Genetic Network between Leaf Senescence and Plant Immunity: Crucial Regulatory Nodes and New Insights.

Leaf senescence is an essential physiological process that is accompanied by the remobilization of nutrients from senescent leaves to young leaves or other developing organs. Although leaf senescence is a genetically programmed process, it can be induced by a wide variety of biotic and abiotic factors. Accumulating studies demonstrate that senescence-associated transcription factors (Sen-TFs) play key regulatory roles in controlling the initiation and progression of leaf senescence process. Interestingly, recent functional studies also reveal that a number of Sen-TFs function as positive or negative regulators of plant immunity. Moreover, the plant hormone salicylic acid (SA) and reactive oxygen species (ROS) have been demonstrated to be key signaling molecules in regulating leaf senescence and plant immunity, suggesting that these two processes share similar or common regulatory networks. However, the interactions between leaf senescence and plant immunity did not attract sufficient attention to plant scientists. Here, we review the regulatory roles of SA and ROS in biotic and abiotic stresses, as well as the cross-talks between SA/ROS and other hormones in leaf senescence and plant immunity, summarize the transcriptional controls of Sen-TFs on SA and ROS signal pathways, and analyze the cross-regulation between senescence and immunity through a broad literature survey. In-depth understandings of the cross-regulatory mechanisms between leaf senescence and plant immunity will facilitate the cultivation of high-yield and disease-resistant crops through a molecular breeding strategy.


Introduction
The leaf is the organ that uses the photosynthetic system to convert light into sugars, thus providing energy for plant growth and development. As leaf age increases, the photosynthesis ability gradually decreases and then enters its final stage: leaf senescence [1]. In Arabidopsis, leaf senescence occupies nearly half of the leaf life history from the onset of senescence to completely dead [2]. Although leaf senescence is basically controlled by developmental age, it can be induced by a variety of internal signals, including phytohormones and reproduction, and external factors, such as darkness, UV-B or ozone, nutrient limitation, heat or cold, drought, high salinity, and pathogen attacks [2]. Leaf senescence is critical for plants' fitness and survival because plants reallocate nutrients from senescent leaves to young leaves and other organs during age-or stress-induced senescence [3,4].
Various molecular, physiological, and biochemical events in cells are genetically regulated in an orderly manner in the entire developmental stage of leaves. Cell cycle, cell wall biogenesis,

Transcription Factors
The Arabidopsis developmental transcriptome based on RNA-seq profiling reveals that a large number of genes are upregulated during senescence [34], which are SAGs. Molecular genetic studies demonstrate that numerous SAGs function as key regulators of leaf senescence [35,36]. Intriguingly, many SAGs have also been reported to be implicated in plant immunity. Among them, NAC, WRKY, TCP, MYB, and bZIP family members are associated with leaf senescence and plant resistance, suggesting a pivotal significance of Sen-TFs in the regulation of these two processes [36,37]. As SA and ROS play important roles in the regulation of leaf senescence and plant disease resistance, and ICS1, RBOHs and CAT2 control age-and pathogen-induced SA and ROS biosynthesis and/or metabolism, respectively, they are subjected to complex regulation by Sen-TFs at the transcriptional level ( Figure 1). demonstrate that numerous SAGs function as key regulators of leaf senescence [35,36]. Intriguingly, many SAGs have also been reported to be implicated in plant immunity. Among them, NAC, WRKY, TCP, MYB, and bZIP family members are associated with leaf senescence and plant resistance, suggesting a pivotal significance of Sen-TFs in the regulation of these two processes [36,37]. As SA and ROS play important roles in the regulation of leaf senescence and plant disease resistance, and ICS1, RBOHs and CAT2 control age-and pathogen-induced SA and ROS biosynthesis and/or metabolism, respectively, they are subjected to complex regulation by Sen-TFs at the transcriptional level ( Figure 1).

Figure 1. Cross-Regulation Network between Leaf Senescence and Plant Immunity Mediated by
Salicylic Acid (SA) and Reactive Oxygen Species (ROS). SA, ROS, and programmed cell death (PCD) play a positive role in the regulation of leaf senescence and resistance against biotrophic pathogens but a negative function for plant resistance to necrotrophic pathogens. TFs that positively regulate SA, ROS and/or PCD, including WRKY75, NTL9, GBF1, and ORE1, also positively regulate leaf senescence and plant immunity. Negative regulators, such as JUB1, represses SA and ROS as well as leaf senescence and plant immunity. EIN3 and NAC019/055/072 directly bind to the promoter of ICS1 and suppress its expression, resulting in a decrease of SA production.

NAC TFs
The plant-specific NAC TF family has more than 100 members in Arabidopsis [38], and many of them are involved in the regulation of leaf senescence and plant immunity (Table 1). Some positive regulators of leaf senescence, such as ORE1 [28], NTL9 [39], NAC032 [40]], and ATAF1 [41], also play important roles in plant immunity. The mutations of these genes delay leaf senescence, while overexpressing plants display precocious senescence phenotypes. Moreover, these mutants support a higher level of hemibiotrophic pathogens, such as Pst DC3000. The overexpression of these genes confers plant resistance against Pst DC3000, but susceptibility to the necrotrophic pathogens, such as B. cinerea [42][43][44][45]. ORE1 has been shown to mediate PCD via directly targeting and activating a senescence-enhanced gene BIFUNCTIONAL NUCLEASE 1 (BFN1), which is associated with PCD [46]. Similarly, NAC087/046 control dPCD by regulating BFN1 in Arabidopsis lateral root cap [47]. Furthermore, BnaNAC87, the homolog of NAC087 in Brassica napus, acts as a positive regulator of ROS metabolism and cell death [48] and it binds the promoter of HIN1 [32,48]. However, the function of NAC087/046 in plant immunity remains unknown. The P. syringae type III effector HopD1 could target NTL9 to suppress ETI and contributes to its virulence [43], indicating that NTL9 is an important component in Arabidopsis immune system against Pst pathogens. Indeed, NTL9 directly binds the promoter of ICS1 in yeast one-hybrid assays and it is required for the induction of ICS1 by flg22 treatment [49]. ANAC032 activates SA signaling by repressing NIMIN1, a key negative regulator of SA-dependent defense, and promotes H 2 O 2 accumulation under stress [40,45]. Additionally, the overexpression of Gossypium hirsutum ATAF1 in cotton also activates SA signaling [44], although the mechanism is unclear. JUNGBRUNNEN1 (JUB1, NAC042) is an H 2 O 2 -induced NAC TF and functions as a negative regulator of longevity in Arabidopsis [6]. The overexpression of JUB1 causes the accumulation of DELLA proteins and antagonizes SA pathway, resulting in impaired resistance to Pst DC3000, but increases resistance against necrotrophic fungus A. brassicicola [55]. Additionally, higher H 2 O 2 accumulation is observed in jub1 mutants compared to Col-0 plants, whereas overexpressing JUB1 could decrease the cellular H 2 O 2 level, suggesting that JUB1 is involved in the regulation of biosynthesis and/or metabolism of H 2 O 2 [6]. Recently, NAC017, NAC082, and NAC090 have been reported to govern the positive-to-negative regulatory shift in leaf senescence, which is referred to as a "NAC troika". A single mutant of nac017, nac082, or nac090 accelerates cell death and leaf senescence, while overexpressing lines show the opposite effect, indicative of their negative regulatory roles in leaf senescence [57]. NAC090 exhibits a predominant role in repressing SA accumulation and responses by directly binding the promoters of target genes ICS1 and EDS5. Different from NAC090, ANAC017 predominantly suppresses ROS levels.
NAC019, NAC055, and NAC072 (RD26) positively regulate age-dependent leaf senescence [58]. However, their roles in plant immunity are complicated. The anac019 anac055 anac072 triple mutant shows increased resistance to P. syringae pv. maculicola (Psm) ES4326 [60]. In contrast, anac019 anac055 double mutant exhibits enhanced resistance to necrotrophic fungus B. cinerea, while the overexpression of ANAC019 or ANAC055 has the opposite effects [61]. ANAC019, ANAC055, and ANAC072 function redundantly in the suppression of SA accumulation by repressing the expression of ICS1 [49], suggesting their promotive role of leaf senescence in a SA-independent manner. Indeed, ANAC019 and ANAC055 function as transcription activators to regulate the expression of JA-related defense genes in a COI1and MYC2-dependent manner [61].
In addition to the above-mentioned transcription factors, several NAC TFs, such as NAC059 (ORS1) [62] and NTL4 [63], have only been implicated in the positive regulation of leaf senescence, which cannot rule out the possibility that they are also involved in plant immunity. Microarray-based expression profiling by using estradiol-inducible ORS1 overexpression lines reveals that several potential targets of ORS1, such as WRKY40 [74], WRKY75 [5], FMO1 [87,88], and ALD1 [89], play critical roles in plant immunity. ChIP assays show that NTL4 induces the accumulation of ROS by directly targeting the promoters of ROS biosynthesis-related genes RBOHs to control PCD during heatand drought-induced leaf senescence [63,64], which implies that NTL4 is involved in drought/heat stress-triggered disease resistance.

WRKY-TFs
WRKY TFs are one of the largest families of plant-specific TFs, with more than 70 members in Arabidopsis [90]. Although WRKY family TFs are well known for their functions in plant immunity, they are also implicated in the regulation of leaf senescence (Table 1). WRKY53, WRKY75, WRKY22, Oryza sativa WRKY6 (OsWRKY6), and Chimonanthus praecox WRKY71 (CpWRKY71) are positive regulators of leaf senescence [5,29,69,70,91] and/or disease resistance against hemibiotrophic pathogens [5,65,69]. Of them, WRKY53, WRKY75, and OsWRKY6 are involved in the regulation of SA and/or ROS signaling ( Figure 1). WRKY53 is partially involved in the SA-signaling pathway [92], and it interacts with the JA-inducible protein EPITHIOSPECIFYING SENESCENCE REGULATOR (ESR/ESP) to antagonistically regulate SA-JA signaling during leaf senescence [93]. WRKY75 promotes SA production by directly binding to the W-box (TTGACT) sequence in the promoter of ICS1 to activate its transcription. Moreover, WRKY75 suppresses the transcription of CAT2 to repress H 2 O 2 scavenging, which results in an accumulation of ROS level. OsWRKY6 directly binds and positively regulates OsICS1 to enhance SA accumulation, leading to constitutive activation of several PR genes [69].
As a negative regulator of leaf senescence, WRKY18 directly binds the W-boxes of WRKY53 promoter and suppresses its expression [72]. WRKY18 acts with its closely related homologs WRKY40 and WRKY60 to redundantly regulate disease resistance. The double mutants wrky18 wrky40 and wrky18 wrky60, as well as the triple mutant wrky18 wrky40 wrky60 display enhanced resistance to P. syringae, but are more susceptible to B. cinerea than Col-0 plants. Moreover, the double mutant wrky18 wrky40 is more resistant to the biotrophic powdery mildew fungus Golovinomyces orontii [73,74]. The triple mutant wrky18 wrky40 wrky60 exhibits a higher level of SA-responsive gene PR1, implying that they negatively regulate SA signaling.
WRKY70 and WRKY54 act redundantly to negatively regulate leaf senescence in Arabidopsis [66], functioning as negative regulators of SA biosynthesis, but positive regulators of SA-mediated gene expression [94]. WRKY70 acts as a common component in both SA-and JA-mediated signal pathways, which is activated by SA and repressed by JA [95]. The elevated expression of WRKY70 results in impaired resistance to necrotroph A. brassicicola, whereas enhances the resistance against biotroph Erysiphe cichoracearum [67], suggesting the dual roles of WRKY54 and WRKY70 in repressing SA biosynthesis and transducing the SA signal.

Other TFs
In addition to NAC and WRKY TF families, other TF family members have also been reported to regulate leaf senescence and plant immunity (Table 1). GBF1, a bZIP protein, controls leaf senescence by directly regulating PAD4 [76] and binding the promoter of CAT2 to suppress its transcription, thus resulting in the decreased H 2 O 2 -scavenging activity [75]. Accordingly, the gbf1 mutant shows a decreased H 2 O 2 level and delayed senescence phenotypes [75]. The GBF1 overexpressing plants are more resistant, whereas gbf1 is susceptible, to Pst pathogens when compared to Col-0 [76]. The circadian clock pathway is known to regulate leaf senescence and plant innate immunity [77,96]. One of the core clock components LUX (LUX ARRHYTHMO, also called PHYTOCLOCK1), an MYB family TF, is essential for circadian rhythmicity that functions as a negative regulator of leaf senescence. The leaf of lux-2 shows earlier yellowing as compared with Col-0 [77], and lux mutants display impaired disease resistance against P. syringae and SA-and JA-mediated defense signaling [78]. TCP TFs constitute a small family of plant-specific TFs that play important roles in plant development [97]. The tcp19 or tcp20 single mutant shows slightly early senescence phenotype in the dark, whereas tcp19 tcp20 double mutant displays significantly accelerated senescence, suggesting that TCP19 and TCP20 redundantly regulate leaf senescence [79]. Although the resistance phenotype of tcp19 tcp20 has yet to be studied, the TCP19 was found to bind the promoters of ICS1, PBS3 (avrPphB SUSCEPTIBLE 3), PAD4, and EDS1 (ENHANCED DISEASE SUSCEPTIBILITY 1), indicative of their possible involvement in plant immunity [49].

Non-TFs
In addition to TFs, other types of genes are also involved in the regulation of leaf senescence and disease resistance (Table 1). SAG101, a gene encoding an acyl hydrolase, plays a positive role in leaf senescence [80]. SAG101 has been demonstrated to function as an important component in plant immunity by forming a heterodimer with EDS1, thus mediating TNL-mediated PCD [23]. Arabidopsis HLS1 (HOOKLESS1) encodes a putative histone acetyltransferase and negatively regulates dark-, pathogen-, and ABA-induced leaf senescence [81]. A higher ROS level is observed in ABA-induced senescing leaves in the hls1 mutant. The loss of HLS1 function leads to an increased susceptibility to B. cinerea with larger disease lesions, enhanced necrosis, and chlorosis when compared to controls [81]. However, hls1 mutants also display enhanced disease symptoms after inoculation with Pst DC3000 (AvrRpm1), but they show a level of bacterial growth under Pst DC3000 inoculation, suggesting that HLS1 manipulates defense responses associated with ETI [81]. JMJ16 is a JmjC domain-containing protein and it is a specific H3K4 demethylase in Arabidopsis. The expression of two positive regulators of leaf senescence, WRKY53 and SAG201, is repressed by JMJ16 in an age-dependent manner through reducing H3K4me3 levels at these loci [82]. The jmj16 mutants display an early senescence phenotype, suggesting that JMJ16 is an important epigenetic regulator of leaf senescence via demethylating H3K4 at SAGs in an age-dependent manner. RNA_seq and ChIP_seq reveal that lots of potential target genes of JMJ16, such as WRKY33, CBP60G, EDS5, and PR5, are associated with plant immunity. However, the disease resistance phenotype of jmj16 is not reported so far.
Arabidopsis FtSH4, a mitochondrial AAA-protease, mediates autophagy and senescence [86], and the ftsh4 mutant shows a significantly increased SA level and accelerated leaf senescence and cell death. Although the function of FtSH4 in disease resistance has not been studied, several SA biosynthesis and signaling genes, such as SID2, NDR1, and NPR1, are upregulated in the ftsh4 mutant. Furthermore, the loss of SID2, NDR1, or NPR1 functions in the ftsh4 mutant restores the early senescence phenotypes. In addition, several WRKY genes, including WRKY40, WRKY46, WRKY51, WRKY60, WRKY63, and WRKY75, display elevated expression levels in ftsh4 mutant. Together, the above data imply that FtSH4 plays a negative role in plant immunity.

The Differences between Age-and Pathogen-Induced SA and ROS
Age-and pathogen-induced changes in SA and ROS can be regulated by a large number of Sen-TFs, as mentioned above. Although Sen-TFs are involved in these two processes, there are still significant differences between them. The spatial and temporal expression of Sen-TFs is strictly regulated, and their transcript levels are gradually upregulated during leaf senescence. Consistently, the contents of SA and ROS gradually increase as the leaf ages. By contrast, pathogen-evoked acute induction of Sen-TFs gene expression as well as the contents of SA/ROS would usually return to basal levels after a certain period of time.
The physiological state of plants, such as age, has complex and delicate regulation in gene expression. For example, the "NAC troika" precisely governs the time-dependent regulatory shift for NAC-TFs in Arabidopsis during leaf senescence. In addition to age, the functional differences of the common regulatory components of SA and ROS are likely dependent on the tissue specificity of gene expression. For instance, NTL9 functions in guard cells for flg22-triggered induction of SA synthesis-related genes and is required for stomatal immunity [49]. However, NTL9 might regulate leaf senescence by regulating the expression of a subset of SAGs in other cell types, such as mesophyll cells. Multi-omics analysis of specific cell types (single-cell sequencing) would contribute to the understanding of the functional differences of Sen-TFs on leaf senescence and plant immunity.

Cross-Talks between SA/ROS and Other Hormones during Leaf Senescence and Plant Immunity
Other phytohormones generally regulate senescence and immune responses by antagonistically or synergistically interacting with the SA/ROS signaling pathway because SA and ROS act as central players in leaf senescence and plant immunity [99]. Cross-talks between SA/ROS and other hormones are discussed here, and the key components of plant hormone pathways involved in leaf senescence and/or plant immunity are summarized in Table 2 and shown in Figure 2.

BR BRI1
A plasma membrane localized leucine-rich repeat receptor kinase involved in brassinosteroid signal transduction AT4G39400 Positive [11] Negative [127] a Resistance ability to biotrophic and hemi-biotrophic pathogens. b Resistance ability to necrotrophic pathogens. Positive [11] Negative [127] a Resistance ability to biotrophic and hemi-biotrophic pathogens. b Resistance ability to necrotrophic pathogens. ET synergistically interacts with JA in plants in response to stresses and generally antagonizes SA signaling [128]. However, the molecular details of the antagonism of JA/ET signaling on the SA pathway are still poorly understood. JA signal is perceived through JA receptor complex that constituted the F-box protein CORONATINE INSENSITIVE 1 (COI1) and JASMONATE ZIMdomain (JAZ) proteins, and activates various downstream TFs, including the IIIe bHLH TFs MYC2, MYC3, and MYC4. Pst pathogen secretes a mimic of JA-Ile virulence factor coronatine (COR) to suppress SA-dependent defenses by activating MYC2 and NAC019/055/072, which repress SA synthesis and/or promote SA metabolism [60]. Consistently, an elevated level of SA is found in the coi1 mutant [107]. JA induces stomatal closure mediated by ROS-dependent signaling pathway. JA increases the ROS level via the NAD(P)H oxidase pathway, but JA-induced ROS accumulation is not observed in coi1 or jar1-1 mutants [129]. ET is perceived by its receptors and then leads to the ET synergistically interacts with JA in plants in response to stresses and generally antagonizes SA signaling [128]. However, the molecular details of the antagonism of JA/ET signaling on the SA pathway are still poorly understood. JA signal is perceived through JA receptor complex that constituted the F-box protein CORONATINE INSENSITIVE 1 (COI1) and JASMONATE ZIM-domain (JAZ) proteins, and activates various downstream TFs, including the IIIe bHLH TFs MYC2, MYC3, and MYC4. Pst pathogen secretes a mimic of JA-Ile virulence factor coronatine (COR) to suppress SA-dependent defenses by activating MYC2 and NAC019/055/072, which repress SA synthesis and/or promote SA metabolism [60]. Consistently, an elevated level of SA is found in the coi1 mutant [107]. JA induces stomatal closure mediated by ROS-dependent signaling pathway. JA increases the ROS level via the NAD(P)H oxidase pathway, but JA-induced ROS accumulation is not observed in coi1 or jar1-1 mutants [129]. ET is perceived by its receptors and then leads to the activation of ETHYLENE-INSENSITIVE 2 (EIN2) [130] and the core TFs EIN3/EIL1 (EIN3-LIKE 1) [131]. EIN3/EIL1 thus activate a large number of downstream genes. For example, EIN3/EIL1 directly target the promoter of SID2 and negatively regulate the accumulation of SA. The ein3 eil1 double mutant thus constitutively accumulates SA, and ROS production is diminished in ethylene-insensitive mutants under Flg22 treatment [132]. In rice, OsEIL1 directly binds the promoters of OsrbohA/OsrbohB to activate their transcription [133]. ET synergistically acts with JA to activate the expression of ERF1 in response to necrotrophic pathogens [99]. JA promotes ABA signaling by inducing the expressions of ABA receptors, such as PYL4 (PYRABACTIN RESISTANCE/PYR1-LIKE/REGULATORY COMPONENT OF ABA RECEPTOR (PYR/PYL/RCAR)). Conversely, ABA promotes JA signaling by regulating the expressions of MYC TFs in response to the herbivorous insect [134,135]. As the key components of GA signaling, DELLA proteins interact with JAZ1 to activate MYC-dependent gene expressions in response to stresses [136]. Auxin enhances JA-induced expressions of defense-related genes and JA-Auxin module is involved in resistance to necrotrophic pathogens [137]. However, JA inhibits apical growth of roots and auxin has the opposite effect, suggesting they antagonistically regulate root growth. A possible model is that JA represses the expressions of auxin-responsive TFs, PLETHORAs (PLTs), which are responsible for stem cell niche maintenance [138]. JA antagonistically interacts with CKs to regulate xylem development. CKs negatively regulate xylem differentiation, while JA treatment promotes the formation of extra xylem [139].
Recent studies have greatly expanded our understandings of the cross-talks between ABA and other hormones. ABA antagonizes plant immune responses by repressing SA responses. The ICS1 transcriptional level is down-regulated in ABA receptor mutant pyl. In rice, ABA significantly suppresses the expression levels of OsWRKY45 and OsNPR1 [140]. Meanwhile, increasing evidence indicates that ABA also regulates ROS production through RBOHF. In the presence of ABA, PYLs inhibit PP2Cs, resulting in activation of one of SNF1-related protein kinases (SnRK2s), OPEN STOMATA 1 (OST1), to phosphorylate the N terminus of RBOHF, thus increasing the ROS level [141]. MYC2 is a critical and positive node in the crosstalk between JA and ABA signaling pathways. ABA interacts with JA signaling via PYL6-MYC2 to regulate cotyledon expansion [142] and the tolerance to drought [143]. Moreover, the Plant U-box (PUB) E3 ligase PUB10 directly interacts with MYC2 to destabilize it, negatively regulating both JA and ABA responses [144]. The antagonistic interactions between ABA and ET have been reported in seed dormancy and germination [145]. One of the mechanisms is that ABA inhibits the transcript level and activity of ACO1 [146]. The SnRK2-APC/C TE module is a regulatory hub that is involved in the cross-talks between GA and ABA [147]. Rice Tiller Enhancer (TE), encoding an activator of the APC/C TE E3 ubiquitin ligase complex, interacts with and degrades ABA receptor OsPYLs. SnRK2 phosphorylates TE to interrupt the interaction between TE and OsPYLs. GA reduces SnRK2s levels and inhibits APC/C TE -mediated degradation of OsPYLs. ABI4 positively regulates ARR5 (Arabidopsis RESPONSE REGULATOR 5) expression, a negative regulator of CK signaling, but it suppresses the transcript level of PIN-FORMED 1 (PIN1), indicating that ABI4 mediates the cross-talks among ABA, CK, and auxin [148]. SnRK2.3 interacts with and phosphorylates HAT1, an important transcriptional regulator in BR signaling, to repress its protein stability and binding activity, which increases expressions of ABA-responsive genes and then enhances tolerance to drought, indicating that a relationship between ABA and BR signaling pathways exists [149]. The cross-talks between ABA and other hormones in plant stress responses are discussed in details in several recently published papers [150,151].
GAs, CKs, auxins, and BRs also play important roles in plant development and immune system. GAs regulate these two processes by mediating the degradation of DELLA proteins [152]. DELLAs sequester the JA signaling repressor JAZ family proteins, leading to the activation of MYC2 and JA signaling. Meanwhile, DELLAs also directly antagonize the SA-mediated defense [120]. The accumulation of DELLAs that is induced by stresses causes the enhanced activity of ROS scavenging enzyme and suppresses ROS levels [153]. CKs are reported as modulators of plant immunity by interacting with SA. ARR2, a key TF of CK signaling pathway, interacts with TGA3 and positively enhances the expression of PR1 gene, suggesting that CKs can also function in the SA signaling pathway [154]. CKs receptor HISTIDINE KINASE3 (AHK3) and ARR2 promote PAMP-triggered stomatal closure and ROS accumulation. ARR2 directly activates the expressions of peroxidases PRX33 and PRX34, but not RBOHs, which are required for SA-and PAMP-triggered ROS production [122]. Auxins regulate plant development and plant immunity via repressing the SA signaling pathway [99]. Biotrophic pathogen evolves strategies to produce auxin or manipulate auxin signaling to suppress host SA signaling, thus contributing to its virulence [155]. Auxins limit the H 2 O 2 levels through restraining H 2 O 2 generation to be implicated in the regulation of stomatal opening. BRs are a unique class of plant steroid hormones that mediate growth and development. BRs signals are perceived and transduced by the receptor-like kinase BRASSINOSTEROID INSENSITIVE1 (BRI1) and BRI1-ASSOCIATED KINASE1 (BAK1). Pathogen Pythium graminicola manipulates plant BR pathway to antagonize SAand GA-mediated defenses to promote its infection [156]. Meanwhile, BRs activate NADPH oxidase activity, which results in an accumulation of H 2 O 2 levels in apoplast [157].
Phytohormones SA, ET, JA, ABA, and BRs play positive roles in regulating leaf senescence, whereas CK, auxins, and GA delay this process [11]. The contents of SA, JA, ET, and ABA increase during leaf senescence and promote this process [1], suggesting that these hormones could synergistically work on leaf senescence process, although many studies describe an antagonistic interaction between the SA and JA/ET/ABA pathways. The application of low concentrations of JA and SA leads to a synergistic effect on the JA-and SA-responsive genes PDF1.2 and PR1, respectively. In addition, a high concentration of JA is required for the induction of H 2 O 2 accumulation, thus JA might promote leaf senescence by partially interacting with ROS [99]. was found to mediate a novel regulatory pathway in cold acclimation independently of SA and TGA [167]. However, the exogenous application of SA improves the cold tolerance in maize, cucumber, and rice [168]. Benzothiadiazole (BTH), an SA analogue, can induce thermosensitive genes, indicating that SA is involved in heat stress [169]. Application of BTH induces bacterial resistance in a NPR1-dependent manner [169]. cpr5 (constitutive expressor of PR genes), a SA constitutive accumulation mutant, displays a high thermotolerance, while SA-deficient NahG transgenic plants exhibit an opposite phenotype. The overexpression of WRKY39 enhances thermotolerance by upregulating SA-related genes [170]. ROS accumulation is required for heat stress responses in plants. Heat stress-induced ROS are mainly produced in chloroplasts by RBOHB and RBOHD. ROS causes the accumulation of nitric oxide (NO), which subsequently activates Calmodulin 3 (CaM3), and then enhances the binding activity of HSFs (heat shock transcription factors) [171]. In biotic stresses, SA accumulation occurs after pathogen attack. Subsequently, SA binds to and activates NPR1 that interacts with TGAs to induce defense-related genes. Meanwhile, ROS is required for changes in redox status of NPR1. Besides, SA represses the transcriptional inhibition activities of NPR3/NPR4 to release defense-related genes. The production of SA/ROS is also triggered by various abiotic stresses including drought, salt cold and heat. SA/ROS further regulates NPR1-dependent or NPR1-independent gene expression. Plasma membrane-located NTL6 is relocated into the nuclear to induce a subset of PR genes in response to cold stress. Heat stress-induced ROS cause the accumulation of NO that activates CaM3 and results in DNA targeting of HSFs. TGA, TGACG motif-binding factor; PTI, PAMP-triggered immunity; ETI, Effector-triggered immunity; SAR, systemic acquired resistance; PRs, Pathogenesis- Figure 3. Roles of SA/ROS in Biotic and Abiotic Stresses. In biotic stresses, SA accumulation occurs after pathogen attack. Subsequently, SA binds to and activates NPR1 that interacts with TGAs to induce defense-related genes. Meanwhile, ROS is required for changes in redox status of NPR1. Besides, SA represses the transcriptional inhibition activities of NPR3/NPR4 to release defense-related genes. The production of SA/ROS is also triggered by various abiotic stresses including drought, salt cold and heat. SA/ROS further regulates NPR1-dependent or NPR1-independent gene expression. Plasma membrane-located NTL6 is relocated into the nuclear to induce a subset of PR genes in response to cold stress. Heat stress-induced ROS cause the accumulation of NO that activates CaM3 and results in DNA targeting of HSFs. TGA, TGACG motif-binding factor; PTI, PAMP-triggered immunity; ETI, Effector-triggered immunity; SAR, systemic acquired resistance; PRs, Pathogenesis-related genes; RBOHF, respiratory burst oxidase homolog; NTL6, NAC with transmembrane motif 1-like; NO, Nitric Oxide; CaM3, Calmodulin 3; HSFs, Heat shock transcription factors.

Roles of SA/ROS in Biotic Stresses
Biotic stresses (focused on pathogen attacks) cause changes of SA and ROS contents by multiple layers of transcriptional regulation (Figure 1). SA is perceived by its potential receptor NPR1 and NPR3/4 [20]. NPR1 or NPR3/4 interacts with a number of TGA TFs, including TGA2/5/6 to positively or negatively regulate SA-induced PR genes expression and disease resistance, respectively [20,158]. Pathogen-induced SA accumulation promotes the activity of NPR1 to further induce the expression of defense-related genes, while SA represses the transcriptional inhibition activities of NPR3/NPR4 to release defense-related genes. In plant-pathogen interactions, the production of ROS is one of the fastest physiological responses observed in plants after MAMP recognition by PRRs. ROS can induce Ca 2+ influx into the cells, activate MAPK cascades, and regulate the redox of TFs, thus activate the expression of defense-related genes [159,160]. Rapid production of ROS leads to HR or HR-like necrosis that contributes to limiting the spread of biotrophs, but it generally benefits the necrotrophs infection [9,10].

Roles of SA/ROS in Abiotic Stresses
Drought, salt, cold, and heat are the most common adverse abiotic stresses that seriously influence plant growth and development. Water deficit increases the levels of SA/ROS, and drought stress induces SA-responsive PR genes [161], suggesting that SA/ROS might play a key role in drought tolerance. The mutation of a SIZ-type small ubiquitin-related modifier (SUMO) E3 ligase causes stomatal closure and then enhances drought tolerance by elevating SA/ROS accumulation [161]. It should be noted that plants can close stomata via SA/ROS signaling after PAMP recognition, termed as stomatal immunity [49,162], implying that SA/ROS are involved in drought stress and plant immunity.
SA is also involved in salt tolerance. The germination of sid2 seeds is hypersensitive to salt stress. The endogenous H 2 O 2 is elevated in wild type and sid2 seeds under high salinity. However, the level of H 2 O 2 is reduced after treatment with SA, suggesting that SA plays an essential role in seed germination under salt stress by balancing ROS [163]. The loss-of-function of RBOHF decreases salinity-induced ROS and increases sodium concentrations in root vasculature, indicating that RBOHF functions in salinity-induced vasculature-specific ROS accumulation and salt tolerance [164].
Cold stress also increases the levels of SA/ROS [165], indicative of a close link between cold stress and immune responses. In Arabidopsis, NTL6 has been demonstrated to be an important regulator in linking cold signals with pathogenesis [166]. Cold could enhance disease resistance by activating NTL6, which upregulates several PR genes by directly binding their promoters, such as PR1, PR2, and PR5. However, NTL6-mediated PR genes expression is independent of SA [166]. Recently, NPR1 was found to mediate a novel regulatory pathway in cold acclimation independently of SA and TGA [167]. However, the exogenous application of SA improves the cold tolerance in maize, cucumber, and rice [168].
Benzothiadiazole (BTH), an SA analogue, can induce thermosensitive genes, indicating that SA is involved in heat stress [169]. Application of BTH induces bacterial resistance in a NPR1-dependent manner [169]. cpr5 (constitutive expressor of PR genes), a SA constitutive accumulation mutant, displays a high thermotolerance, while SA-deficient NahG transgenic plants exhibit an opposite phenotype.
The overexpression of WRKY39 enhances thermotolerance by upregulating SA-related genes [170]. ROS accumulation is required for heat stress responses in plants. Heat stress-induced ROS are mainly produced in chloroplasts by RBOHB and RBOHD. ROS causes the accumulation of nitric oxide (NO), which subsequently activates Calmodulin 3 (CaM3), and then enhances the binding activity of HSFs (heat shock transcription factors) [171].

Concluding Remarks
Numerous signaling components are involved in both leaf senescence and plant immunity, which suggests that these two events are not independent biological processes and share partial regulatory networks. It is apparent that SA and ROS play important and overlapping roles in leaf senescence and disease resistance. The co-players promote leaf senescence and immune response by converging on the SA and ROS pathways, which explains the phenomenon that the early-senescing mutants with increased SA and/or ROS levels are more resistant to biotrophic pathogens, but more susceptible to necrotrophic pathogens. The relationships between these two processes have not been systematically studied, despite outstanding progresses have been made over the past few decades in the individual field of leaf senescence and plant immunity. Based on our above-mentioned gene network analysis, it is reasonable to speculate that a large number of SAGs are also involved in regulating plant immunity, and vice versa. Thus, in-depth understandings of the cross-regulatory mechanisms between leaf senescence and plant immunity will facilitate the cultivation of high-yield and disease-resistant crops through molecular breeding strategy.