Salt-induced Changes of Antioxidant Enzymes Activity in Winter Canola (Brassica napus) Cultivars in Growth Chamber

Document Type : Research Paper

Authors

Tarbiat Modares University, Tehran, Iran

Abstract

The effect of salinity was assessed on the activity of some major antioxidant enzymes i.e., superoxide dismutase (SOD), peroxidase (POD), catalase (CAT), in the seedlings’ roots or shoots of three winter canola (Brassica napus L.) cultivars, Colvert (tolerant), Symbol (semi tolerant) and Agat (susceptible). Seedlings were treated with 0 (control), 50, 100 and 150 mM NaCl for 24 h in hydropoic conditions. The data were analyzed, using two-factorial balanced analysis of variance on the basis of completely randomized design with three replications. The results showed significant differences among cultivars and among salt treatments. With increasing level of salt treatment, the fresh and dry weight of roots and shoots were reduced in the cultivars under study; Colvert was influenced less than the other two canola cultivars. Salt stress enhanced the activity of SOD, POD and CAT. Almost, the maximum activity of these enzymes was detected in Colvert, the salt tolerant cultivar, followed by the other two cultivars.
 
 

Keywords

Full Text

Introduction

Salt stress is regarded as a major environmental stress and a substantial constraint to crop production (Mahajan and Tuteja 2005). About half of world's irrigated lands and nearly 20% of the world's cultivated area are affacted by salinity (Zhu 2001). Salt stress is an ever-present threat to crop yield, especially in countries where irrigation is an essential aid to agricultuer (Flower 2004). Salinity alters various biochemical and physiological responses in plant, and thus affects almost all plant processes including photosynthesis, growth and development (Iqbal et al. 2006). In plant, salt stress leads to the imbalance of production and escavenging the reactive oxgen species (ROS) as peroxidizing agents such as hydrogen peroxide (H2O2), superoxide anions (O2· ‾) and hydroxyl radical (OH·) at many sites (Mittler 2002). ROS can seriously disturb normal metabolism through oxidative damage to membrane lipids, proteins, pigments and nucleic acids (Misra and Gupta 2006). There are several known sources for ROS that include the leakage of electrons to O2 from electron transport chains in the chloroplast and mitochondria of the plant cell (Dat et al. 2000). Oxidative damage in the most plant tissues is lessened by a concerted action of both enzymatic and non-enzymatic antioxidant metabolisms (Hasegawa et al. 2000). Some investigators have shown that plants with high levels of antioxidants are more resistant to damage by ROS and better adapted to tolerate abiotic stress conditions (Prasad et al. 1999; Koca et al. 2007; Javadian et al. 2010; Zamani et al. 2011). The increase in antioxidant enzymes, such as superoxide desmutase (SOD, EC: 1.15.1.1), catalase (CAT, EC: 1.11.1.6) and peroxidase (POD, EC: 1.11.1.17), is closely related to salt tolerance of many plants (Lee et al. 2001; Tseng et al. 2007; Gao et al. 2008).

SOD is a major scavenger of O2·‾ and its enzymatic action result in the formation of H2O2 and molecular O2 (Tuna et al. 2008). The CAT and POD enzymes are scavengers of H2O2. A more efficient antioxidant system may correlate with tolerance to salt stress(Lin and Kao 2000). POD is involved in various processes, including lignification, auxin metabolism, salt tolerance and heavy metal stress in higher plants (Passardi et al. 2005). POD has often served as a parameter of metabolism activity in growth alteration and environmental stress conditions (Gao et al. 2008). Different affinities of important antioxidant enzymes including APX and CAT (µM and mM, respectively) for H2O2 suggest that they belong to the two different classes of H2O2-scavenging enzymes: CAT might be responsible for removal of the excess ROS during stress, whereas APX might be responsible for the fine modulation of ROS for signaling (Mittler 2002). Under environmental stress circumstances, increased antioxidant enzyme system lead to the decrease of ROS in plants (Abd El-baky et al. 2003). Salt stress causes increase in superoxide radical levels and an upregulation of antioxidant defense system (Vital et al. 2008). Many reports showed intimate relationship between enhanced constitutive antioxidant enzyme activities and increased resistance to environmental stresses (Vranova et al. 2002; Bor et al. 2003).

Oilseed rape is the second largest oilseed crop in the world (Raymer 2002) which is growing in many parts of Iran. Canola has high oil levels for agronomical benefits (Omidi et al. 2008). This study was aimed to assess the effect of salt stress on the activity of major antioxidant enzymes (SOD, POD, CAT) in the seedlings’ roots and shoots of three (salt tolerant, semi tolerant and susceptible) winter canola cultivars.

 

Materials and Methods

Plant growth conditions and experimental treatments

Seeds of three winter canola (Brassica napus L.) cultivars, Colvert (salt tolerant), Symbol (semi tolerant to salt) and Agat (salt susceptible), were obtained from the Seed and plant Improvement Institute (SPII), Karaj, Iran. The seeds were surface sterilized with 50% (v/v) sudium hypochlorite solution for five minutes followed by three times rinsing with distilled water. They were then germinated in petry dishes between two moisted layers of Watmann paper for 5 d and the seedlings were grown in aerated Hoaglandۥs solution in an environmentally controlled growth chamber (Department of Plant Biology, Faculty of Biological Sciences, Tarbiat Modares University, Iran) with 16 h photoperiod at 22 ± 1ºC. Salt treatments were achieved as 0 (Control), 50, 100 and 150 mM NaCl for 24 h (Ashraf et al. 2001; Sergeeva et al. 2005; Ahmadi and Ardakani 2006; Mokhamed et al. 2006). After the treating period, roots and shoots were collected separately. Aliquotes were kept at -80 ºC to be used for enzyme assay. The remained samples were used for measuring fresh and dry weights.

 

 

Enzymes assay

For the extraction of SOD enzyme, roots and shoots (0.2 g of fresh weight) were homogenized in HEPES-KOH buffer (pH 7.3), containing 0.1 mM EDTA. The homogenate was centrifuged at 13000 × g for 15 min at 4 ºC and the supernatant was used for assaying the activity of SOD enzyme. This activity was assayed by monitoring its ability to inhibit the photochemical reduction of Nitro Blue Tetrazolium (NBT; Giannopolitis and Ries 1977). One unit of SOD is defined as the amount of enzyme required to result in 50% inhibition of the rate of NBT reduction at the 560 nm absorbance and was recorded by using spectrophtometre GBC Cintra 6 (Australia). Reaction mixture (3 ml) contained HEPES-KOH buffer (pH 7.3), 0.1 mM EDTA, 50 mM Na2CO3 (pH 10.2), 12 mM L-methionine, 75 mM NBT, 1 μM riboflavine and 100 μl of crude enzyme. Roots and shoots tissues (0.2 g) were homogenized in 50 mM sodium phosphate buffer (pH 7.0), centrifuged at 13000 × g for 15 min at 4 ºC and the supernatant was used for assaying the activities of POD and CAT enzymes (Chance and Maehley 1955). The POD activity was assayed by adding tissue extract (100 μl) to the reaction mixture, containing 13 mM guaicol, 5 mM H2O2 and 50 mM sudium phoshate buffer. Changes in the absorbance at 470 nm were read every 15 s (Chance and Maehley 1955).

 

Data analysis

The data were first tested for normality and then analyzed, using two-factorial balanced analysis of variance (ANOVA) on the basis of completely randomized design with three replications, using Minitab Statistical Software (Minitab Inc., State College, PA, USA; Ryan and Joiner 2001). Cultivars and salt treatments were considered as factors with three and four levels, respectively. Means were compared by the LSD method using MSTATC Statistical Software.

 

Results and Discussion

According to their capacity for growth on high salt medium, plants are classified as glycophytes or halophytes. Most glycophytes can not tolerate salt-stress (Sairam and Tyagi 2004). Results of ANOVA showed that for both roots and shoots, the main effects were highly significant (P<0.001) for all five parameters studied (Table 1). The interactions were also significant in shoots and roots except for root's dry weight and SOD activity and shoot's catalase activity (Table 1). Based on mean comparisons, high level of salinity caused more reduction in root and shoot fresh and dry weight in all canola cultivars (Figures 1 and 2) Colvert, the salt tolerant cultivar, showed smaller decrease than Symbol and Agat. This finding was in agreement with that reported by Ashraf and Ali (2008) in canola (cvs. Cyclon, Dunkeld, CON-III and Rainbow). Salt stress caused more reduction in fresh and dry weights in Cyclon (sensitive) than those in Dunkeld (tolerant). CON-III and Rainbow had intermediate shoot and root weights under salt stress. Similar findings were reported by other workers (Ashraf et al. 2001; Qasim et al 2003; Jamil et al. 2005).

 

 

 

Table 1. Analysis of variance for physiological parameters in roots (a) and shoots

 (b) of three winter canola cultivars

SOV

df

MS

Fresh weight

Dry weight

SOD

Peroxidase

Catalase

a) Root

 

 

 

 

 

 

Salt (S)

3

7.651***

6.560***

4.519***

4.254***

4.254***

Cultivar (C)

2

4.237***

6.018***

4.239***

2.763***

2.763***

S × C

6

0.159**

0.069ns

0.501n.s

1.982***

1.982***

Error

24

0.041

0.051

0.347

0.132

0.132

 

 

 

 

 

 

 

b) Shoot

 

 

 

 

 

 

Salt (S)

3

7.527***

8.303***

8.628***

8.627***

4.974***

Cultivar (C.)

2

4.772***

3.628***

2.827***

2.821***

8.327***

S ×C

6

0.056*

0.096**

0.120*

0.120*

0.055ns

Error

24

0.021

0.026

0.046

0.046

0.060

Total

35

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

*, **, *** Significant at 0.05, 0.01 and 0.001 probability levels, respectively

ns Not significant at 0.05 probability level

 

 


b

bc

de

a

cd

ef

ef

fg

i

gh

hi

j

a)

a

c

de

b

d

fg

ef

h

i

gh

j

k

Agat

Colvert

Symbol

b)

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 


Figure 1. Fresh weight (g) of a) root and b) shoot of three winter canola cultivars

at four salt stress treatments

 

 

With the increase in salt concentration, SOD activity was enhanced in roots and shoots of all cultivars. However,  Colvert had the highest SOD activity at all conditions (Figures 3a and 3b). In the stress conditions, SOD constitutes the first line of defence against ROS (Alscher et al. 2002). Since SOD activity was high, ROS, in particular superoxide radical, scavenging was done properly and therefore, damage to membranes and oxidative stress decreased, leading to the increase of tolerance to oxidative stress (Esfandiari et al. 2007). Khosravinejad et al. (2008) reported that under saline stress, activities of protective enzymes (APX, CAT, GPX and SOD) were increased in roots and shoots of barley cultivars. In the present work, the higher POD activity in roots, was detected for Symbol and Colvert cultivars (Figure 4a) and to a lesser extent in Agat. POD activity was increased with increasing salt concentrations in all studied cultivars. Colvert, the salt tolerant cultivar, had the highest POD activity in the shoots followed by Symbol  and Agat cultivars  (Figure 4b).

 

 

 

 

Agat

Colvert

Symbol

a

bc

de

b

cd

ef

fg

gh

ij

hi

j

k

a

b

de

a

bc

fg

cd

ef

i

gh

h

j

a)

b)

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 


  

 

 

Figure 2. Dry weight (g) of a) root and b) shoot of three winter canola cultivars at four salt stress treatments

 

 

 

A significant increase in CAT activity was  detected in the roots. Except for Colvert, the highest CAT activity in other cultivars were observed at 150 mM NaCl (Figure 5a). CAT activity of roots in the Symbol was very similar to Colvert. In shoots, the highest CAT activity was recognized in Colvert, the salt tolerant cultivar (Figure 5b) followed by Symbol and Agat, the semi tolerant and sensitive canola cultivars, respectively. Uunder salt stress, antioxidant enzymes activity were increased in roots and shoots, but this increase was more in shoots than in roots. Lin and Kao (2000) reported that the activity of antioxidant enzymes (SOD, POD, CAT) increased at 200 mM NaCl salt stress in the rice leaves. In other work, Ashraf and Ali (2008) reported that salt stress (150 mM NaCl) increased the activity of antioxidant enzymes in diploid Brassica species. They noticed that SOD, POD and CAT activities of  tolerant cultivars were higher than sensitive cultivars. Our data were in agreement with those reported by the above-mentioned workers. With respect to asseyed parameters, Colvert was more tolerant to salt stress than the other two cultivars. In conclusion, our results showed that enhanced activites of antioxidant enzymes could be related to salt stress tolerance in the canola cultivars under study.

 

 

 

 

 

 

Agat

Colvert

Symbol

j

i

ef

fg

hi

bc

de

de

a

b

cd

b)

gh

b-d

f

f

c-e

ef

de

bc

b-e

de

a

ab

c-e

a)

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

Figure 3. Superoxide desmutase (SOD; DAbs 560/min/mg protein) enzyme activity in a) root and b) shoot of three winter canola cultivars at four salt stress treatments

 

 

 

 

Agat

Colvert

Symbol

gh

hi

j

e-g

ef

i

cd

de

fg

a

b

bc

fg

c-e

g

bc

c-e

d-f

bc

cd

g

a

ab

e-g

a)

b)

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

Figure 4. Peroxidase (POD; DAbs 470/min/mg protein) enzyme activity in

a)   root and b) shoot of three winter canola cultivars at four salt stress treatments

 

 

 

Agat

Colvert

Symbol

e

f

de

de

e

cd

ab

bc

cd

a

a

bc

a)

fg

gh

j

d

de

i

bc

cd

h

a

b

ef

b)

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

Figure 5. Catalase (CAT; DAbs 240/min/mg protein) enzyme activity in

a) root and b) shoot of three winter canola cultivars at four salt stress treatments

References

References

Abd El-Baky HH, Mohamed AA and Hussein MM, 2003. Influence of salinity on lipid peroxidation, antioxidant enzymes and electrophoretic patterns of protein and isoenzymes in leaves of some onion cultivars. Asian Journal of Plant Science 2: 633-638.
Ahmadi SH and Ardakani J, 2006. The effect of water salinity on growth and physiological stage of eight canola (Brassica napus) cultivars. Irrigation Science 25: 11-20.
Alscher RG, Erturk N and Heath LS, 2002. Role of superoxide dismutases in controlling oxidative stress in plant. Journal of Experimental Botany 53: 1331-1341.
Ashraf M and Ali Q, 2008. Relative membrane permeability and activities of some antioxidant enzymes as the key determinants of salt tolerance in canola (Brassica napus L.). Environmental and Experimental Botany 63: 266-273.
Ashraf M, Nazir N and McNeilly T, 2001. Comparative salt tolerance of amphidiploid and diploid Brassica species. Plant Science 160: 683-689.
Bor M, Ozdemir F and Turken I, 2003. The effect of salt stress on lipid peroxidation and antioxidants in leaves of sugarbeet (Beta vulgaris L.) and wild beet (Beta maritima L.). Plant Science 164: 77-84.
Chance B and Maehley AC, 1955. Assay of catalases and peroxidases. Methods in Enzymology 2: 764-775.
Dat J, Vandenabeele S, Van Montagu M, Inze D and Van Breusegem F, 2000. Dual action of the active oxygen species during plant stress response. Cellular and Molecular Life Sciences 57: 779-779.
Esfandiari E, Shekari F and Esfandiari M, 2007. The effect of salt stress on antioxidant enzymes activity and lipid peroxidation on the wheat seedling. Notulae Botanicae Horti Agrobotanici Cluj-Napoca35: 48-56.
Flower, TJ, 2004. Improving crop salt tolerance. Journal of Experimental Botany 55: 307-319.
Gao S, Ouyang C, Wang S, Xu Y, Tang L and Chen F, 2008. Effects of salt stress on growth, antioxidant enzyme and phenylalanine ammonia-lyase activities in Jatropha curcas L. seedlings. Plant, Soil and Environment 54: 374-381.
Giannoplitis CN and RiesSK, 1977. Superoxide dismutases: I. Occurrence in higher plants. Plant Physiology 59: 309-314.
Guan LM, Zhao J and Scadalios JG, 2000. Cis-elements and trans-factors that regulate expression of the maize Cat1 antioxidant gene in response to ABA and osmotic stress: H2O2 is the likely intermediary signaling molecule for the response. Plant Journal 22: 87-95.
Hasegawa RA, Zhu JK and Bohnert HJ, 2000. Plant cellular and molecular responses to high salinity. Annual Review of Plant Physiology and Plant Molecular Biology 51: 436-499.
Iqbal M, Ashraf M, Jamil A and Rehman S, 2006. Dose seed priming induce changes in the levels of some endogenous plant hormones in hexaploid wheat plants under salt stress? Journal of Integrative Plant Biology 48: 181-189.
Jamil M, Lee CC, Rehman, SU, Lee DB and Ashraf, M. 2005. Salinity (NaCl) tolerance of Brassica species at germination and early seedling growth. Electronic Journal of Environmental Agricultural and Food Chemistry 4: 970-979.
Javadian N, Karimzadeh G, Mahfoozi S and Ghanati F, 2010. Cold-induced changes of enzymes, proline, carbohydrates and chlorophyll in wheat. Russian Journal of Plant Physiology 57: 540-547.
Koca H, Bor M, Ozdemir F and Turkan I, 2007. The effect of salt stress on lipid peroxidation, antioxidative enzymes and proline content of sesame cultivars. Environmental and Experimental Botany 60: 344-350.
Kosravinejad F, Heydari R and Farboodnia T, 2008. Antioxidant responses of two barley varieties to saline stress. Pakistan Jourrnal of Biological Science 11: 905-909.
Lee DH, Kim YS and Lee CB, 2001. The inductive responses of the antioxidant enzymes by salt stress in the rice (Oryza sativa L.). Plant Physiology 158: 737-745.
Lin CC and Kao CH, 2000. Effect of NaCl stress on H2O2 metabolism in rice leaves. Journal of Plant Growth Regulation 30: 151-155.
Mahajan S and Tuteja N, 2005. Cold, salinity and drought stresses. An overview. Archives of Biochemistry and Biophysics 444: 139-158.
Misra N and GuptaAK, 2006. Effect of salinity and different nitrogen sources on the activity of antioxidant enzymes and indole alkaloid content in Catharanthuse roseus seedling. Journal of Plant Physiology 163: 11-18.
Mittler R, 2002. Oxidative stress, antioxidants and stress tolerance. Trends in Plant Science 7: 405-410.
Mittler R, Vanderauwera S, Gollery M and Van Breusegem F, 2004. Reactive oxygen gene network of plants. Trends in Plant Science 9: 490-498.
Mokhamed AM, Raldugina GN, Kholodova VP and Koznetov VV, 2006. Osmolyte accumulation in different rape genotypes under sodium chloride salinity. Russian Journal of Plant Physiology 53: 649-655.
Omidi H, Tahmasebi Z, Torabi H and Miransari M, 2008. Soil enzymatic activities and available P and Zn as affected by tillage practices, canola (Brassica napus L.) cultivars and planting date. Europian Journal of Soil Biology 44: 443-450.
Passardi F, Cosio C, Penel C and Dunand C, 2005. Peroxidases have more functions than a Swiss army knife. Plant Cell Reporters 24: 255-265.
Prasad KVSK, Paradha Saradhi P and Sharmila P, 1999. Concerted action of antioxidant enzymes and curtailed growth under zinc toxicity in Brassica juncea. Environmental and Experimental Botany 42: 1-10.
Qasim M, Ashraf M, Ashraf MY, Rehman SU and Rha ES, 2003. Salt-induced changes in two canola cultivars differing in salt tolerance. Biologia Plantarum 46: 629-632.
Raymer P, 2002. Canola: an emerging oilseed crop. Pp. 122-126. In: Janick J and Whipkey A (Eds). Trends in New Crops and New Uses, ASHS Press, Alexandria, VA.
Ryan B and Joiner BL, 2001. Minitab Handbook. 4th edn. Duxbury Press, California, USA.
Sairam PK and Tyagi A, 2004. Physiology and molecular biology of salinity stress tolerance in plants. Current Science 86: 407-421.
Sergeeva E, Shah S and Glick B, 2005. Growth of transgenic canola (Brassica napus cv. Westar) expressing a bactrial 1-aminocyclopropan-1-carboxylate (ACC) deaminase gene on high concentrations of salt. World Journal of Microbiology and Biotechnology 22: 277-282.
Tseng MJ, Liu CW and Yiu JC, 2007. Enhanced tolerance to sulfur dioxide and salt stress of transgenic Chinese cabbage plants expressing both superoxide dismutase and catalase chloroplasts. Plant Physiology and Biochemistry 45: 822-833.
Tuna AL, Kaya C, Dikilitas M and Higga D, 2008. The combined effects of gibberellic acid and salinity on some antioxidant enzyme activites, plant growth parameters and nutritional status in maize plants. Journal of Experimental Botany 62: 1-9.
Vital SA, Fowler RW, Virgen A, Gossett DR, Banks SW and Rodriguez J, 2008. Opposing roles for superoxide and nitric oxide in the NaCl stress-induced upregulation of antioxidant enzyme activity in cotton callus tissue. Environmental and Experimental Botany 62: 60-68.
Vranova E, Inze D and Brensegem FV, 2002. Signal transduction during oxidative stress. Environmental and Experimental Botany 53: 1227-1236.
Zamani S, NezamiMT, Bybordi A, Behdad M and KhorshidiMB, 2011. Effect of different NaCl salinity on antioxidant enzyme activity and relative water in winter canola (Brassic napus). Journal of Research in Agricultural Science 7(1): 49-57.
Zhu JK, 2001. Overexpression of a delta-pyrroline-5-carboxylate synthetase gene and analysis of tolerance to water and salt stress in transgnic rice. Trends in Plant Science 6: 66-72.

Files

Share

How to cite

Statistics