Autophagy Dances with Phytohormones upon Multiple Stresses

Autophagy is an evolutionarily conserved process for turning over unwanted cellular components, thus promoting nutrient recycling and maintaining cellular homeostasis, which eventually enables plants to survive unfavorable growth conditions. In addition to plant growth and development, previous studies have demonstrated that autophagy is involved in the responses to various environmental challenges through interplaying with multiple phytohormones, including abscisic acid (ABA), jasmonic acid (JA), and salicylic acid (SA). In this review, we summarize the advances made in their synergistic interactions in response to multiple abiotic and biotic stresses; we also discuss the remaining issues and perspectives regarding their crosstalk.


Introduction
In recent years, crop yield and productivity have been adversely challenged by the occurrence of extreme climate and environmental changes, such as drought, heat, or pathogen attack [1]. Accordingly, researchers and breeders have to develop new cultivars in order to adapt to these unfavorable conditions. Therefore, elucidating the relevant mechanisms underlying responses to environmental stresses is of particularly importance for crop genetic improvement.
Unlike animals that can migrate to avoid stressful environments, plants have to evolve a wide variety of mechanisms in order to adapt their morphology, physiology, and metabolism to survive different biotic (including pathogen invasion and herbivores) and abiotic stresses (including nutrient deficiency, cold, heat, drought, salt stress, etc.) [2]. One of most important strategies for plants to overcome stresses is the "self-eating" regulation, which is also designated as autophagy. Autophagy is a highly conserved degradation mechanism in eukaryotes, in which the unwanted or dysfunctional cytoplasmic materials, such as proteins, protein complexes, nucleic acid aggregates, and even entire organelles, are targeted to the vacuole/lysosome for degradation [3]. Such a regulatory mechanism functions as a standby emergency supply system, providing nutrients for plants exposed to multiple environmental stresses, and then ensuring the minimum requirement for their growth and development, eventually promoting survival.
Until now, there are three distinct types of autophagy described in plants: microautophagy, macroautophagy, and mega-autophagy [4] (Figure 1). In terms of macroautophagy, cargo is trapped in upon sucrose starvation and darkness treatment [16]. Taken together, these studies suggested that autophagy is modulated by a potential complicated regulation of plant hormone and stress signaling.
famine pathogen Phytophthora infestans physically interacted with the host ATG8CL to antagonize the binding of Joka2 and ATG8CL, which activated autophagy in host for arresting the pathogen infection [76]. Considering that SA and JA are remarkably involved in biotic stress, especially the HR and PCD regulation, it could be speculated that autophagy-mediated biotic response may be likely associated with these phytohormones.
In summary, autophagy is comprehensively involved in multiple stress responses ( Figure 1). However, there are still interesting open questions regarding these regulations, such as how the ATG genes are activated by various stress signals and whether there is the specific role of each ATG gene in response to different stresses. Figure 1. Regulation of stress response by AuTophaGy-related (ATG)-mediated autophagy. Multiple ATG genes operate autophagy. AtATG5 positively regulates the nitrogen remobilization and tolerance to carbon starvation while AtATG4 and AtATG7 are known to modulate tolerance to carbon starvation. In addition, AtATG5 is also involved in regulating the homeostasis of micronutrients, such as Fe/Mn/Zn. Unfold proteins were accumulated under heat stress, which has been implicated to be degraded via the ATG5-and ATG7-mediated autophagy route in Arabidopsis and tomato, eventually alleviating the unfold protein-mediated endoplasmic reticulum (ER) stress. Similarly, accumulation of H2O2 and oxidized proteins are also selectively turned over by the AtATG2-and AtATG5dependent autophagy in Arabidopsis and the OsATG10-dependent autophagy in rice, respectively, ultimately relieving oxidative stress. MdATG3, MdATG10, and MdATG18 positively enhance drought tolerance in apple, and a similar role is also found in AtATG18a. Furthermore, AtATG2, AtATG5, Figure 1. Regulation of stress response by AuTophaGy-related (ATG)-mediated autophagy. Multiple ATG genes operate autophagy. AtATG5 positively regulates the nitrogen remobilization and tolerance to carbon starvation while AtATG4 and AtATG7 are known to modulate tolerance to carbon starvation. In addition, AtATG5 is also involved in regulating the homeostasis of micronutrients, such as Fe/Mn/Zn. Unfold proteins were accumulated under heat stress, which has been implicated to be degraded via the ATG5and ATG7-mediated autophagy route in Arabidopsis and tomato, eventually alleviating the unfold protein-mediated endoplasmic reticulum (ER) stress. Similarly, accumulation of H 2 O 2 and oxidized proteins are also selectively turned over by the AtATG2and AtATG5-dependent autophagy in Arabidopsis and the OsATG10-dependent autophagy in rice, respectively, ultimately relieving oxidative stress. MdATG3, MdATG10, and MdATG18 positively enhance drought tolerance in apple, and a similar role is also found in AtATG18a. Furthermore, AtATG2, AtATG5, AtATG7, and AtATG10 also play positive roles in regulating submergence response, finally mediating osmotic stress. Under abiotic stress, AtATG7 positively regulates necrotrophic fungal pathogen resistance, and pexRD54 arrests pathogen infection by boosting autophagy activity. Moreover, autophagy positively regulates hypersensitive response (HR) cell death to resist biotic stress. Solid lines represent the activation or repression with known evidence. Dashed lines represent the proposed activation or repression.

Regulation of Autophagy
In the past two decades, about 40 ATG components involved in autophagy machinery have been identified in yeast, and these ATG proteins exhibit a canonical route for autophagy [3], which enables the characterization of plant autophagy by genetic analysis of the homologous ATGs in plants (such as Arabidopsis, rice, tobacco, maize, etc.) [18][19][20][21][22]. To date, the autophagy machinery has been well-characterized among the plant kingdom, including autophagy induction; membrane delivery; vesicle nucleation; phagophore expansion and closure; and autophagosome formation and delivery, fusion, and digestion [3,23]. Accumulating evidence has elaborated the conserved role of autophagy in the growth and development among plant species, especially in Arabidopsis and rice regarding the senescence and pollen fertility [24,25]. For example, recent studies have indicated that over-expression of ATG genes enhance the yield and nitrogen use efficiency (NUE) in both rice and Arabidopsis [26], Plants 2020, 9, 1038 4 of 16 whereas the seed yield and nitrogen harvest index decreased in autophagy-deficient mutants due to the reduction of nitrogen remobilization for grain filling [27,28], indicating that autophagy has great potential to be of benefit in improving crop yield and productivity under either normal or suboptimal conditions. The target of rapamycin (TOR) complex is one of the most important negative regulators of autophagy, which is composed of TOR itself and two binding partners, the regulatory-associated protein of TOR (RAPTOR) and the lethal with Sec thirteen 8 (LST8) [29]. TOR functions upstream of autophagy in regulating plant growth and stress response [3,30,31]. Autophagy could be induced and promoted by inactivation of TOR via RNA interference (RNAi); TOR kinase inhibitors such as rapamycin and AZD8055 [32]; or disruption of its constituents, the RAPTOR and LST8 [33][34][35]. Notably, repression of autophagy by upregulation of TOR was specifically detected under the nutrient starvation, salt, and osmotic stresses, whereas such repression could not be identified under oxidative and ER stresses [33,36], suggesting that the TOR-mediated autophagy was only involved in the response to certain types of stresses. Previously, it has already shown that auxin functioned upstream of TOR [37]. Further analysis demonstrated that auxin also modulated autophagy in the TOR-dependent stresses response, as the exogenous application of the auxin analogue 1-naphthylacetic acid (NAA) could activate TOR to inhibit autophagy activity under salt and osmotic stresses rather than oxidative and ER stresses [36,38]. Taking into account the fact that auxin is regulated by the plant-specific family of Rho GTPases2 (ROP2) [37,39], it is supposed that ROP2 might also influence autophagy activity through the auxin-TOR pathway. Additionally, the ABA metabolism is also regulated by TOR kinase. The ABA hormone level is strongly decreased in lst8-1 or raptor1b mutants, as well as in wild-type (WT) plants treated with AZD8055 [40]. These studies suggest that ABA and auxin participate in a TOR-dependent route of autophagy regulation.
The energy sensor SNF-related kinase 1 (SnRK1) is a highly conserved eukaryotic kinase protein, which responds to the nutrient and energy deficiency in plants [41]. It has been reported that sugar phosphates affect TOR activity through the modulation of SnRK1, which was shown to act upstream of TOR in Arabidopsis [42][43][44]. In particular, autophagy was inhibited by trehalose 6-phosphate (T6P), an inhibitor of SnRK1, in response to abiotic stresses [42], suggesting SnRK1 functions as an activator of autophagy. Moreover, it was also found that SNF1-RELATED PROTEIN KINASE1.1 (KIN10), a catalytic subunit of SnRK1, activates autophagy through affecting the phosphorylation of ATG1 in Arabidopsis, indicating that SnRK1 could also regulate autophagy in a TOR-independent manner [45]. This implies that SnRK1-triggered autophagy may be associated with TOR-independent stress responses, such as the responses to oxidative and ER stresses [42]. A recent study demonstrated that the number of autophagosomes was decreased in response to misfolded protein accumulation-induced ER stress in the inositol-requiring enzyme 1b (ire1b) mutants as compared with WT plants [46], indicating that activation of autophagy upon ER stress relies on the functional IRE1b in Arabidopsis. Unfortunately, the relationship between SnRK1 and IRE1b in regulating TOR-independent autophagy remains unclear. Collectively, either TOR or SnRK1 functions upstream of autophagy, and then integrates autophagy and hormone signaling to regulate multiple stress responses.

Oxidative Stress
Oxidative stress is produced by free radicals, which is considered an important factor leading to aging and diseases. ROS accumulation generally causes oxidative stress, and subsequently damages most cell components, including proteins, lipids, and DNA. It has been implicated that the oxidized proteins were degraded by autophagy during oxidative stress in Arabidopsis. For example, dramatic accumulation of H 2 O 2 could be detected in Arabidopsis atg5 and atg2 mutants [47][48][49][50]. Knockdown expression of AtATG18a in seedlings increased the sensitivity to oxidative stress as compared to WT, and other autophagy-defective plants also presented a chlorotic phenotype [50]. Furthermore, the rice osatg10b mutants were more sensitive to high salt and methyl viologen (MV, as an inducer of autophagy), and accumulated more oxidized proteins upon MV treatment compared with wild-type plants [14], suggesting that these oxidized proteins were selectively degraded by autophagy. Further analysis of these kinds of proteins, such as whether they could interact with ATG8 and then be transported into the vacuole for degradation, or whether over-expressing ATG genes could alleviate the oxidative stress, would extend our knowledge about the role of autophagy in plant responses to oxidative stress. Taken together, these studies suggest that autophagy protects plant cells from oxidative stress by degrading oxidized proteins.

Nutrition Starvation
An increasing number of studies have demonstrated that autophagy is involved in the recycling and remobilization of nutrients at the whole-plant level [51,52]. With respect to the nitrogen recycling, the ATG genes played an important role for plant survival under nitrogen-limiting conditions, since nitrogen remobilization was found to be markedly decreased in atatg5 mutants at the vegetative stage [53,54]. Similar observations were also obtained in terms of the carbon remobilization. For instance, the atatg4, atatg5, and atatg7 mutants displayed delayed growth under carbon starvation as compared with WT at the seedling stage [55]. Additionally, a recent study has shown that phosphate limitation could also stimulate autophagy in the root tips of Arabidopsis, and the phosphate deficiency response-2 (PDR2) and the low phosphate response-1 (LPR1) were required for the activation of autophagy under Pi starvation conditions [56]. Notably, the expression level of ATG genes was significantly different under carbon starvation and sucrose starvation in Arabidopsis. For instance, the AtATG8B was dramatically up-regulated upon sucrose starvation rather than other ATG genes, whereas AtATG8A, AtATG8B, and AtATG8H were significantly induced under carbon starvation rather than AtATG8D, AtATG8E, and AtATG8I [16], suggesting a distinct role of ATG genes in regulating these stresses. Furthermore, it is quite interesting that the transport of Fe, Mn, and Zn also required autophagy in addition to nitrogen and carbon, since an obvious decreasing of these micronutrients was identified in the seed of atatg5 mutant. Further investigation of the double mutant of atatg5 and salicylic acid induction deficient 2 (sid2) that attenuates senescence in Arabidopsis revealed that there was a two-step mechanism underlying autophagy activity, in which the nutrients firstly were translocated into vegetative organs (such as leaf) and then remobilized to seeds [52]. Nutrition deficiency could result in early senescence of leaf, which can also be caused by darkness treatment. Taking into account that both nutrition deficiency and darkness could induce autophagy, it raises an issue as to whether these two stresses stimulate autophagy through similar or distinct mechanisms. In addition, it also needs to be explored whether autophagy would modulate nutrient transport at the EPCS, where the autophagosomes form, through affecting ion transporters. Taken together, these findings provide an insight into the fact that autophagy is essential for nutrient translocation and remobilization in plants under adverse situations.

Osmotic Stress
Salinity, drought, and osmotic stress caused by both these factors are the most common environmental stresses affecting plant growth and development. Knockdown of AtATG18a resulted in more sensitivity to salt and drought stresses as compared to WT plants [15], demonstrating that ATG-mediated autophagy participates in plant responses to these osmotic stresses. In accordance with the phenotype observed upon oxidative stress, the oxidized proteins in the atatg2 and atatg7 mutants were accumulated compared to WT plants under salt stress [57]. In addition, overexpression of MdATG3 or MdATG10 in apple enhances their drought tolerance [58,59]. The similar phenotype also displayed in the MdATG18a-overexpressing tomato [60]. Furthermore, a recent study identified a plant-specific gene, Constitutively Stressed 1 (COST1), which negatively regulates drought resistance by influencing the autophagy pathway in Arabidopsis [61]. It is worth mentioning that waterlogging and submergence, as the opposite effect of drought also induces autophagosome formation in Arabidopsis. For example, the Arabidopsis atatg2, atatg5, atatg7, and atatg10 mutants showed more sensitivity to submergence compared to WT plants [62], suggesting an extensive involvement of autophagy in maintaining cellular homeostasis. Notably, the morphological responses of Arabidopsis and rice to waterlogging are quite different. For Arabidopsis, the entire plant is subjected to waterlogging, while for rice the internode elongation would be triggered to escape from waterlogging. Therefore, it is interesting to characterize and compare the conserved and divergent mechanisms of autophagy in regulating waterlogging between these two species. Overall, these results illustrate that autophagy broadly regulates different types of osmotic stresses.

Heat and ER Stresses
High temperature is one of the major threats to plant growth and development. Heat stress causes protein misfolding and denaturation, which could also lead to ER stress [46]. Both atatg5 and atatg7 displayed hypersensitivity to heat stress compared to WT plants, and accumulation of insoluble protein aggregates tagged by ubiquitin was found in the atatg7 mutant [36]. Silencing of ATG5 or ATG7 in tomato presents consistent response upon heat stress [63]. A recent report validated the fact that autophagy induced by heat stress actually resulted from ER stress, since the excessive unfolded proteins caused by heat were accumulated in the ER. The result was further confirmed by the sodium 4-phenylbutyrate (PBA) treatment assay, in which this chemical eliminates unfolded proteins in ER and thus reduces the heat-induced autophagy [46]. Considering the fact that autophagy turns over impaired proteins, it is strongly possible that accumulated unfolded protein would be degraded through autophagy. As expected, treatment of Arabidopsis seedlings with ER stress inducers, such as tunicamycin (TM) and dithiothreitol (DTT), precisely induced autophagosome formation [64]. Taken together, it is supposed that autophagy is responsible for the clearance of unfolded proteins existing in the ER upon heat or even other stresses.

Regulation of Autophagy under Biotic Stress
Biotic stress also influences autophagic events in addition to abiotic stress. Enhanced disease susceptibility 1 (EDS1) is a key component responsible for salicylic acid (SA)-mediated defense against diseases and pathogens [65]. Previously, it was verified that autophagy deficiency could repress the EDS1-mediated hypersensitive response (HR) cell death, a type of PCD in plants [66], suggesting a parallel role of autophagy with other PCD pathways in HR regulation. Interestingly, autophagy has been known to coordinate with SA to regulate leaf senescence [49], implying a possibility that the EDS1 or other SA regulators might be the direct targets of autophagy in response to biotic stress. Recently, other studies have further demonstrated the important role of autophagy in plant defense against pathogens, as well as the connection between autophagy and HR during plant innate immunity [42,[66][67][68][69]. For example, disruption of AtATG7 resulted in elevated susceptibility to the necrotrophic fungal pathogen, and the selective autophagy limited the cauliflower mosaic virus (CMV) infection by NBR1-mediated targeting of viral capsid protein and particles [70,71], suggesting a positive role of autophagy in biotic stress. A recent study proved that NBR1 modulates ABA signaling in Arabidopsis [72], suggesting that autophagy-mediated CMV resistance might be also correlated with ABA signaling. Surprisingly, autophagy also restricts HR, which may be due to the different age of the plants used in the experiments, and thus a hypothesis was proposed that the role of autophagy is likely varied according to the specific pathogen [42,[73][74][75]. Notably, pathogens could in turn interfere with the autophagy response from host plant. For instance, the PexRD54 from potato famine pathogen Phytophthora infestans physically interacted with the host ATG8CL to antagonize the binding of Joka2 and ATG8CL, which activated autophagy in host for arresting the pathogen infection [76]. Considering that SA and JA are remarkably involved in biotic stress, especially the HR and PCD regulation, it could be speculated that autophagy-mediated biotic response may be likely associated with these phytohormones.
In summary, autophagy is comprehensively involved in multiple stress responses (Figure 1). However, there are still interesting open questions regarding these regulations, such as how the ATG genes are activated by various stress signals and whether there is the specific role of each ATG gene in response to different stresses.

The Regulation of Autophagy by Hormones
Autophagy could be regulated by hormones at the transcriptional level while hormones could be also modulated by autophagy in response to various stresses ( Figure 2). Transcriptome analyses in petunia and Arabidopsis clearly indicated that autophagic genes could be transcriptionally regulated by hormones [77][78][79], implying phytohormones may modulate autophagy through the signaling transduction.
ET is well known to play a dominant role in senescence and stress responses in plants. It has also been shown that ET is involved in autophagy-mediated stress response. For example, knockdown of mitochondrial alternative oxidase (AOX) decreased the level of autophagy in ET-mediated drought tolerance in tomato [79]. Inhibition of autophagy by 3-methyladenine (3-MA) resulted in decreasing disease resistance, which could be rescued by exogenous ET in banana [80]. Furthermore, autophagy genes GmATG8i and GmATG4, and ethylene biosynthesis and signaling factors GmACS and GmERF were induced in soybean under sugar or nitrogen starvation [81]. In addition, the ET signaling transcription factor, ethylene response factor 5 (ERF5), directly binds to the promoters of SlATG8d and SlATG18h and then promotes the activity of autophagy, ultimately leading to the autophagy-mediated drought tolerance in tomato [82]. Although it has been proven that the submergence-sensitive phenotype of atatg2, atatg5, atatg7, and atatg10 was dependent on the SID2-mediated complete SA pathway, the expression of ET responsive regulators was also significantly altered in parallel with that of ATG genes upon submergence in Arabidopsis [62]. Therefore, it is intriguing to ask whether ET signaling-associated TF, such as ethylene insensitive-2 (EIN2) and EIN3, could also modulate the autophagy activity by regulating the expression of ATG genes. On the other hand, ET regulates the waterlogging through the modulation of GA-mediated elongation of internode in rice [83], implying there might be distinct crosstalk of autophagy with ET signaling between dicot and monocot plants. Taken together, these studies indicated that ET interplays with autophagy in both stress response and development in plants.
Although auxin could trigger the TOR pathway to regulate autophagy [38], it is reasonable to propose that auxin may also directly inhibit autophagy through auxin response factor (ARF) transcription factor, which may bind to the AtATG promoter and then modulate the gene expression (Figure 2), because the cis-elements of ARF have been found in the AtATG promoters [16]. However, this hypothesis still needs to be further explored, including the analysis of the co-expression pattern of ARF and AtATGs and the binding of ARFs with AtATG promoters. As an antagonist of auxin, ABA promotes bud dormancy, leaf shedding, and inhibition of cell growth. It has been mentioned that raptor1b mutant was unable to inhibit autophagy by exogenous NAA application [33]. Nonetheless, raptor1b mutant also presented a decreasing ABA level [84], suggesting that RAPTOR1B-mediated autophagy might be associated with ABA metabolism or signal. Furthermore, overexpression of the gene encoding heat-shock transcription factor A1a (HsfA1a) enhanced autophagy activity in tomato, whereas down-regulation of HsfA1a raised the plant sensitivity to ABA-mediated stomatal closure [85]. In addition, the Arabidopsis tryptophan-rich sensory protein (AtTSPO) was not only induced upon osmotic and salt stresses, but was also induced by ABA and then physically interacted with ATG8 via its AIM [86,87]. Moreover, the other two ATG-interacting proteins, ATI1 and ATI2, associated with the ER and chloroplast development, were involved in ABA-mediated seed germination [88]. Notably, TOR can phosphorylate ABA receptor PYL under favorable conditions so as to prevent the activation of stress response, which also attenuated the activity of SnRK2 kinases. Conversely, the ABA-activated SnRK2 can phosphorylate RAPTOR, thus inhibiting TOR-mediated autophagy [84]. These studies revealed that crosstalk between autophagy and ABA signaling is mediated by the phosphorylation modification of corresponding regulators [17]. GA antagonistically interplays with ABA in multiple biological processes, but little has been known about this antagonism in regulating autophagy. However, it has been implicated that GA could repress the positive regulator of ABA signaling, SnRK2, in rice [89], implying that GA might be also involved in regulating autophagy through the ABA-SnRK2 signaling pathway.
AtATG7, and AtATG10 also play positive roles in regulating submergence response, finally mediating osmotic stress. Under abiotic stress, AtATG7 positively regulates necrotrophic fungal pathogen resistance, and pexRD54 arrests pathogen infection by boosting autophagy activity. Moreover, autophagy positively regulates hypersensitive response (HR) cell death to resist biotic stress. Solid lines represent the activation or repression with known evidence. Dashed lines represent the proposed activation or repression.

The Regulation of Autophagy by Hormones
Autophagy could be regulated by hormones at the transcriptional level while hormones could be also modulated by autophagy in response to various stresses ( Figure 2). Transcriptome analyses in petunia and Arabidopsis clearly indicated that autophagic genes could be transcriptionally regulated by hormones [77][78][79], implying phytohormones may modulate autophagy through the signaling transduction. Figure 2. Regulation of autophagy by plant hormones. Phytohormones can modulate autophagy at the transcriptional level and through protein regulations. In respect to the former, the transcription factors ethylene response factor 5 (ERF5) in ethylene pathway and brassinazole-resistant 1 (BZR1) in the brassinolide (BR) pathway directly bind to the corresponding ATG promoters and then activate gene expression to promote autophagy. In contrast, the auxin regulator auxin response factor (ARF) also likely binds to the AtATG8 promoter to repress its expression, eventually leading to attenuating autophagy activity. In addition, auxin also can repress autophagy by promoting target of rapamycin (TOR) activity. On another hand, abscisic acid (ABA) can promote the SnRK2 and TSPO to positively regulate autophagy. By contrast, gibberellin (GA) seems to antagonize ABA in regulating autophagy through inhibiting SnRK2 activity. Alternatively, GA may also directly modulate autophagy through an unknown component. Jasmonic acid (JA) and salicylic acid (SA) induce the expression of WRKY33, Figure 2. Regulation of autophagy by plant hormones. Phytohormones can modulate autophagy at the transcriptional level and through protein regulations. In respect to the former, the transcription factors ethylene response factor 5 (ERF5) in ethylene pathway and brassinazole-resistant 1 (BZR1) in the brassinolide (BR) pathway directly bind to the corresponding ATG promoters and then activate gene expression to promote autophagy. In contrast, the auxin regulator auxin response factor (ARF) also likely binds to the AtATG8 promoter to repress its expression, eventually leading to attenuating autophagy activity. In addition, auxin also can repress autophagy by promoting target of rapamycin (TOR) activity. On another hand, abscisic acid (ABA) can promote the SnRK2 and TSPO to positively regulate autophagy. By contrast, gibberellin (GA) seems to antagonize ABA in regulating autophagy through inhibiting SnRK2 activity. Alternatively, GA may also directly modulate autophagy through an unknown component. Jasmonic acid (JA) and salicylic acid (SA) induce the expression of WRKY33, and then WRKY33 directly triggers the expression of ATG genes, consequently promoting autophagy. Solid lines represent the activation or repression with known evidence. Dashed lines represent the proposed activation or repression.
Plants 2020, 9, 1038 9 of 16 SA plays an essential role in the activation and regulation of biotic and abiotic stress responses [90]. A recent study has shown that a high level of SA caused autophagy-mediated PCD in apple, and the phenotype of accelerated PCD during senescence and immunity in atatg5 mutant was through the SA-dependent rather than the intact JA or ET signaling pathway [49]. Similar to SA, JA also participates in response to various biotic stresses, and the JA-related WRKY genes have already been implicated as mediating autophagy gene expression upon heat stress and fungal pathogen infection [17]. For example, WRKY33 was not only involved in the JA-mediated signaling pathway to regulate plant resistance to necrotrophic fungal pathogens, but also directly interacted with ATG18a to regulate autophagy in Arabidopsis [17,91], suggesting WRKY33 coordinates the JA signaling and autophagy pathway to regulate the pathogen stress.
Additionally, the BR-activated transcription factor brassinazole-resistant 1 (BZR1), functioning as a positive regulator of the BR signaling pathway, was found to also directly bind to the promoters of SlATG2 and SlATG6 in tomato [92]. Considering the homologous conservation of BZR1 in plants, such as Arabidopsis and rice, it is supposed that BR could also regulate autophagy through BZR1-dependent regulation of ATG expression.
Actually, the crosstalk between autophagy and various phytohormone signaling is indeed complicated. For example, a study has been demonstrated that the decreased resistance of banana to Fusarium wilt by inhibiting autophagy could be rescued by exogenous ET, SA, and JA [80], suggesting autophagy might also in turn modulate the homeostasis of phytohormones. This topic is further discussed below.

Autophagy Regulates Hormone Biosynthesis and Signaling
Apart from being regulated by hormones, autophagy can also influence hormone biosynthesis and signaling (Figure 3). For instance, a previous study has indicated that SA is accumulated in the atatg5 mutant [49]. Furthermore, two further studies revealed that the SA signaling genes, including EDS1, PAD4, SID2, and nonexpresser of PR genes (NPR) 1-4, and the ET biosynthetic and signaling genes, including AtACS2, ethylene response 2 (ETR2), and constitutive triple response 1 (CTR1), were upregulated in atatg5 and atatg9 mutants upon energy starvation [79]. It is worthwhile mentioning that the soybean EIN3 accumulated upon starvation stress [82], implying that autophagy might be involved in the ET signaling transduction through selective degradation of this protein. Overexpression of MdATG18a resulted in less H 2 O 2 but more SA, thereby enhancing the resistance to Diplocarpon mali infection [93]. In addition to SA, it has also revealed that the endogenous CK and GA concentration was significantly reduced in osatg7 mutant in rice, and exogenous application of GA partially restored the pollen defect of osatg7 [94]. In contrast to the Arabidopsis atatg5 and atatg7, the contents of SA, JA, and ABA were not obviously altered in the osatg7, which might be due to different tissues used in the experiments or there is indeed a distinct role of autophagy in regulating phytohormones in rice. To address this issue, the metabolic profiling of Arabidopsis pollen and rice leaf are needed. In addition, the selective autophagy also regulated BR signaling through degrading the transcription factor BRI1-EMS-suppressor 1 (BES1) through the interaction of ATG8 with dominant suppressor of KAR 2 (DSK2) that binds BES1 [95]. Nevertheless, the interaction of NBR1 with ABA regulator protein suggests that NBR1 also plays a role in ABA signaling by modulating its homeostasis or activity. On the other hand, NBR1 directly interacts with ATG8, further suggesting an autophagic route-dependent role of NBR1 in fine-tuning ABA-mediated drought tolerance [13,72]. Collectively, these studies demonstrated that autophagy modulates the dynamic homeostasis of phytohormone level in addition to the signaling transduction. However, whether autophagy directly controls the turnover of the phytohormone biosynthetic proteins or the compounds remains elusive.

Future Perspectives
A steadily growing amount of evidence has revealed the essential role of autophagy in plant growth, development, and stress adaptation [36,42,48]. However, the synergistic interaction between autophagy and phytohormones upon various stresses still remains to be further exploited. Moreover, the specific regulators underlying their crosstalk needs to be identified and fully characterized. More than 20 selective autophagy receptors have been characterized from various plants, which contain the specific Atg8-interacting motif (AIM) for direct interaction with ATG8 [3,96]. The AIM generally consists of [WFY]-X-X-[LIV] consensus sequences, in which the W site is restricted by either W, F, or Y amino acid, and the L site is either L, I, or V, whereas the X represents any amino acid. Recently, two bioinformatic analyses rephrased the regular pattern of the consensus of AIM. One regular expression pattern of AIM is the [

ADEFGLPRSK] [DEGMSTV] [WFY] [DEILQTV]
[ADEFHIKLMPSTV] [ILV] that is termed the extended LC3-interacting region (LIR) motif (xLIRmotif) [96], while the other is composed of five regular patterns with the preference of acidic amino acids surrounding the W and L site [97]. Therefore, identification of AIM-containing proteins by bioinformatic analysis of these consensus sequences may provide a cue for autophagy-targeted, phytohormone-related proteins in addition to the traditional yeast two-hybrid screening. In the autophagic machinery, ATG5 and ATG7 are responsible for the conjugation of ATG8 to phosphatidylethanolamine (PE), which is essential for the formation of ATG8-mediated phagophore. Subsequently, the expansion of phagophore membrane and vesicle nucleation is modulated by the ATG9, which is accompanied by its interaction with ATG18, finally leading to the generation of entire autophagosome. The phytohormone-related proteins, including BRI1-EMS-suppressor 1 (BES1) and dominant suppressor of KAR 2a (DSK2a) relevant to brassinolide (BR), ATI1/2, and NBR1 relevant to ABA, and unknown components from cytokinin (CK) and GA, are transported into autophagosome by interacting with ATG8, eventually being degraded in the vacuole. (B) Regulation of phytohormones homeostasis by autophagy. The activation of autophagy (A) results in the suppression of phytohormones genes, such as the enhanced disease susceptibility 1 (EDS1), PAD4, salicylic acid induction deficient 2 (SID2) and nonexpresser of PR genes (NPRI)1-4 that are involved in regulating SA signaling, and ACS, ERT2 and constitutive triple response 1 (CTR1) that are involved in regulating ET biosynthesis and signaling.

Future Perspectives
A steadily growing amount of evidence has revealed the essential role of autophagy in plant growth, development, and stress adaptation [36,42,48]. However, the synergistic interaction between autophagy and phytohormones upon various stresses still remains to be further exploited. Moreover, the specific regulators underlying their crosstalk needs to be identified and fully characterized. More than 20 selective autophagy receptors have been characterized from various plants, which contain the specific Atg8-interacting motif (AIM) for direct interaction with ATG8 [3,96]. The AIM generally consists of [WFY]-X-X-[LIV] consensus sequences, in which the W site is restricted by either W, F, or Y amino acid, and the L site is either L, I, or V, whereas the X represents any amino acid. Recently, two bioinformatic analyses rephrased the regular pattern of the consensus of AIM. One regular expression pattern of AIM is the [

ADEFGLPRSK] [DEGMSTV] [WFY] [DEILQTV] [ADEFHIKLMPSTV]
[ILV] that is termed the extended LC3-interacting region (LIR) motif (xLIR-motif) [96], while the other is composed of five regular patterns with the preference of acidic amino acids surrounding the W and L site [97]. Therefore, identification of AIM-containing proteins by bioinformatic analysis of these consensus sequences may provide a cue for autophagy-targeted, phytohormone-related proteins in addition to the traditional yeast two-hybrid screening. Additionally, a recent study revealed that the ubiquitin-interacting motif Plants 2020, 9, 1038 11 of 16 (UIM) could also interact with ATG8 [98], providing a wider range of target protein candidates that may be phytohormone-or stress-related.
Recent studies have elaborated that overexpressing either OsATG8a or OsATG8c positively enhanced the yield and NUE in rice and the ectopic expression of OsATG8b in Arabidopsis also increased the yield and NUE [26,99,100], indicating that autophagy possesses great potential for boosting agronomic productivity under suboptimal condition in crops. However, whether such autophagy-mediated regulation is related with phytohormones is still poorly understood. Given the role of autophagy in turning over proteins, it may be quite interesting to explore whether phytohormone-related proteins that mediate yield and productivity are autophagy substrates. On the other hand, given that autophagy positively regulates stress response, it is worthwhile to decipher how autophagy coordinates phytohormones to maintain the cellular homeostasis under normal conditions and how it triggers the stress response upon unfavorable conditions. In summary, further exploring the regulatory network between autophagy and phytohormone signaling would extend our understanding about the stress regulation and consequently provide some new strategies and candidates for crop improvement, eventually promoting both stress resistance and yield.