022. http://dx.doi.org/10.1038/2251019a0. PMid:16056901
» http://dx.doi.org/10.1038/2251019a0
Kalaitzis, P., Solomos, T., & Tucker, M. L. (1997). Three different polygalacturonases are expressed in tomato leaf and flower abscission, each with a different temporal expression pattern. Plant Physiology, 113, 1303-1308. http://dx.doi.org/10.1104/pp.113.4.1303. PMid:9112778
» http://dx.doi.org/10.1104/pp.113.4.1303
Lu, D. Z., Fu, J. R., & Song, S. Q. (1997). Plant senescence and Its regulation. Beijing: China Agriculture Press, p. 65-92.
McManus, M. T. (2008). Further examination of abscission zone cells as ethylene target cells in higher plants. Annals of Botany, 101, 285-292. http://dx.doi.org/10.1093/aob/mcm269. PMid:17965027
» http://dx.doi.org/10.1093/aob/mcm269
Meir, S., Philosoph-Hadas, S., Sundaresan, S., Selvaraj, K. S., Burd, S., Ophir, R., Kochanek, B., Reid, M. S., Jiang, C. Z., & Lers, A. (2010). Microarray analysis of the abscission-related transcriptome in the tomato flower abscission zone in response to auxin depletion. Plant Physiology, 154, 1929-1956. http://dx.doi.org/10.1104/pp.110.160697. PMid:20947671
» http://dx.doi.org/10.1104/pp.110.160697
Michael, S. R. (1985). Ethylene and abscission. HortScience, 20, 45-50.
Mishra, A., Khare, S., Trivedi, P. K., & Nath, P. (2008). Effect of ethylene, 1-MCP, ABA and IAA on break strength, cellulase and polygalacturonase activities during cotton leaf abscission. South African Journal of Botany, 74, 282-287. http://dx.doi.org/10.1016/j.sajb.2007.12.001.
» http://dx.doi.org/10.1016/j.sajb.2007.12.001
Mishra, S., Nailwal, T. K., & Pant, R. C. (2014). In vitro study of role of ethylene during tillering in sugarcane. Sugar Tech, 16, 255-263. http://dx.doi.org/10.1007/s12355-013-0251-8.
» http://dx.doi.org/10.1007/s12355-013-0251-8
Patterson, S. E. (2001). Cutting loose. Abscission and dehiscence in Arabidopsis. Plant Physiology, 126, 494-500. http://dx.doi.org/10.1104/pp.126.2.494. PMid:11402180
» http://dx.doi.org/10.1104/pp.126.2.494
Patterson, S. E., & Bleecker, A. B. (2004). Ethylene-dependent and -independent processes associated with floral organ abscission in Arabidopsis. Plant Physiology, 134, 194-203. http://dx.doi.org/10.1104/pp.103.028027. PMid:14701913
» http://dx.doi.org/10.1104/pp.103.028027
Plummer, J. A., Mullins, M. G., & Vine, J. H. (1991). Seasonal changes in endogenous ABA and IAA and the influence of applied ABA and auxin in relation to shoot growth and abscission in Valencia Orange. Plant Growth Regulation, 10, 139-151. http://dx.doi.org/10.1007/BF00024960.
» http://dx.doi.org/10.1007/BF00024960
Schupp, J. R., & Greene, D. W. (2004). Effect of aminoethoxyvinylglycine (AVG) on preharvest drop, fruit quality, and maturation of ‘McIntosh’ apples. I. Concentration and timing of dilute applications of AVG. HortScience, 39, 1030-1035.
Shukla, L. N., Irvinder, S., & Sandhar, N. S. (1991). Design development and testing of sugarcane cleaner. Agricultural Mechanization in Asia, 22, 55-58.
Singh, J., Singh, A. K., Sharma, M. P., Singh, P. R., & Srivastava, A. C (2011). Mechanization of Sugarcane cultivation in India. Sugar Tech, 13, 310-314. http://dx.doi.org/10.1007/s12355-011-0101-5.
» http://dx.doi.org/10.1007/s12355-011-0101-5
Srivastava, A. C., & Kishan, S. (1990). Development of a power-driven sugarcane detrasher. Agricultural Mechanization in Asia, 21, 49-52.
Tabuchi, T., Ito, S., & Arai, N. (2000). Development of the abscission zones in pedicels of galapagos wild tomatoes. CAB Direct, 69, 443-445.
Taylor, J. E., & Whitelaw, C. A. (2001). Signals in abscission. The New Phytologist, 151, 323-340. http://dx.doi.org/10.1046/j.0028-646x.2001.00194.x.
» http://dx.doi.org/10.1046/j.0028-646x.2001.00194.x
Uheda, E., & Nakamura, S. (2000). Abscission of Azolla branches induced by ethylene and sodium azide. Plant & Cell Physiology, 41, 1365-1372. http://dx.doi.org/10.1093/pcp/pcd071. PMid:11134422
» http://dx.doi.org/10.1093/pcp/pcd071
Uthaichay, N., Ketsa, S., & van Doorn, W. G. (2007). G.1-MCP pretreatment prevents bud and flower abscission in Dendrobium orchids. Postharvest Biology and Technology, 43, 374-380. http://dx.doi.org/10.1016/j.postharvbio.2006.09.015.
» http://dx.doi.org/10.1016/j.postharvbio.2006.09.015
Wang, A. Q., Fan, Y. G., Zhao, X. Y., He, L. F., Yang, L. T., & Li, Y. R. (2008). The relationship between Ethylene induced three members of ACC synthase gene family to express in the stem and ethylene production as well as sugar accumulation in sugarcane. Crop Science, 34, 418-422.
Wang, Y. C., Li, T. L., & Hou, J. P. (2003). The impact of Ethylene processing on Tomato Pedicel shedding. Gardening Journal, 5, 554-558.
Wei, Y. W., Deng, Z. N., Hung, C. M., & Li, Y. R. (2011). Ethephon regulated differential gene expression in sugarcane. Journal of Southern Agriculture, 1, 6-10.
Ye, Y. P., Li, Y. R., Luo, T., Pang, G. Y., & Yang, L. T. (2005). Influence of ethylene pretreatment with seeds on drought resistance. Chinese Agricultural Science Bulletin, 6, 387-389.
Zheng, Z. Y., Sun, X. L., Liu, S. Q., & Gao, J. F. (2003). Preliminary study on ethylene distribution and dynamic annual variations in cucumber. Shandong Agricultural Sciences, 4, 15-17.

Publication Dates

Publication in this collection
June 2015

History

Received
20 Oct 2014
Accepted
18 Feb 2015

This is an Open Access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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[2] Abeles, F. B., Morgan, P. W., & Saltveit, M. E. (1992). Ethylene in plant biology. (p. 135-159). New York: Academic Press.

[3] Campillo, E., & Bennett, A. B. (1996). Pedicel breakstrength and cellulase gene expression during tomato flower abscission. Plant Physiology, 111, 813-820. http://dx.doi.org/10.1104/pp.111.3.813. PMid:8754682
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[5] Fong Chong, B., Mills, E., Bonnett, G. D., & Gnanasambandam, A. (2010). Early exposure to ethylene modifies shoot development and increases sucrose accumulation rate in sugarcane. Journal of Plant Growth Regulation, 29, 149-163. http://dx.doi.org/10.1007/s00344-009-9118-3.
» http://dx.doi.org/10.1007/s00344-009-9118-3

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» http://dx.doi.org/10.1016/S1360-1385(97)01132-1

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[8] Hadfield, K. A., & Bennett, A. B. (1998). Polygalacturonases: many genes in search of a function. Plant Physiology, 117, 337-343. http://dx.doi.org/10.1104/pp.117.2.337. PMid:9625687
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[9] Jackson, M. B., & Osborne, D. J. (1970). Ethylene, the natural regulator of leaf abscission. Nature, 225, 1019-1022. http://dx.doi.org/10.1038/2251019a0. PMid:16056901
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[10] Kalaitzis, P., Solomos, T., & Tucker, M. L. (1997). Three different polygalacturonases are expressed in tomato leaf and flower abscission, each with a different temporal expression pattern. Plant Physiology, 113, 1303-1308. http://dx.doi.org/10.1104/pp.113.4.1303. PMid:9112778
» http://dx.doi.org/10.1104/pp.113.4.1303

[11] Lu, D. Z., Fu, J. R., & Song, S. Q. (1997). Plant senescence and Its regulation. Beijing: China Agriculture Press, p. 65-92.

[12] McManus, M. T. (2008). Further examination of abscission zone cells as ethylene target cells in higher plants. Annals of Botany, 101, 285-292. http://dx.doi.org/10.1093/aob/mcm269. PMid:17965027
» http://dx.doi.org/10.1093/aob/mcm269

[13] Meir, S., Philosoph-Hadas, S., Sundaresan, S., Selvaraj, K. S., Burd, S., Ophir, R., Kochanek, B., Reid, M. S., Jiang, C. Z., & Lers, A. (2010). Microarray analysis of the abscission-related transcriptome in the tomato flower abscission zone in response to auxin depletion. Plant Physiology, 154, 1929-1956. http://dx.doi.org/10.1104/pp.110.160697. PMid:20947671
» http://dx.doi.org/10.1104/pp.110.160697

[14] Michael, S. R. (1985). Ethylene and abscission. HortScience, 20, 45-50.

[15] Mishra, A., Khare, S., Trivedi, P. K., & Nath, P. (2008). Effect of ethylene, 1-MCP, ABA and IAA on break strength, cellulase and polygalacturonase activities during cotton leaf abscission. South African Journal of Botany, 74, 282-287. http://dx.doi.org/10.1016/j.sajb.2007.12.001.
» http://dx.doi.org/10.1016/j.sajb.2007.12.001

[16] Mishra, S., Nailwal, T. K., & Pant, R. C. (2014). In vitro study of role of ethylene during tillering in sugarcane. Sugar Tech, 16, 255-263. http://dx.doi.org/10.1007/s12355-013-0251-8.
» http://dx.doi.org/10.1007/s12355-013-0251-8

[17] Patterson, S. E. (2001). Cutting loose. Abscission and dehiscence in Arabidopsis. Plant Physiology, 126, 494-500. http://dx.doi.org/10.1104/pp.126.2.494. PMid:11402180
» http://dx.doi.org/10.1104/pp.126.2.494

[18] Patterson, S. E., & Bleecker, A. B. (2004). Ethylene-dependent and -independent processes associated with floral organ abscission in Arabidopsis. Plant Physiology, 134, 194-203. http://dx.doi.org/10.1104/pp.103.028027. PMid:14701913
» http://dx.doi.org/10.1104/pp.103.028027

[19] Plummer, J. A., Mullins, M. G., & Vine, J. H. (1991). Seasonal changes in endogenous ABA and IAA and the influence of applied ABA and auxin in relation to shoot growth and abscission in Valencia Orange. Plant Growth Regulation, 10, 139-151. http://dx.doi.org/10.1007/BF00024960.
» http://dx.doi.org/10.1007/BF00024960

[20] Schupp, J. R., & Greene, D. W. (2004). Effect of aminoethoxyvinylglycine (AVG) on preharvest drop, fruit quality, and maturation of ‘McIntosh’ apples. I. Concentration and timing of dilute applications of AVG. HortScience, 39, 1030-1035.

[21] Shukla, L. N., Irvinder, S., & Sandhar, N. S. (1991). Design development and testing of sugarcane cleaner. Agricultural Mechanization in Asia, 22, 55-58.

[22] Singh, J., Singh, A. K., Sharma, M. P., Singh, P. R., & Srivastava, A. C (2011). Mechanization of Sugarcane cultivation in India. Sugar Tech, 13, 310-314. http://dx.doi.org/10.1007/s12355-011-0101-5.
» http://dx.doi.org/10.1007/s12355-011-0101-5

[23] Srivastava, A. C., & Kishan, S. (1990). Development of a power-driven sugarcane detrasher. Agricultural Mechanization in Asia, 21, 49-52.

[24] Tabuchi, T., Ito, S., & Arai, N. (2000). Development of the abscission zones in pedicels of galapagos wild tomatoes. CAB Direct, 69, 443-445.

[25] Taylor, J. E., & Whitelaw, C. A. (2001). Signals in abscission. The New Phytologist, 151, 323-340. http://dx.doi.org/10.1046/j.0028-646x.2001.00194.x.
» http://dx.doi.org/10.1046/j.0028-646x.2001.00194.x

[26] Uheda, E., & Nakamura, S. (2000). Abscission of Azolla branches induced by ethylene and sodium azide. Plant & Cell Physiology, 41, 1365-1372. http://dx.doi.org/10.1093/pcp/pcd071. PMid:11134422
» http://dx.doi.org/10.1093/pcp/pcd071

[27] Uthaichay, N., Ketsa, S., & van Doorn, W. G. (2007). G.1-MCP pretreatment prevents bud and flower abscission in Dendrobium orchids. Postharvest Biology and Technology, 43, 374-380. http://dx.doi.org/10.1016/j.postharvbio.2006.09.015.
» http://dx.doi.org/10.1016/j.postharvbio.2006.09.015

[28] Wang, A. Q., Fan, Y. G., Zhao, X. Y., He, L. F., Yang, L. T., & Li, Y. R. (2008). The relationship between Ethylene induced three members of ACC synthase gene family to express in the stem and ethylene production as well as sugar accumulation in sugarcane. Crop Science, 34, 418-422.

[29] Wang, Y. C., Li, T. L., & Hou, J. P. (2003). The impact of Ethylene processing on Tomato Pedicel shedding. Gardening Journal, 5, 554-558.

[30] Wei, Y. W., Deng, Z. N., Hung, C. M., & Li, Y. R. (2011). Ethephon regulated differential gene expression in sugarcane. Journal of Southern Agriculture, 1, 6-10.

[31] Ye, Y. P., Li, Y. R., Luo, T., Pang, G. Y., & Yang, L. T. (2005). Influence of ethylene pretreatment with seeds on drought resistance. Chinese Agricultural Science Bulletin, 6, 387-389.

[32] Zheng, Z. Y., Sun, X. L., Liu, S. Q., & Gao, J. F. (2003). Preliminary study on ethylene distribution and dynamic annual variations in cucumber. Shandong Agricultural Sciences, 4, 15-17.

Leaf positions	Clone	Ethylene production (nL· g^–1· h^–1× 10^–4)
Leaf positions	Clone	Early stage	Mid stage	Harvest stage
2^nd	CYZ03-194	255±3.21A	142±3.61A	107±1.53B
	CMT69-421	243±1.52B	117±2.00B	113±1.00A
	GT02-467	227±1.73C	97±1.00C	88±2.00C
	CYZ99-91	93±2.15D	60±10.00D	53±2.52D
5^th	CYZ03-194	215±2.08A	139±2.65A	89±2.65B
	CMT69-421	199±1.34B	109±1.00B	106±1.00A
	GT02-467	149±3.51C	85±1.00C	76±2.65C
	CYZ99-91	64±1.53D	50±1.73D	47±1.00D
10^th	CYZ03-194	105±1.00A	—	—
	CMT69-421	68±1.00C	—	—
	GT02-467	87±1.00B	—	—
	CYZ99-91	29±1.00D	—	—

Leaf positions	Clone	Ethylene production (nL· g^-1· h^-1× 10^-4)
Leaf positions	Clone	Early stage	Mid stage	Harvest stage
2^nd	CYZ03-194	222±1.00A	108±1.00A	102±2.08A
	CMT69-421	181±2.65B	97±1.00B	88±1.00B
	GT02-467	175±2.00B	84±1.00C	72±1.00C
	CYZ99-91	55±3.00C	50±1.73D	43±1.73D
5^th	CYZ03-194	191±1.00A	107±1.53A	91±8.50A
	CMT69-421	168±1.00B	96±2.65B	88±1.53B
	GT02-467	140±2.65C	76±1.53C	56±3.21C
	CYZ99-91	53±1.73D	46±1.00D	38±1.00C
10^th	CYZ03-194	73±1.00A	58±1.00A	43±1.00A
	CMT69-421	54±1.73B	38±1.00B	28±1.00B
	GT02-467	29±1.00C	25±1.00C	21±1.73C
	CYZ99-91	14±1.00D	13±2.00D	9.2±0.17D

Stages	Leaf sheath		Leaf scar
Stages	r	P-value	r	P-value
Early stage	0.843	0.009	0.843	0.009
Mid stage	0.862	0.006	0.871	0.003
Harvest stage	0.331	0.424	0.436	0.201

Brasil

Brasil

Relationship between endogenous ethylene production and natural defoliation traits during the maturation of sugarcane

Abstract

1 INTRODUCTION

2 MATERIAL AND METHOD

Sugarcane cultivars

Determination of ethylene production

Data analysis

3 RESULTS

Validation of ethylene GC detection methods

Natural defoliation rate

Ethylene production by leaf sheaths at the mature stage

Ethylene production by leaf scars at the mature stage

Correlation analysis between ethylene production by leaf sheaths and leaf scars and defoliation rate during maturation

4 DISCUSSION

5 CONCLUSION

ACKNOWLEDGEMENTS

REFERENCES

Publication Dates

History