The Synthesis of Ascorbic Acid in Rice Roots Plays an Important Role in the Salt Tolerance of Rice by Scavenging ROS

The root plays an important role in the responses of plants to stresses, but the detailed mechanisms of roots in stress responses are still obscure. The GDP-mannose pyrophosphate synthetase (GMPase) OsVTC1-3 is a key factor of ascorbic acid (AsA) synthesis in rice roots. The present study showed that the transcript of OsVTC1-3 was induced by salt stress in roots, but not in leaves. Inhibiting the expression of OsVTC1-3 by RNA interfering (RI) technology significantly impaired the tolerance of rice to salt stress. The roots of OsVTC1-3 RI plants rapidly produced more O2−, and later accumulated amounts of H2O2 under salt stress, indicating the impaired tolerance of OsVTC1-3 RI plants to salt stress due to the decreasing ability of scavenging reactive oxygen species (ROS). Moreover, exogenous AsA restored the salt tolerance of OsVTC1-3 RI plants, indicating that the AsA synthesis in rice roots is an important factor for the response of rice to salt stress. Further studies showed that the salt-induced AsA synthesis was limited in the roots of OsVTC1-3 RI plants. The above results showed that specifically regulating AsA synthesis to scavenge ROS in rice roots was one of important factors in enhancing the tolerance of rice to salt stress.


Introduction
Ascorbic acid (known as Vitamin C, AsA), one of the essential vitamins for human beings, also has important roles in growth and development [1,2]. As the most abundant antioxidant of plants, AsA is involved widely in scavenging reactive oxygen species (ROS) during the photosynthetic electron transfer and stress responses [2]. Therefore, the synthesis of AsA is related closely to environmental stresses [2,3].
AsA has been known for about one century [4]. Several alternative pathways, such as galacturonate and glucuronate, etc., have been suggested, and studies showed that the D-mannose/L-galactose pathway is the domain pathway of AsA synthesis in higher plants; all the genes and enzymes involved have been identified [5][6][7][8][9]. The guanosine diphosphate -mannose pyrophosphate synthetase (GMPase), which catalyzes the generation of GDP-mannose, plays a very important role in the AsA biosynthesis in plants. The AsA content of Arabidopsis GMPase point mutant vtc1-1 is only 25-30% of that in wild type plants [10]. Inhibiting the expression of GMPase genes can significantly reduce AsA (SOD), and H 2 O 2 can be further scavenged by AsA peroxidase (APX), so AsA is important for plants to scavenge ROS under stress conditions [10,14,19,20]. The studies from the analysis of salt tolerance of rice and tomato varieties showed that AsA content has a positive correlation with the salt tolerance of rice and tomato. The varieties with low AsA content were more sensitive to salt stress, while those with high AsA content were more tolerant to salt stress [21]. Plants can dynamically regulate endogenous AsA synthesis under stresses. Oxidative stresses, such as O 3 and H 2 O 2 , can induce the expression of GMPase gene VTC1 and promote AsA synthesis [10]. Under salt stress, the transcript factor AtERF98 regulates the expression of VTC1 to enhance the synthesis of AsA and improves the salt stress tolerance of Arabidopsis [14]. Therefore, the GMPase gene has an important role in the regulation of AsA synthesis in the responses to environmental conditions [10,14,22,23].
The root is not only an important organ for plants to fix the plant body and absorb water and nutrients, but is involved in the responses of plants to environmental stresses. Under normal conditions, the root absorbs water and nutrients from the soil to support the growth and development of plants and maintain cellular homeostasis. Under unfavorable conditions, the root is forced to adopt several structural and cellular physiological functional modifications to adapt to adverse environmental conditions; even under certain conditions, such as high salt, the root is the front line to respond to environmental stress [24,25]. Therefore, though the responses of roots to abiotic stresses in plants are of particular importance [26,27], the root local abiotic stress responsive mechanism is still obscure. Rice encodes three GMPase homologous genes OsVTC1-1, OsVTC1-3 and OsVTC1-8. A previous study showed that OsVTC1-1 and OsVTC1-3 were responsible for AsA synthesis in leaf and root, respectively. In contrast, OsVTC1-8 may not be involved in AsA synthesis [17], and OsVTC1-1 plays an important role in the response of rice to salt stress by regulating the redox homeostasis in the rice foliar organ [28]. The results from this study showed that rice GMPase gene OsVTC1-3 plays a major role in scavenging the rapidly accumulated ROS in rice root and enhances the tolerance of rice to salt stress by regulating AsA synthesis in rice root.

Salt Induces the Expression of OsVTC1-3 in Rice Root
GMPase plays an important role in AsA synthesis and stress responses in plants [10,19,20]. Previous studies showed that rice GMPase OsVTC1-1 and OsVTC1-3 were responsible for the foliar and root AsA synthesis, respectively [17], and the redox homeostasis in rice roots played an important role in the stress tolerance [29,30]. Is the regulated AsA biosynthesis by OsVTC1-3 in rice roots involved the response of rice to environmental stresses, and what is role of OsVTC1-3 in the response of rice to environmental stresses? To analyze the physiological function of OsVTC1-3 in the response of rice to environmental stresses, firstly, we used real-time quantitative PCR (qPCR) to analyze the expression of OsVTC1-3 in different rice tissues. The results showed that the expression of OsVTC1-3 varied greatly in different tissues. The expression level of OsVTC1-3 in rice root was very high, which was similar to that of Actin, and about more than five-times that in rice sheath and leaf. The expression level of OsVTC1-3 in rice leaf and sheath was relatively low, which was about 18% of Actin ( Figure S1). The promoter of OsVTC1-3 was cloned, and the GUS reporter gene was used to further analyze the expression level of OsVTC1-3 in different tissues of rice. The results also showed that OsVTC1-3 was mainly expressed in root, and the expression level of OsVTC1-3 in root was significantly higher than that in leaf and sheath ( Figure S1). The above data were identical to the previous results [17].
Studies showed that the expression of GMPase gene was closely related to the responses of plants to salt stress [20,21]. Salt stress is one of the main environmental stresses faced by rice and has a serious impact on rice yield [31,32]. The transcripts of OsVTC1-3 had an important role in AsA biosynthesis of rice roots [17]. To study the role of OsVTC1-3 in the response of rice to salt stress, the expression pattern of OsVTC1-3 under salt treatment was analyzed. Salt treatment was performed on rice leaves and roots by spraying 150 mM NaCl solution and soaking in 150 mM NaCl solution for different time courses, respectively. The RNA was isolated, and the expression level of OsVTC1-3 was analyzed by qPCR. The results showed that the expression level of OsVTC1-3 in rice root with the 150 mM NaCl treatment at 2 h was about 1.8-times that under the control condition, and reached the highest at 12 h ( Figure 1A). On the contrary, the expression level of OsVTC1-3 in rice leaves with the 150 mM NaCl treatment did not show an obvious difference ( Figure 1B), indicating that OsVTC1-3 may be involved in the response of rice to salt stress in rice roots, but not leaves. of OsVTC1-3 varied greatly in different tissues. The expression level of OsVTC1-3 in rice root was very high, which was similar to that of Actin, and about more than five-times that in rice sheath and leaf. The expression level of OsVTC1-3 in rice leaf and sheath was relatively low, which was about 18% of Actin ( Figure S1). The promoter of OsVTC1-3 was cloned, and the GUS reporter gene was used to further analyze the expression level of OsVTC1-3 in different tissues of rice. The results also showed that OsVTC1-3 was mainly expressed in root, and the expression level of OsVTC1-3 in root was significantly higher than that in leaf and sheath ( Figure S1). The above data were identical to the previous results [17]. Studies showed that the expression of GMPase gene was closely related to the responses of plants to salt stress [20,21]. Salt stress is one of the main environmental stresses faced by rice and has a serious impact on rice yield [31,32]. The transcripts of OsVTC1-3 had an important role in AsA biosynthesis of rice roots [17]. To study the role of OsVTC1-3 in the response of rice to salt stress, the expression pattern of OsVTC1-3 under salt treatment was analyzed. Salt treatment was performed on rice leaves and roots by spraying 150 mM NaCl solution and soaking in 150 mM NaCl solution for different time courses, respectively. The RNA was isolated, and the expression level of OsVTC1-3 was analyzed by qPCR. The results showed that the expression level of OsVTC1-3 in rice root with the 150 mM NaCl treatment at 2 h was about 1.8-times that under the control condition, and reached the highest at 12 h ( Figure 1A). On the contrary, the expression level of OsVTC1-3 in rice leaves with the 150 mM NaCl treatment did not show an obvious difference ( Figure 1B), indicating that OsVTC1-3 may be involved in the response of rice to salt stress in rice roots, but not leaves.

OsVTC1-3 Plays a Key Role in the Salt Stress Response of Rice
Previous studies showed that salt induced the expression of OsVTC1-3 in rice roots, suggesting that OsVTC1-3 may play an important role in the response of rice roots to salt stress. In order to analyze the function of OsVTC1-3 in the salt tolerance of rice, we treated the high specificity OsVTC1-3 RNAi lines, which only suppressed the expression of OsVTC1-3 [17], with 150 mM NaCl. It was found that the salt tolerance of OsVTC1-3 RNAi lines decreased significantly ( Figure 2). After 10 days of salt treatment with another seven days of recovery, the survival rates of two-week-old OsVTC1-3 RNAi seedlings were significantly lower than those of the wild type (WT). For example, the survival rate of RNAi line RNA interfering (RI)-2 was only about 40%; in contrast, the survival rate of WT was high, up to 75% ( Figure 2B), after salt treatment. The above results showed that OsVTC1-3 played a key role in the response of rice to salt stress.

OsVTC1-3 Plays a Key Role in the Salt Stress Response of Rice
Previous studies showed that salt induced the expression of OsVTC1-3 in rice roots, suggesting that OsVTC1-3 may play an important role in the response of rice roots to salt stress. In order to analyze the function of OsVTC1-3 in the salt tolerance of rice, we treated the high specificity OsVTC1-3 RNAi lines, which only suppressed the expression of OsVTC1-3 [17], with 150 mM NaCl. It was found that the salt tolerance of OsVTC1-3 RNAi lines decreased significantly ( Figure 2). After 10 days of salt treatment with another seven days of recovery, the survival rates of two-week-old OsVTC1-3 RNAi seedlings were significantly lower than those of the wild type (WT). For example, the survival rate of RNAi line RNA interfering (RI)-2 was only about 40%; in contrast, the survival rate of WT was high, up to 75% ( Figure 2B), after salt treatment. The above results showed that OsVTC1-3 played a key role in the response of rice to salt stress. Control indicates that rice seedlings were grown under normal conditions, and NaCl indicates that seedlings were treated with 150 mM NaCl. (B) The survival rate percentage of OsVTC1-3 RI lines after salt treatment in the experiment in (A). WT represents ZH17 rice variety; RI-1 and RI-2 indicate different independent RNA interference lines of OsVTC1-3 in the ZH17 background, respectively. About 50-60 seedlings were used in each experiment. The bars represent SE (±) of three independent assays, and the asterisk indicates results significantly different from that of WT (** p < 0.01 and * p < 0.05). Significance was evaluated by using the t-test. Control indicates that rice seedlings were grown under normal conditions, and NaCl indicates that seedlings were treated with 150 mM NaCl. (B) The survival rate percentage of OsVTC1-3 RI lines after salt treatment in the experiment in (A). WT represents ZH17 rice variety; RI-1 and RI-2 indicate different independent RNA interference lines of OsVTC1-3 in the ZH17 background, respectively. About 50-60 seedlings were used in each experiment. The bars represent SE (±) of three independent assays, and the asterisk indicates results significantly different from that of WT (** p < 0.01 and * p < 0.05). Significance was evaluated by using the t-test.

Inhibiting the Expression of OsVTC1-3 Decreases the Ability of Rice Roots to Scavenge ROS under Salt Stress
The accumulated ROS under stress seriously affect the growth and development of plants, so the ability to scavenge ROS is of great significance for plants to improve the tolerance to stresses [33][34][35]. OsVTC1-3 has an important role in AsA synthesis of rice roots, and AsA is closely related to scavenging of ROS. Therefore, we thought that OsVTC1-3 may be involved in the response of rice to salt stress by regulating the ability of rice roots to scavenge ROS under salt stress. To analyze how OsVTC1-3 regulates the salt stress response in rice, we analyzed the content of ROS in OsVTC1-3 RNAi plants under salt stress. Rice roots were treated with 150 mM NaCl for 1 h and then were stained with the nitroblue tetrazolium (NBT) to analyze superoxide anion (O 2 − ) content in rice roots after salt treatment.
The results showed that O 2 − accumulated rapidly in the roots of OsVTC1-3 RNAi plants after salt treatment. In contrast, the O 2 − content in WT roots was significantly lower than that in the root of OsVTC1-3 RNAi plants ( Figure 3A).

Inhibiting the Expression of OsVTC1-3 Decreases the Ability of Rice Roots to Scavenge ROS under Salt Stress
The accumulated ROS under stress seriously affect the growth and development of plants, so the ability to scavenge ROS is of great significance for plants to improve the tolerance to stresses [33][34][35]. OsVTC1-3 has an important role in AsA synthesis of rice roots, and AsA is closely related to scavenging of ROS. Therefore, we thought that OsVTC1-3 may be involved in the response of rice to salt stress by regulating the ability of rice roots to scavenge ROS under salt stress. To analyze how OsVTC1-3 regulates the salt stress response in rice, we analyzed the content of ROS in OsVTC1-3 RNAi plants under salt stress. Rice roots were treated with 150 mM NaCl for 1 h and then were stained with the nitroblue tetrazolium (NBT) to analyze superoxide anion (O2 − ) content in rice roots after salt treatment. The results showed that O2 − accumulated rapidly in the roots of OsVTC1-3 RNAi plants after salt treatment. In contrast, the O2 − content in WT roots was significantly lower than that in the root of OsVTC1-3 RNAi plants ( Figure 3A). Rice was treated with 150 mM NaCl for five days, and the contents of H2O2 were measured. The results showed that the H2O2 content was not significantly different in the roots of wild type and OsVTC1-3 RNAi plants in the control condition, but after five days of salt treatment, an amount of H2O2 accumulated in the roots of OsVTC1-3 RNAi plants. The H2O2 in the roots of OsVTC1-3 RNAi plants was significantly higher than that in the root of wild type (WT). After five days of salt treatment, the H2O2 content increased about 12-15-times in the roots of different OsVTC1-3 RNAi lines; in contrast, the H2O2 content in the roots of WT increased only six times ( Figure 3B). The above results indicated that OsVTC1-3 played an important role in controlling the ROS content in rice roots under salt stress. Bars represent SE (±) of three independent assays, and the asterisk indicates that the results were significantly different from that of WT (** p < 0.01 and * p < 0.05). Significance was evaluated by the t-test.

AsA Plays an Important Role in OsVTC1-3 Regulating Salt Response in Rice Root
The data from above results showed that OsVTC1-3 plays a key role in the salt-induced AsA synthesis in rice root under salt stress. It is well known that AsA has an important effect on scavenging the accumulating ROS under salt stress to enhance the tolerance of plants to salt stress, so we further analyzed the role of AsA in OsVTC1-3 regulating the response of rice roots to salt stress by supplying exogenous AsA. The results showed that the salt tolerance of OsVTC1-3 RNAi plants was mostly recovered after supplying 10 μM exogenous AsA (Figure 4). Similar to the above results, Bars represent SE (±) of three independent assays, and the asterisk indicates that the results were significantly different from that of WT (** p < 0.01 and * p < 0.05). Significance was evaluated by the t-test.

AsA Plays an Important Role in OsVTC1-3 Regulating Salt Response in Rice Root
The data from above results showed that OsVTC1-3 plays a key role in the salt-induced AsA synthesis in rice root under salt stress. It is well known that AsA has an important effect on scavenging the accumulating ROS under salt stress to enhance the tolerance of plants to salt stress, so we further analyzed the role of AsA in OsVTC1-3 regulating the response of rice roots to salt stress by supplying exogenous AsA. The results showed that the salt tolerance of OsVTC1-3 RNAi plants was mostly recovered after supplying 10 µM exogenous AsA (Figure 4). Similar to the above results, OsVTC1-3 RNAi lines showed a salt-sensitive phenotype after 10 days of treatment with 150 mM NaCl; however, the exogenous AsA significantly enhanced the tolerance of OsVTC1-3 RNAi lines to salt stress ( Figure 4). The survival rates of OsVTC1-3 RNAi lines RI-1 and RI-2 were about 46% and 33%, respectively. With exogenous AsA, the survival rate of OsVTC1-3 RNAi lines RI-1 and RI-2 increased up to about 68% and 66%, respectively, which was almost the same as the 72% survival rate of the wild type (WT) ( Figure 4B). This result indicated that AsA plays a key role in OsVTC1-3 regulating the response of rice roots to salt stress. OsVTC1-3 RNAi lines showed a salt-sensitive phenotype after 10 days of treatment with 150 mM NaCl; however, the exogenous AsA significantly enhanced the tolerance of OsVTC1-3 RNAi lines to salt stress (Figure 4). The survival rates of OsVTC1-3 RNAi lines RI-1 and RI-2 were about 46% and 33%, respectively. With exogenous AsA, the survival rate of OsVTC1-3 RNAi lines RI-1 and RI-2 increased up to about 68% and 66%, respectively, which was almost the same as the 72% survival rate of the wild type (WT) ( Figure 4B). This result indicated that AsA plays a key role in OsVTC1-3 regulating the response of rice roots to salt stress. NaCl indicates that rice seedlings were grown in soil by watering with 150 mM NaCl; AsA indicates that rice seedlings were grown in soil by supplied with 10 μM AsA; and NaCl + AsA represents rice seedlings grown in soil with 150 mM NaCl and 10 μM AsA. The above assays were repeated three times. About 50-60 seedlings were used in each experiment. The bars represent SE (±). The asterisk indicates results significantly different from WT (** p < 0.01 and * p < 0.05). Significance was evaluated by the t-test.

OsVTC1-3 Regulates AsA Synthesis in Rice Root under Salt Stress
Previous studies have shown that OsVTC1-3 had an important regulatory role in AsA synthesis in rice roots [17]. What is the relationship between OsVTC1-3 regulating AsA synthesis and salt stress in rice? Firstly, we analyzed the effects of salt stress on AsA synthesis in rice. Rice was treated with 150 mM NaCl for five days, and then, the AsA content in rice roots was measured. The results showed that the AsA content in the roots of OsVTC1-3 RNAi plants was less than that of WT under salt treatment. For example, the AsA content in RI-2 roots increased only about 0.11 μM/g·FW (from 0.21 μM/g·FW-0.32 μM/g·FW) after five days of salt treatment; in contrast, the AsA content in WT roots increased 0.42 μM/g·FW (from 0.47 μM/g·FW-0.89 μM/g·FW). The increasing AsA content in WT roots was about four-times that in RI-2 ( Figure 5A). Further studies found that the expression of Control indicates that rice seedlings were grown under normal conditions; NaCl indicates that rice seedlings were grown in soil by watering with 150 mM NaCl; AsA indicates that rice seedlings were grown in soil by supplied with 10 µM AsA; and NaCl + AsA represents rice seedlings grown in soil with 150 mM NaCl and 10 µM AsA. The above assays were repeated three times. About 50-60 seedlings were used in each experiment. The bars represent SE (±). The asterisk indicates results significantly different from WT (** p < 0.01 and * p < 0.05). Significance was evaluated by the t-test.

OsVTC1-3 Regulates AsA Synthesis in Rice Root under Salt Stress
Previous studies have shown that OsVTC1-3 had an important regulatory role in AsA synthesis in rice roots [17]. What is the relationship between OsVTC1-3 regulating AsA synthesis and salt stress in rice? Firstly, we analyzed the effects of salt stress on AsA synthesis in rice. Rice was treated with 150 mM NaCl for five days, and then, the AsA content in rice roots was measured. The results showed that the AsA content in the roots of OsVTC1-3 RNAi plants was less than that of WT under salt treatment. For example, the AsA content in RI-2 roots increased only about 0.11 µM/g·FW (from 0.21 µM/g·FW-0.32 µM/g·FW) after five days of salt treatment; in contrast, the AsA content in WT roots increased 0.42 µM/g·FW (from 0.47 µM/g·FW-0.89 µM/g·FW). The increasing AsA content in WT roots was about four-times that in RI-2 ( Figure 5A). Further studies found that the expression of OsVTC1-3 in the OsVTC1-3 RNAi plants was inhibited under salt stress. The expression of OsVTC1-3 in WT under salt was about 2.4-times as high as that under the normal growing conditions; in contrast, there were no significant differences in OsVTC1-3 RNAi roots between salt treatment and normal growing conditions ( Figure 5B). The above results indicated that salt-induced expression of OsVTC1-3 was necessary for AsA synthesis in rice roots under salt stress.

OsVTC1-3 in the OsVTC1-3 RNAi plants was inhibited under salt stress. The expression of OsVTC1-3
in WT under salt was about 2.4-times as high as that under the normal growing conditions; in contrast, there were no significant differences in OsVTC1-3 RNAi roots between salt treatment and normal growing conditions ( Figure 5B). The above results indicated that salt-induced expression of OsVTC1-3 was necessary for AsA synthesis in rice roots under salt stress. The AsA content of OsVTC1-3 RI plants under salt stress. Control indicates that plants were grown under normal conditions, and NaCl indicates that plants were treated with 150 mM NaCl for five days. The bars represent SE (±) of three independent assays, and the asterisk indicates results significantly different from that of the normal condition (** p < 0.01 and * p < 0.05). Significance was evaluated by the t-test.

Discussion
Root is an important organ for plants to absorb water and nutrients, as well as the responses to abiotic stresses, such as salt and drought [23]. Salt is one of the most important adverse environmental factors that seriously impairs rice production. However, few studies have focused on the mechanisms of plant roots in salt stress response [36]. This study found that the expression of GMPase gene OsVTC1-3 in rice roots under salt stress is a key for rice to accelerate AsA synthesis to scavenge the accumulated ROS and enhance the salt tolerance.
GMPase is a key enzyme of the AsA synthesis pathway in higher plants. The activity of GMPase has an important effect on the AsA synthesis of plants [3,5,6]. Plants can regulate the activity of GMPases in vivo by regulating their transcript or protein stability [14,16,17,23]. For example, salt stress and light can induce the expression of the GMPase gene to promote AsA synthesis [14,15,17]. The expression of OsVTC1-3 was predominant in rice roots. When the function of OsVTC1-3 was impaired in OsVTC1-3 RI plants, the AsA content in rice roots decreased obviously, The bars represent SE (±) of three independent assays, and the asterisk indicates results significantly different from that of the normal condition (** p < 0.01 and * p < 0.05). Significance was evaluated by the t-test.

Discussion
Root is an important organ for plants to absorb water and nutrients, as well as the responses to abiotic stresses, such as salt and drought [23]. Salt is one of the most important adverse environmental factors that seriously impairs rice production. However, few studies have focused on the mechanisms of plant roots in salt stress response [36]. This study found that the expression of GMPase gene OsVTC1-3 in rice roots under salt stress is a key for rice to accelerate AsA synthesis to scavenge the accumulated ROS and enhance the salt tolerance.
GMPase is a key enzyme of the AsA synthesis pathway in higher plants. The activity of GMPase has an important effect on the AsA synthesis of plants [3,5,6]. Plants can regulate the activity of GMPases in vivo by regulating their transcript or protein stability [14,16,17,23]. For example, salt stress and light can induce the expression of the GMPase gene to promote AsA synthesis [14,15,17]. The expression of OsVTC1-3 was predominant in rice roots. When the function of OsVTC1-3 was impaired in OsVTC1-3 RI plants, the AsA content in rice roots decreased obviously, but the AsA content in leaves did not change significantly, indicating that the transcript level of OsVTC1-3 was closely related to the AsA synthesis of rice root (Figures S1 and S2). The expression of OsVTC1-3 was induced by salt stress. The inhibition of OsVTC1-3 expression induced by salt in OsVTC1-3 RI plants significantly reduced the AsA synthesis in rice roots ( Figure 5), indicating that the transcript of OsVTC1-3 was important for rice root to improve AsA synthesis under salt stress. Different from Arabidopsis, which has only one GMPase gene, rice has three homologous genes encoding full-length GMPase, so rice can specifically regulate GMPase genes to express in different tissues and organs to maintain AsA synthesis in the response to environmental stresses.
The accumulated ROS in plants has an important influence on plant growth and development in adversity. Therefore, the ability of plant organs and tissues to scavenge ROS is closely related to the adaptability of plants to adverse environments [18][19][20]22]. Studies have shown that GMPase plays an important role in scavenging ROS in leaves of Arabidopsis and rice [10,22,37]. The mutation of the GMPase gene reduced the ROS scavenging ability of Arabidopsis, which not only significantly impaired the tolerance of Arabidopsis to O 3 and other oxidizing substances, but also decreased the tolerance of Arabidopsis to salt stress [10,22]. Inhibiting the expression of OsVTC1-3 resulted in the rapid accumulation of H 2 O 2 in rice roots under salt stress; in contrast, there was no obvious H 2 O 2 accumulation in rice leaves ( Figure 3). Different from OsVTC1-3, the previous study showed that rice GMPase gene OsVTC1-1 played an important role in scavenging ROS in rice leaves [28], indicating that rice GMPase homologous genes OsVTC1-1 and OsVTC1-3 may be involved in the salt response in rice different organs, OsVTC1-1 in leaves and OsVTC1-3 in roots by regulating ROS dynamics.
Under stress conditions, plants can regulate the expression of GMPase genes to upregulate AsA synthesis and enhance the stress tolerance of plants [14,23,35]. For example, the expression of VTC1 and other AsA synthesis genes was activated by transcription factor AtERF98 in Arabidopsis to promote AsA synthesis and enhance the salt tolerance of Arabidopsis [14]. The exogenous AsA rescued most tolerance of OsVTC1-3 RI plants to salt stress, showing that the role of OsVTC1-3 in regulating AsA synthesis was important for rice roots to scavenge ROS and enhance the tolerance of rice to salt stress ( Figure 4) Salt stress rapidly induced OsVTC1-3 expression and increased AsA biosynthesis in rice roots (Figure 1), and decreasing the expression of OsVTC1-3 significantly impaired the salt-induced AsA synthesis in rice roots ( Figure 5), indicating that OsVTC1-3 is involved in rice salt response by regulating AsA synthesis in rice roots under salt stress. In contrast, the homologous OsVTC1-1 played an important role in salt response in rice leaves due to regulating AsA biosynthesis in rice leaves [17,28]. In all, the results from the present work suggested that, different from homologous OsVTC1-1, which regulates AsA biosynthesis and the salt response of rice leaves, rice can specifically activate the transcript of OsVTC1-3 in rice roots to promote AsA synthesis to scavenge ROS in rice roots to improve the salt tolerance of rice under salt stress.

The Cultivation of Plant Materials
The wild type rice variety used in this work is (Oryza sativa L. ssp. japonica cv. Zhonghua 17) (ZH17). OsVTC1-3's RNA interfering materials (RI-1 and RI-2) were two independent transgenic lines with the knocked down expression of OsVTC1-3 by RNA interfering technology in the background of ZH17. The expression of OsVTC1-3 in RI-1 and RI-2 materials was approximately 60% and 20% of that in the wild type, respectively (the expression of OsVTC1-3 in RI-1 and RI-2 was shown by Qin et al. [17]. To germinate rice seeds, the rice seeds were soaked and cultured at 37 • C for 2 days. To analyze the expression of OsVTC1-3 with the GUS reporter gene, the germinated rice seeds were grown in the liquid of 1/2 MS (Murashige and Skoog). To grow rice in soil, the germinated seeds were planted in soil and then grown in a greenhouse at 25-30 • C with a 16-h light and 8-h dark cycle.

The Generation of Transgenic Rice
To generate OsVTC1-3 RNA interference (RNAi) plants, the specific 3 -UTR sequence of OsVTC1-3 was designed as the targeted sequence. The specific targeted sequences were cloned into the pUCCRNAi vector using the Xho I and Bgl II sites, and then, the constructed pUCCRNAi vector was digested with Sal I and BamH I. Following this, the digested DNA fragment was linked with the digested fragment of Xho I and Bgl II to get the DNA fragments that contained the forward and reverse targeted sequences, which further were cloned into the plant vector pCAMBIA2300 by the Pst I site. Then, the resultant plasmid was introduced into ZH17 by using Agrobacterium-mediated transformation. The transformed plants were selected by G418. The efficiency and specificity of the RNAi lines were confirmed by real-time quantitative PCR (Q-PCR). Transgenic rice lines with reduced expression levels of OsVTC1-3 were denoted as RI-x (here, x indicates the numbering of different independent transgenic lines). The primers for RNAi vector construction were positive primer 5 -CTCTCGAGCCTCCTTTTATGTTATGGTA-3 and reverse primer 5 -CCAGATCTAAGAACAAAGTACAAGGCTG-3 . The primers for identifying the expression level of OsVTC1-3 in RNAi lines were positive primer 5 -CGAGGGACTACATCACCGGG-3 and reverse primer 5 -CTCGTGGACGAGCACGTTG-3 .

The Analysis of OsVTC1-3 Expression by qPCR
A 0.2-g sample was used to extract total RNA by TRIzol (No. DP421, Tian Gen, Beijing, China). Then, cDNA was synthesized according to the kit (No. 18080051, Invitrogen, Carlsbad, CA, USA). The 1 µL of diluted cDNA (the Ct value of the Actin of the cDNA template was about 20) was used as the template. Then, the qPCR was carried out in accordance with the experimental manual of IQ5 (BIO-RAD, Hercules, CA, USA) to detect the relative expression level of OsVTC1-3, and the detail was described by Qin et al. [17]. Actin was used as the internal control. Each experiment was repeated 3 times, and the results showed the means and experimental errors of three independent experiments. The qPCR primers for OsVTC1-3 were positive primer 5 -CGAGGGACTACATCACCGGG-3 and reverse primer 5 -CTCGTGGACGAGCACGTTG-3 , and qPCR primers for Actin were positive primer 5 -GACCTTGCTGGGCGTGAT-3 and reverse primer 5 -GTCATAGTCCAGGGCGATGT-3 .

The Determination of the Content of AsA
Zero-point-one-seven-five grams of ascorbic acid were added into a 15-mL tube and 10 mL 6% perchloric acid (HClO 4 ) added to prepare the 100 mM AsA solution. The AsA mother liquor was diluted with 6% perchloric acid to 10 µM, 5 µM, 1 µM, 500 nM, 200 nM, 100 Nm and 50 nM AsA standard solutions. Then, each 200-µL standard sample was added into a 2-mL centrifuge tube with 1800 µL 0.2 M sodium butyrate buffer (pH = 12.7) and set on ice in the dark for 20 min. Following that, the absorption value of each sample was measured at A 265 to make the standard curve.
The measurement protocol was described by Zhang et al. [14]. About 0.2-g rice samples were ground into a fine power in liquid nitrogen, and then, the ground well samples were transferred into 5-mL centrifuge tubes containing 1 mL 6% HClO 4 , then on ice for 5 min, avoiding light. Following that, samples were centrifuged at 12,000× g rpm for 10 min. Then, 200 µL of supernatant were taken into a 5-mL centrifuge tube containing 1800 µL 0.2 M sodium succinate buffer (pH = 12.7) and 60 µL 1 M DTT. After being mixed and left at room temperature in the dark for 20 min, the OD1 was measured at A 265 by a spectrophotometer. Another 200 µL supernatant were added into tube containing 1800 µL, 0.2 M sodium succinate buffer (pH = 12.7) and 4U ascorbic acid oxidase (AAO, No. PM0131, Sigma, Tokyo, Japan). After being mixed and left at room temperature in the dark for 20 min, the OD2 was measured at A 265 . The total AsA content of each sample was calculated by the value of OD1-OD2 according to the standard curve.

The Identification of the Salt Tolerance of Rice Materials
The germinated rice seeds were planted and grown in pots for 2 weeks and then treated with 150 mM NaCl solution or 150 mM NaCl and 10 µM AsA solution. After 5-10 days of salt treatment, rice seedlings were restored under normal growing conditions for another 7 days. Then, photos were taken of different rice materials, and their survival rates were counted.

The Determination of O 2 − Content in Rice by NBT Staining
The 2-week rice seedlings were treated with 150 mM NaCl for 1 h, and then, the O 2 − content in rice roots was detected by NBT staining. The rice roots treated with water (control) and salt (NaCl) were placed in the tubes with 10 mL of staining solution (including 1 mg/mL DAB; 50 mM, pH = 3.8, NaAc-HAc), respectively. After being evacuated by vacuum for 10 min, these samples were placed in darkness at room temperature for 8 h. The roots were taken out of tubes and then rinsed with distilled water, before the samples were decolored by 10 mL 95% ethanol solution overnight. Then, the dyeing samples were observed and pictures of them taken [14].

The Determination of H 2 O 2 Content
Rice seedlings were treated with salt for 5 days and then were used to measure the H 2 O 2 content in rice root. About 0.1 g of rice root were ground into a fine power in liquid nitrogen, then the ground well samples were moved into tubes containing 1 mL of precooled acetone, on an ice bath for 3 min. Following that, H 2 O 2 was extracted from the samples, and the H 2 O 2 content was determined according to the H 2 O 2 measuring kit (No. S0051, Bi Yun Tian, Shanghai, China). The detailed process was also described by the protocol of the kit.

GUS Staining of Rice Tissue
The roots, leaves and sheaths of 10-day water-cultured rice seedlings were taken into 10-mL tubes containing 5 mL of GUS staining solution, respectively. The rice materials in GUS-dyed solution were evacuated for 15 min with a vacuum pump and then incubated at 37 • C for 24 h. Following that, the chlorophyll of rice materials was removed by ethanol, and then, the expression level of the GUS reporter gene in the rice tissue was observed. The detailed process was described in the GUS Staining Kit (No. G3060, Solarbio, Beijing, China).