Nitric Oxide Is Involved in the Regulation of the Ascorbate–Glutathione Cycle Induced by the Appropriate Ammonium: Nitrate to Mitigate Low Light Stress in Brassica pekinensis

Low light intensity is common in northern China due to fog or haze, and causes stress for crop plants. To solve the problem of low light intensity stress on the growth and development of vegetable crops in China, new cropping strategies must be developed. We previously showed that an appropriate ratio of ammonium and nitrate (NH4+:NO3−) can alleviate the effect of low light stress on plants, although it is not clear what mechanism is involved in this alleviation. We propose the hypothesis that an appropriate ammonium/nitrate ratio (10:90) can induce NO synthesis to regulate the AsA-GSH cycle in mini Chinese cabbage seedlings under low light intensity. To test the hypothesis, we conducted a series of hydroponic experiments. The results indicated that, under low light intensity conditions, appropriate NH4+:NO3− (N, NH4+:NO3− = 10:90) decreased the contents of malondialdehyde (MDA), hydrogen peroxide (H2O2), and superoxide anion (O2−) in leaves compared with nitrate treatment. Exogenous nitric oxide (SNP) had the same effects on MDA, H2O2, and O2−. However, with the addition of a NO scavenger (hemoglobin, Hb) and NO inhibitors (N-nitro-l-arginine methyl ester, L-NAME), NaN3 (NR inhibitor) significantly increased the contents of MDA, H2O2, and O2-. The application of N solution enhanced the AsA-GSH cycle by increasing the activities of ascorbate peroxidase (APX), glutathione reductase (GR), monodehydroascorbate reductase (MDHAR), dehydroascorbate reductase (DHAR), and ascorbate oxidase (AAO), compared with control (NH4+:NO3− = 0:100). Meanwhile, exogenous SNP significantly increased the above indicators. All these effects of N on AsA-GSH cycle were inhibited by the addition of Hb, L-NAME and NaN3 in N solution. The results also revealed that the N and SNP treatments upregulated the relative expression level of GR, MDHAR1, APXT, DHAR2, and AAO gene in mini Chinese cabbage leaves under low light stress. These results demonstrated that the appropriate NH4+:NO3− (10:90) induced NO synthesis which regulates the AsA-GSH cycle in mini Chinese cabbage seedlings under low light stress.


Introduction
Low light intensity is common in northern China due to fog or haze, and causes a stress to crop plants [1]. In addition, it has been reported that a significant reduction in solar radiation reaching the earth has occurred during the last 50 years [2]. Low light environment usually reduces plant size, plant height, and stem thickness, and may also affect energy distribution in specific parts of the plant as well as the reproductive capacity of plants [3]. It has been reported that net photosynthesis in plants usually decreases under low light intensity [4,5]. Ding et al. [6] reported that under low light stress, soluble protein content, and catalase activity decreased; however, the content of malondialdehyde (MDA) and activities of superoxide dismutase (SOD) and peroxidase (POD) increased in sweet corn, suggesting an activation of the reactive oxygen species (ROS) controlling pathways. Environmental stress can lead to overproduction of reactive oxygen species (ROS), which can cause oxidative damage to plants [7]. It is well known that most plants can resist oxidative damage through the ascorbate-glutathione (AsA-GSH) cycle in chloroplasts by increasing the activity of ascorbate peroxidase (APX, EC 1.11.1.11), monodehydroascorbate reductase (MDHAR, EC 1.6.5.4), dehydroascorbate reductase (DHAR, EC 1.5.5.1), and glutathione reductase (GR, EC 1.6.4.2) [8]. AsA-GSH cycle system can play an important role in maintaining protein stability, structural integrity of the biofilm system, and defense against membrane lipid peroxidation, such as nitric oxide (NO) induced by exogenous jasmonic acid (JA) upregulated the activity of the AsA-GSH cycle and had important role in drought tolerance [9]; the protective ability of exogenous triacontanol (TRIA) to modulate the redox status through the antioxidant pathway AsA-GSH cycle, so reducing Cd-induced oxidative stress [10]. Therefore, the AsA-GSH cycle is important for the protection against oxidative damage induced by stresses.
Nitric oxide, a ubiquitous signal molecule, plays important roles in different plant tissues and participates in a variety of physiological processes. NO may also participate in the process of plant resistance to stress by regulating the production of endogenous hormones and increasing antioxidant enzyme activities in plants [11][12][13][14]. It has been reported that NO can participate in the activity of ABA-induced antioxidant enzymes, and can relieve the oxidative damage caused by high-intensity light stress in leaves of tall fescue [15]. Shan et al [16] demonstrated that NO regulated the AsA-GSH cycle in Agropyron cristatum under water stress. Previously, we studied the effect of ammonium nitrogen and nitrate nitrogen on seedlings of Chinese cabbage under low light stress. The results showed that supplying appropriate concentration of ammonium nitrogen could alleviate low light stress in the seedlings [17]. However, it is not clear what mechanism is involved in this alleviation. It is generally accepted that nitrite or L-arginine (L-Arg) is the main substrate for NO synthesis, both via enzymatic and non-enzymatic routes in plants [18]. The enzymatic pathway involves nitrate reductase (NR)/nitrite-NO reductase (Ni-NOR) or nonidentified nitric oxide synthase (NOS)-like enzyme [19]. The non-enzymatic pathway relies on nitrite reduction at acidic pH or through the action of the mitochondrial electron transport chain under anaerobic conditions [20]. Moreover, in hydroponic condition, the addition of ammonium in solution will affect the pH value of solution and nitrate metabolic pathway. Based on the NO synthesis in plants, we propose the hypothesis that NO participated in the regulation of the ascorbate-glutathione cycle induced by the appropriate ammonium: nitrate to mitigate low light stress.
Mini Chinese cabbage (Brassica pekinensis), a subspecies of Brassica rapa belonging to the Cruciferae, is a mini-type Chinese cabbage. Because of its compact size, light texture, good taste, and high nutrient content, it is very popular among the people of China. In northwestern China, mini Chinese cabbage is widely cultivated during winter in solar-greenhouses where low light intensity (between 85 and 150 µmol m −2 s −1 in day) is a major abiotic stress factor limiting plant growth and crop productivity [21]. How to solve the problem of low light intensity stress on the growth and development of mini Chinese cabbage in China has become a priority for research. To address this, we propose the hypothesis that appropriate ammonium/nitrate ratio (10:90) can induce NO synthesis to regulate the AsA-GSH cycle in mini Chinese cabbage seedlings under low light intensity. The objectives of the experiment were (1) the effect of exogenous NO on the response of mini Chinese cabbage seedlings to low light stress; (2) to find out whether appropriate ammonium:nitrate ratio (10:90) can induce NO synthesis to regulate the AsA-GSH cycle in mini Chinese cabbage seedlings under low light intensity. seedling are considered as important indices of evaluating the degree of membrane lipid damage to low light stress. As shown in Figure 1, under low light condition, the MDA contents in NH 4 + :NO 3 − (10:90) and SNP treated leaf significantly decreased by 42.3% and 67.63% compared to the solo nitrate treated leaf, respectively. Whereas the addition of NO inhibitors (NaN 3 , L-NAME) and scavenger (Hb) in N treatment solution significantly increased the MDA contents compared with N treatment ( Figure 1A).

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ammonium:nitrate ratio (10:90) can induce NO synthesis to regulate the AsA-GSH cycle in mini Chinese cabbage seedlings under low light intensity.

Effects of NO and NH4 + :NO3 − Ratio on Membrane Lipidation Damage in Leaf under Low Light Stress
Hydrogen peroxide (H2O2) and superoxide anion (O2 − ), malondialdehyde (MDA) contents in seedling are considered as important indices of evaluating the degree of membrane lipid damage to low light stress. As shown in Figure 1, under low light condition, the MDA contents in NH4 + :NO3 − (10:90) and SNP treated leaf significantly decreased by 42.3% and 67.63% compared to the solo nitrate treated leaf, respectively. Whereas the addition of NO inhibitors (NaN3, L-NAME) and scavenger (Hb) in N treatment solution significantly increased the MDA contents compared with N treatment ( Figure 1A). Effects of NO and NH4 + :NO3 − ratio on membrane lipidation damage in mini Chinese cabbage leaves under low light stress. The seedlings cultivated in black containers filled with different solutions, CK (NH4 + :NO3 − = 0:100); N (NH4 + :NO3 − = 10:90); SNP (100 μmol/L); N + Hb (0.1%); N + L-NAME (25 μmol/L); N + NaN3 (50 μmol/L) were treated for 7 days. Capital letters A to C represent MDA content, H2O2 content, O2 − content, respectively. Bars indicated the SE (n = 3). Significant differences (p < 0.05) between treatments are indicated by different letters, for low light condition.  GSH and AsA are two important antioxidants, which are two key components in the AsA-GSH cycle to maintain the cellular redox status. As shown in Figure 2A Compared with the N treatment, the addition of L-NAME, NaN 3 , and Hb in N solution decreased AsA contents, which reversed the effects of N on AsA content (Figure 2A). Similarly, the treatments of N and SNP were significantly increased the GSH contents by 66.1% and 93.3% compared with the control, respectively. The addition of NO inhibitors (NaN 3 , L-NAME) and scavenger (Hb) in N solution obviously decreased the GSH contents, as compared to the N treatment ( Figure 2B). The data revealed that NO induced by appropriate NH 4 + :NO 3 − ratio (10:90) plays an important role in increasing the AsA and GSH contents of mini Chinese cabbage seedlings under low light stress.
Under low light stress, compared with the solo nitrate treatment, the appropriate NH4 + :NO3 -ratio and exogenous NO treatments decreased H2O2 content by 42.5% and 57.34%, respectively and significantly reduced O2 -content by 42.3% and 52.54%, respectively. However, the treatment of N + NaN3, N + L-NAME, and N + Hb markedly increased the contents of H2O2 and O2 − (Figures 1B and 1C). The results suggested that the NO induced by appropriate NH4 + :NO3 − ratio participates in the regulation of the membrane lipid oxidation damage in mini Chinese cabbage seedlings under low light stress.

Effects of NO and NH4 + :NO3 − Ratio on the Contents of Redox State of Ascorbate and Glutathione in Leaf under Low Light Stress
GSH and AsA are two important antioxidants ， which are two key components in the AsA-GSH cycle to maintain the cellular redox status. As shown in Figure 2A, the AsA contents in N (NH4 + :NO3 − = 10:90) treated leaves was 96.3% higher than that in control (NH4 + :NO3 − = 0:100) treated leaves. The exogenous NO (SNP) treatment was markedly increased AsA contents, being about 4-fold of the control. Compared with the N treatment, the addition of L-NAME, NaN3, and Hb in N solution decreased AsA contents, which reversed the effects of N on AsA content (Figure 2A). Similarly, the treatments of N and SNP were significantly increased the GSH contents by 66.1% and 93.3% compared with the control, respectively. The addition of NO inhibitors (NaN3, L-NAME) and scavenger (Hb) in N solution obviously decreased the GSH contents, as compared to the N treatment ( Figure 2B). The data revealed that NO induced by appropriate NH4 + :NO3 − ratio (10:90) plays an important role in increasing the AsA and GSH contents of mini Chinese cabbage seedlings under low light stress.

Effects of NO and NH 4 + :NO 3 − Ratio on the Activities of Key Enzymes Involved in the AsA-GSH Cycle in Leaf under Low Light Stress
The interconversions between oxidized and reduced ascorbic and glutathione in leaves were also investigated. As shown in Figure 3, the appropriate NH 4 + :NO 3 − and exogenous NO enhanced the activities of AAO, APX, DHAR, GR, and MDHAR in leaves compared with the solo nitrate treatment. AAO is a key enzyme involved in the metabolism of substances in plants. It is a copper-containing enzyme that oxidizes ascorbic acid-producing water and dehydroascorbic acid (DHA). Compared with the control (NH 4 + :NO 3 − = 0:100), the treatments of N and SNP were significantly increased the activities of AAO enzymes in leaves by 106% and 84.67%, respectively ( Figure 3A). However, the activity of AAO was significantly decreased when the L-NAME, NaN 3 , and Hb were added in N treatment solutions separately.

Effects of NO and NH4 + :NO3 − Ratio on the Gene Expression Level Related to Antioxidative Enzymes in the AsA-GSH Cycle under Low Light Stress
To further verify whether NO induced by the appropriate NH4 + :NO3 − ratio participates in the regulation of AsA-GSH cycle under low light stress, we used the RT-PCR technique to verify the relative expression levels of genes coded with the related enzymes which are involved in the AsA-GSH cycle. The relative expression level of GR gene in SNP-treated seedlings were significantly higher than that in solo nitrate-treated leaves, which increased by 38.72% ( Figure 4A). Compared with the control, exogenous SNP treatment and N treatment slightly upregulated the relative gene APX is an important enzyme that scavenges excess of H 2 O 2 by catalyzing it into water and divalent oxygen. As shown in Figure 3B, compared with control, the N and exogenous NO (SNP) treatment also markedly increased the activities of the APX enzymes with the values of 83.3% and 104%, respectively. However, the application of L-NAME, NaN 3 , and Hb in N treatment solution markedly decreased the activities of APX enzyme under low light stress, as compared to the treatment of N ( Figure 3B).
In the process of plant resistance to stress, the enzymes of DHAR and GR are two key enzymes that remove ROS and maintain the stability contents of AsA and GSH in plants. As shown in Figure 3C,D, compared to the control, the activity of DHAR enzyme was obviously increased by 152.6% after the application of SNP, but when plants exposed to the treatments of N + NaN 3 , N+ L-NAME and N + Hb, the activity of DHAR decreased by 46.31%, 49.47%, and 47.36%, respectively ( Figure 3C). The application of SNP slight increased the GR activity by 28.51%, as compared to the treatment of N, while the treatments of N + NaN 3 , N+ L-NAME, and N + Hb significant decreased the activity of GR enzymes when compared with the N treatment, and there is no significant difference between these treatments ( Figure 3D).
Compared with the control, the activity of MDHAR enzyme in leaves treated with N and exogenous NO was increased by 102% and 70.7%, respectively ( Figure 3E). However, the application of L-NAME, NaN 3 , and Hb in N solution markedly decreased the MDHAR activity ( Figure 3E). These results suggested that NO induced by appropriate NH 4 + :NO 3 − ratio participated in the regulation of the key enzymes involved in AsA-GSH cycle under low light stress.

Effects of NO and NH 4 + :NO 3 − Ratio on the Gene Expression Level Related to Antioxidative Enzymes in the AsA-GSH Cycle under Low Light Stress
To further verify whether NO induced by the appropriate NH 4 + :NO 3 − ratio participates in the regulation of AsA-GSH cycle under low light stress, we used the RT-PCR technique to verify the relative expression levels of genes coded with the related enzymes which are involved in the AsA-GSH cycle. The relative expression level of GR gene in SNP-treated seedlings were significantly higher than that in solo nitrate-treated leaves, which increased by 38.72% ( Figure 4A). Compared with the control, exogenous SNP treatment and N treatment slightly upregulated the relative gene expression level of MDHAR1, but the relative expression level of MDHAR1 gene in N + NaN 3 , N + L-NAME, and N + Hb treated seedlings significantly downregulated when compared with N treatment ( Figure 4B). From Figure 4C,D, we could see that the application of N and SNP were significantly upregulated the relative expression levels of APXT and DHAR2 genes when compared with the control, which increased by 72.3% and 57.6%; and 57.7% and 56.9%, respectively. However, the application of L-NAME, NaN 3 , and Hb in N solution markedly downregulated the relative expression levels of the APXT and DHAR2 genes ( Figure 4C,D). The AAO gene expression level in N-and SNP-treated seedling were higher than that in solo nitrate-treated leaf, and increased by 20.6% and 8.4%, respectively ( Figure 4E). The results from the transcriptional level verified that NO induced by appropriate NH 4 + :NO 3 − ratio upregulated some vital genes coded with related enzymes involved in the AsA-GSH cycle. NO induced by appropriate NH4 + :NO3 − ratio upregulated some vital genes coded with related enzymes involved in the AsA-GSH cycle.

Effects of NO and NH4 + :NO3 − Ratio on the NO Level in Root Tissues under Low Light Stress
The NO-dependent fluorescence intensity in root tips were detected to further prove that appropriate NH4 + :NO3 − ratio induced NO synthesis and then participated in regulating AsA-GSH cycle under low light intensity. The levels of NO in root tips were determined according to the intensity of fluorescence. As shown in Figure 5, the levels of NO in root tips under N treatment were 38% higher than that under CK treatment. This suggests that appropriate NH4 + :NO3 − ratio promoted the production of NO in root tips. Moreover, when Hb, NaN3, and L-NAME were applied in N solution, the levels of NO in root tips significantly decreased by 56.8%, 53.8%, and 32%, respectively, compared with N treatment. These data suggested that appropriate NH4 + :NO3 − ratio increased biosynthesis of NO in tissues in mini Chinese cabbage under low light intensity.

Effects of NO and NH 4 + :NO 3 − Ratio on the NO Level in Root Tissues under Low Light Stress
The NO-dependent fluorescence intensity in root tips were detected to further prove that appropriate NH 4 + :NO 3 − ratio induced NO synthesis and then participated in regulating AsA-GSH cycle under low light intensity. The levels of NO in root tips were determined according to the intensity of fluorescence. As shown in Figure 5, the levels of NO in root tips under N treatment were 38% higher than that under CK treatment. This suggests that appropriate NH 4 + :NO 3 − ratio promoted the production of NO in root tips. Moreover, when Hb, NaN 3 , and L-NAME were applied in N solution, the levels of NO in root tips significantly decreased by 56.8%, 53.8%, and 32%, respectively, compared with N treatment. These data suggested that appropriate NH 4 + :NO 3 − ratio increased biosynthesis of NO in tissues in mini Chinese cabbage under low light intensity.

Discussions
Low light is one of the main factors that limit the productivity of many cultivated crops. However, accumulation of ROS such as O2 − and H2O2 occurred under low light condition was associated with signs of oxidative damage to lipids [7]. Malonaldehyde, which is a by-product of lipid peroxidation, is usually considered as an indicator of oxidative stress [22]. In previous studies, under 0 ℃ low temperature stress, the O2 − generation rate and H2O2 content increased rapidly in ginkgo leaf. Meanwhile, MDA content and membrane permeability increased remarkably, and the growth and development of the plant are hindered [23]. Membrane lipid oxidative damage occurred in Vicia faba seedlings under Cd stress, NO could reduce the contents of MDA, hydrogen peroxide, and reactive oxygen species (ROS) [24]. The appropriate ratio of ammonium and nitrate is more favorable for plant growth and development than the single application of ammonium nitrogen or nitrate nitrogen [25]. Our previous study showed that the application of appropriate NH4 + :NO3 − (10:90; total nitrogen concentration 5 mmol/L) ratio could alleviate low light stress in mini Chinese cabbage seedlings [17]. In our present study, the accumulation of MDA, H2O2, and O2 − in appropriate N-and SNP-treated plants was lower than those in solo nitrate-treated plants, which alleviated the membrane lipid damage in plant and the alleviation effect of NO is more obvious than that of N under low light stress (Figure 1). That is to say, the same alleviation effects of N (appropriate NH4 + :NO3 − ratio) on low light intensity was observed once again in the present study. Moreover, we found that exogenous NO could also decrease the contents of MDA, H2O2, and O2 − in mini Chinese cabbage under low light intensity, suggesting the exogenous NO had the similar effect with N on mitigating low light intensity stress. However, the alleviation effect of N on membrane lipid peroxidation was reversed by the addition of NO scavenger (Hb) and NO synthesis inhibitors (L-NAME and NaN3) in the N treatment solution (Figure 1). The NO level in root tissue under N treatment was significantly higher than that under nitrate only treatment ( Figure 5). All these data suggested that the alleviation role of N on membrane lipid damage was due to the induction of endogenous NO synthesis.
The ascorbate-glutathione (AsA-GSH) cycle is recognized to be a key player in H2O2 metabolism in higher plants and components of the cycle mainly located in plant cell, cytosol, mitochondria, and peroxisomes as well as the chloroplast [26]. AsA and GSH are the two important redox compounds of the antioxidant system and they can defense against stress-induced ROS to keep cellular redox homeostasis in plants [27][28][29]. Among the AsA-GSH cycle, there are four key

Discussions
Low light is one of the main factors that limit the productivity of many cultivated crops. However, accumulation of ROS such as O 2 − and H 2 O 2 occurred under low light condition was associated with signs of oxidative damage to lipids [7]. Malonaldehyde, which is a by-product of lipid peroxidation, is usually considered as an indicator of oxidative stress [22]. In previous studies, under 0°C low temperature stress, the O 2 − generation rate and H 2 O 2 content increased rapidly in ginkgo leaf.
Meanwhile, MDA content and membrane permeability increased remarkably, and the growth and development of the plant are hindered [23]. Membrane lipid oxidative damage occurred in Vicia faba seedlings under Cd stress, NO could reduce the contents of MDA, hydrogen peroxide, and reactive oxygen species (ROS) [24]. The appropriate ratio of ammonium and nitrate is more favorable for plant growth and development than the single application of ammonium nitrogen or nitrate nitrogen [25].
Our previous study showed that the application of appropriate NH 4 + :NO 3 − (10:90; total nitrogen concentration 5 mmol/L) ratio could alleviate low light stress in mini Chinese cabbage seedlings [17]. In our present study, the accumulation of MDA, H 2 O 2 , and O 2 − in appropriate N-and SNP-treated plants was lower than those in solo nitrate-treated plants, which alleviated the membrane lipid damage in plant and the alleviation effect of NO is more obvious than that of N under low light stress (Figure 1). That is to say, the same alleviation effects of N (appropriate NH 4 + :NO 3 − ratio) on low light intensity was observed once again in the present study. Moreover, we found that exogenous NO could also decrease the contents of MDA, H 2 O 2 , and O 2 − in mini Chinese cabbage under low light intensity, suggesting the exogenous NO had the similar effect with N on mitigating low light intensity stress. However, the alleviation effect of N on membrane lipid peroxidation was reversed by the addition of NO scavenger (Hb) and NO synthesis inhibitors (L-NAME and NaN 3 ) in the N treatment solution (Figure 1). The NO level in root tissue under N treatment was significantly higher than that under nitrate only treatment ( Figure 5). All these data suggested that the alleviation role of N on membrane lipid damage was due to the induction of endogenous NO synthesis. The ascorbate-glutathione (AsA-GSH) cycle is recognized to be a key player in H 2 O 2 metabolism in higher plants and components of the cycle mainly located in plant cell, cytosol, mitochondria, and peroxisomes as well as the chloroplast [26]. AsA and GSH are the two important redox compounds of the antioxidant system and they can defense against stress-induced ROS to keep cellular redox homeostasis in plants [27][28][29]. Among the AsA-GSH cycle, there are four key enzymes (APX, GR, MDHAR, and DHAR) involved in interdependence and independence of AsA and GSH in H 2 O 2 metabolism [26,30]. The AAO located in apoplast plays vital role in regulating the redox state of extracellular AsA pool, similar function with APX located in intracellular. Wu et al. reported that the value of oxidation/reduction ratio of AsA pool is regulated by AAO when cucumber seedlings were suffered from salt stress, and they deemed that it was the first defense of cells against stress damages [31]. As we known, the excess accumulation of H 2 O 2 under abiotic stress will damage the membrane system and cell organelles of plants. Although AsA-GSH cycle is known as the antioxidant defense system in plant cell, its activity can also be regulated by environmental stresses [32][33][34]. In general, when plants were subjected to various stresses, the contents of GSH and AsA were changed and the activities of APX, GR, MDHAR, and DHAR were triggered [32,35]. Kanwar et al. [35] reported that arsenic toxicity treatments significantly enhanced the modulations of various stress markers like proteins, antioxidative enzymes (SOD, CAT, POD, APX, GR, MDHAR, and DHAR) and MDA content. Maintaining the efficient recycling of AsA via MDHAR and DHAR is crucial to maintaining AsA in a high redox state so that it can efficiently scavenge H 2 O 2 via the catalytic reaction of APX and AAO [36]. In our present study, the exogenous NO and appropriate NH 4 + :NO 3 − ratio increased the contents of AsA and GSH ( Figure 2). Whereas the contents of AsA and GSH decreased significantly when the seedlings were treated with NO scavengers (Hb) and inhibitors (L-NAME, NaN 3 ) in N solutions ( Figure 2). Moreover, the NO level was significantly higher in appropriate NH 4 + :NO 3 − ratio treated root than that in solo nitrate-treated root ( Figure 5), indicating that NO induced by appropriate NH 4 + :NO 3 − ratio participated in the antioxidant defense system under low light stress. Meanwhile, N and NO enhanced the activities of the key enzymes involved in GSH-ASA cycle under low light stress to maintain a favorable redox status (Figure 3). Similarly, it was noted that exogenous NO treatment effectively increased GSH content, effectively prevented wheat seedlings from being damaged under salt stress, and improved their resistance [37]. Based on our results, the activities of key enzymes involved in the AsA-GSH cycle and the contents of AsA and GSH under NO and N treatments were higher than those under the control treatment (Figures 2  and 3). The scavengers and synthesis inhibitors of NO inhibited the production of endogenous NO in plants. The application of Hb, L-NAME, and NaN 3 in N treatment solutions markedly decreased the activities of GR, AAO, MDHAR, DHAR, and APX enzymes under low light stress ( Figure 3). It was suggested that NO involved in the regulation of the AsA-GSH cycle in mini Chinese cabbage seedling under low light stress. The results are similar to that reported by Shan et al. [9], who indicated that NO participated in the regulation of the AsA-GSH cycle in wheat seedlings under drought stress with the application of exogenous jasmonic acid. Similar results have also been reported in other stressed plants [38,39]. Begara-Morales et al. [40] demonstrated that ROS and NO interacted during plant responses to biotic/abiotic stresses and it was NO-related posttranslational modifications (PTMs), such as S-nitrosylation and/or tyrosine nitration, that regulated proteins linked to ROS metabolism. Moreover, they deemed that the enzymes involved in the AsA-GSH cycle were identified as NO targets using proteomic analytical techniques. The expression levels of GR, MDHAR1, and APXT genes were upregulated by N and SNP treatments, whereas they were downregulated by the N + Hb, N + L-NAME, and N + NaN 3 treatments ( Figure 4A-C). Similar phenomena were observed in the relative expression levels of DHAR 2 and AAO genes ( Figure 4D,E). The upregulation of the DHAR 2 and AAO genes in NO-treated leaf was significant when compared with those in control-treated leaf and N + Hb, N + L-NAME, and N + NaN 3 treated leaves (Figure 4). Previous research demonstrated that nitric oxide triggers multiple redox regulatory (defense-related) genes expression in stressed plants [41]. Sun et al. [39] reported that NO protects wheat root against Al-induced oxidative stress, possibly through the regulation of the AsA-GSH cycle, and NO application enhanced the related gene transcriptional level of AsA-GSH cycle in wheat genotypes, which is consistent with our results. The NO and N treatments upregulated the relative expression levels of GR, MDHAR1, APXT, DHAR2, and AAO genes and the application of L-NAME, NaN 3 , and Hb in N treatment solution markedly downregulated these gene expression levels. Moreover, the NO level in appropriate NH 4 + :NO 3 − ratio treated root was significantly higher than that in solo nitrate-treated root ( Figure 5), which suggesting that appropriate NH 4 + :NO 3 − (10:90) mitigated low light intensity in mini Chinese cabbage seedling via inducing endogenous NO synthesis to regulate the AsA-GSH cycle.
In summary, we found that endogenous NO induced by appropriate NH

Plant Material and Growth Conditions
Mini Chinese cabbage (Brassica pekinensis cv. "Jinwa no. 2") seeds were purchased from Gansu Agricultural Institute (Lanzhou, China). The seeds were surface-sterilized in 5% sodium hypochlorite for 10 min, then washed with water. The seeds were soaked in water for 6 h then placed in petri dishes with double-layer filter paper moistened with distilled water, and finally kept in the dark to germinate at 25 • C for 16 h. After germination, uniformly geminated seeds were sown in pots filled with clean quartz sand and cultured with half-strength whole Hoagland's nutrient solution for 10 days, with a photoperiod of 12 h, temperature of 23 ± 2/13 ± 2 • C (day/night), and light fluence about 200 µmol m −2 ·s −1 , in a modern climate controlled greenhouse.

Treatments and Experimental Design
At the two-leaf stage, uniform seedlings were transferred into distilled water for 1 d, after that, groups of four uniform seedlings were transplanted into a black circular container (diameter 12 cm, height 4.5 cm) filled with 250 mL the following treatment liquid for cultivation: CK (NH 4 + :NO 3 − = 0:100, total nitrogen concentration 5 mmol/L); N (NH 4 + :NO 3 − = 10:90,total nitrogen concentration 5 mmol/L); SNP (NO donor, sodium nitroprusside, 100 µmol/L); N + Hb (NO scavenger, hemoglobin, 0.1%); N + L-NAME (NOS inhibitor, N-nitro-l-arginine methyl ester, 25 µmol/L); N + NaN 3 (NR inhibitor, sodium azide, 50 µmol/L). Each treatment had six replications. 7 µmol/L nitrification inhibitor dicyandiamide (C 2 H 4 N 4 ) was added to each pot of treatment solution, which inhibited the conversion of nitrate nitrogen to ammonium nitrogen. The pH of the treatment solution was adjusted to 6.5-7.0 with 0.1 mol·L −1 hydrochloric acid or sodium hydroxide. The seedlings cultivated in black containers filled with different solutions were placed in a light incubator, the light intensity was 100 µmol·m −2 ·s −1 (moderately low light stress), the photoperiod was 12 h/12 h, and the temperature was 25 ± 1 • C/18 ± 1 • C (day/night), and the humidity is 60%. In order to avoid root hypoxia and lack of nutrient solution, replace the treatment solution once every 2 days. After 7 days of treatment, measurement of various indicators began. Sample of leaf tissue (0.5 g) was homogenized in 0.1% (w/v) cold trichloroacetic acid (TCA). After centrifugation at 12,000 g for 20 min, the extracted supernatant was used for determination of H 2 O 2 , O 2 − , and MDA content following the method of Alexieva et al. [42] with a few modifications. The reaction mixture contained 0.5 mL extracted supernatant, 0.5 mL 100 mM phosphate buffer (pH 6.8) and 2 mL reagent (1 M KI w/v in fresh double-distilled water). 0.1% TCA solution without material extract was used as the blank. The mixture was incubated for 1 h in the dark and the absorbance was measured at 390 nm. The content of hydrogen peroxide was calculated according to a standard curve.
To determine the content of MDA, the reaction mixture contained 0.5 mL extracted supernatant and 1 mL 0.5% (w/v) thiobarbituric acid (TBA) in 20% TCA. The mixture was incubated at 100 • C for 30 min, and the samples were centrifuged at 10,000× g for 10 min, and the absorbance of supernatants was measured at 532 nm. The value for non-specific absorption at 600 nm was subtracted.
The O 2 − level was analyzed according to the method of Nakajima et al. [43] with some modifications, the reaction mixture contained 2 mL extracted supernatant, 1.5 mL phosphate buffer, and 0.5 mL hydroperamine hydrochloride. The mixture was incubated for 20 min in 25 • C water bath. The 2 mL the above reaction solution was mixed with 2 mL 17 mM aminobenzene sulfonic acid for 30 • C constant temperature reaction for 30 min, and the absorbance of supernatants was measured at 530 nm.

Determination of Glutathione (GSH) and Ascorbate (AsA)
GSH and AsA contents of mini Chinese cabbage leaves were measured using the GSH and AsA determination Kit (Beijing Solarbio Science & Technology Co., Beijing, China) following the manufacturer's instructions.

Transcript Level Estimation with RT-PCR
Total RNA was isolated from 100 mg (fresh weight) of excised mini Chinese cabbage seedling leaves by grinding with mortar and pestle in liquid nitrogen to obtain a fin paste using TaKaRa reagent (TaKaRa Bio, Japan) according to the manufacturer's instructions. Each treatment was replicated three times. Primers designed for the genes and reference genes are detailed in Table 1. Each reaction (20 µL total volume) consisted of 10 µL SYBR Premix Ex Taq II, 2 µL of diluted cDNA and 0.8 µL of forward and reserve primers. PCR amplification conditions were as follows: 1 min at 95 • C followed by 40 cycles of 5s at 95 • C and 20 s at 60 • C with data collection at the annealing step. After the 40 cycles, the dissociation/melting curve stage with 0 s at 95 • C, 15 s at 65 • C, 0 s at 95 • C and 30 s at 50 • C was included. The relative quantification of mRNA levels is based on the method of Livak and Schmittgen [44]. The expression level relative to the control for each sample was expressed as 2 −∆∆Ct . The NO-dependent fluorescence in root tissues was detected with the fluorescence indicator 4, 5-diaminofluorescein diacetate (DAF-2 DA; Sigma, Ronkonkoma, NY, USA) which can permeate into the cell membrane and emit fluorescence upon binding to NO. The root samples were incubated for 2 h under dark condition with 20 µM DAF-2DA in 50 µM Tris-HCl buffer (pH 7.5), and washed three times in fresh buffer. These were then visualized under a fluorescence microscope (Leica 400×, Planapo, Wetzlar, Germany) with excitation and emission wavelengths of 485 and 538 nm, respectively. The fluorescence intensity of fluorescent image was determined by ZEN2 software (Carl Zeiss). The fluorescence intensity, called 'relative fluorescence unit', was expressed in color level on a scale ranging from 0 to 255.

Statistical Analysis
The analysis of variance was performed using SPSS Statistics 17.0 software. The significance of means difference between treatments was tested by Duncan's multiple tests (p < 0.05).