The Interplay between Hydrogen Sulfide and Phytohormone Signaling Pathways under Challenging Environments

Hydrogen sulfide (H2S) serves as an important gaseous signaling molecule that is involved in intra- and intercellular signal transduction in plant–environment interactions. In plants, H2S is formed in sulfate/cysteine reduction pathways. The activation of endogenous H2S and its exogenous application has been found to be highly effective in ameliorating a wide variety of stress conditions in plants. The H2S interferes with the cellular redox regulatory network and prevents the degradation of proteins from oxidative stress via post-translational modifications (PTMs). H2S-mediated persulfidation allows the rapid response of proteins in signaling networks to environmental stimuli. In addition, regulatory crosstalk of H2S with other gaseous signals and plant growth regulators enable the activation of multiple signaling cascades that drive cellular adaptation. In this review, we summarize and discuss the current understanding of the molecular mechanisms of H2S-induced cellular adjustments and the interactions between H2S and various signaling pathways in plants, emphasizing the recent progress in our understanding of the effects of H2S on the PTMs of proteins. We also discuss future directions that would advance our understanding of H2S interactions to ultimately mitigate the impacts of environmental stresses in the plants.


Introduction
The in-depth understanding of mechanisms/processes involved in plant growth and development is critical for improving crop quality and productivity, as well as the development of more stable and climate-resilient crops. Due to their sessile nature, plants have evolved several adaptive mechanisms for survival. Among them, phytohormones are complex signaling factors that regulate a myriad of physio-biochemical processes to maintain optimum growth, development, and performance [1]. The synthesis and level of hormones could vary significantly in different plant tissues, during different developmental stages, and under different environmental conditions [2]. Furthermore, there is less knowledge about the coordination of the spatial and temporal distribution of plant hormones and how these dynamic processes trigger diverse responses in plants [3].
Recently, numerous investigations have revealed hydrogen sulfide (H 2 S) as one of the critical components in various acclimation processes in plants under normal and stressful 2 of 29 conditions ( Figure 1). H 2 S is a colorless, lipophilic, toxic, volatile, inflammable, and watersoluble gas with a pungent odor, similar to that of rotten eggs. Amidst the emergence of life on Earth approximately 3.8 billion years ago, H 2 S acted as a major energy source; however, H 2 S-dependent organisms disappeared after a burst of oxygen [4]. Nevertheless, the biogeochemical sulfur cycle was preserved in organisms and is presently limited to some vital metabolic and signaling events [5,6]. H 2 S receives extensive attention in the animal field due to its multiple physiological and pathophysiological functions in different organs due to clear and well-established experimental models/approaches [7]. However, it was not until recently that the roles of H 2 S in plants have gained the attention of scientists due to the involvement of H 2 S in adverse stress conditions via regulation of gene expression, post-translational modifications (PTMs), and crosstalk with other gaseous signals and phytohormones [8,9]. stressful conditions (Figure 1). H2S is a colorless, lipophilic, toxic, volatile, inflammable, and water-soluble gas with a pungent odor, similar to that of rotten eggs. Amidst the emergence of life on Earth approximately 3.8 billion years ago, H2S acted as a major energy source; however, H2S-dependent organisms disappeared after a burst of oxygen [4]. Nevertheless, the biogeochemical sulfur cycle was preserved in organisms and is presently limited to some vital metabolic and signaling events [5,6]. H2S receives extensive attention in the animal field due to its multiple physiological and pathophysiological functions in different organs due to clear and well-established experimental models/approaches [7]. However, it was not until recently that the roles of H2S in plants have gained the attention of scientists due to the involvement of H2S in adverse stress conditions via regulation of gene expression, post-translational modifications (PTMs), and crosstalk with other gaseous signals and phytohormones [8,9].
The fine-tuned interaction of H2S with other gaseous signaling biomolecules and hormones orchestrates molecular, metabolic, and physiological adaptive responses and permits the plants to respond properly to changing environmental conditions. In this review article, we will explain the central role of H2S in the regulation of various physiological and molecular processes. We will also discuss how hormonal homeostasis plays a crucial role in stress conditions and how H2S synergistically/antagonistically regulates the biosynthesis and degradation of the associated plant hormones and modulates their signaling to generate adaptive responses in plants. Overview of hydrogen sulfide (H2S) production and the regulation of several physiological, metabolic, and morphological processes by H2S to optimize growth in plants.

H2S Biosynthesis in Different Organelles and Associated Enzymes
Plant roots absorb sulfate (SO4 2− ), which is reduced into H2S via the action of APS reductase (adenosine-5′-phosphoryl sulfate reductase) and SiR (sulfite reductase). H2S is later transformed into cysteine amino acid via catalysis of O-Acetylserine (thiol) lyase (OASTL), as a final step of sulfate assimilation in plants ( Figure 2). In A. thaliana, cytosolic

Role of H2S in the Modulation of Abiotic Stress Responses
H2S plays a vital role in protecting plants against several abiotic stressors. Environmental stress factors such as salinity, drought, waterlogging, high temperature, excessive light, heavy metals, and chilling could adversely affect plant growth and development ( Figure 3) [40][41][42][43]. Generally, under most stress conditions, plants reduce uptake of CO2 due to the closure of stomata and limiting CO2 fixation. This condition causes alternation in cell metabolism due to restricted photosynthetic capacity that leads to the generation by APS reductase after it is activated to APS. Under the catalysis of SiR, the sulfite is then reduced to sulfide (S 2− ) using six electrons transferred from ferredoxin. As a result, sulfide is produced, which is used to produce cysteine. The OASTL enzyme catalyzes the synthesis of cysteine along with O-acetylserine. The enzyme CDes and pyridoxal 5-phosphate (PLP) participate in degrading cysteine to generate H 2 S. In mitochondria, serine acetyltransferase (SAT) catalyzes the conversion of serine (Ser) into OAS and produces cysteine, which is converted to H 2 S via the catalytic activity of β-cyanoalanine synthase (β-CAS).
H 2 S is also synthesized in the chloroplasts and mitochondria when cysteine is reduced by cysteine desulfhydrase (CDes) and β-cyanoalanine synthase (β-CAS), respectively ( Figure 2). Genetic and molecular evidence indicated that mitochondrial isoforms of CAS are CYS-C1 (At3g61440) and OAS-C (At3g59760), and chloroplastic isoforms of CAS are OAS-B (At2g43750) and SCS (At3g03630) [17]. The cytosolic release of H 2 S is dependent upon the functioning of D/L cysteine desulfhydrases (L/D-CDes). Several L-CDes of the Arabidopsis plant are well characterized and are involved in the breakdown of L-cysteine to sulfide, NH 3, and pyruvate [18][19][20]. However, D-CDes are completely different proteins and belong to the pyridoxal 5-phosphate (PLP)-dependent enzyme superfamily, and its activity is PLP dependent [21,22]. The model plant Arabidopsis contains two putative D-cysteine desulfhydrases (D-CDes) genes (At1g48420 and At3g26115) [21][22][23], while two D-CDes are also functionally characterized in rice (OsDCD1 and OsLCD2) and some other crops [24,25]. The D-cysteine desulfhydrases 2 carry out the decomposition of both L-and D-Cystine into H 2 S. Accumulating evidence signifies that NifS-like L-CDes are also involved in the generation of H 2 S. The presence of H 2 S in plant peroxisomes and its interaction with catalase is also observed; however, the synthesis mechanisms and involved enzymes are still unknown [26].
The mitochondria play a vital role in the catabolism of H 2 S and maintain its steadystate levels in cells. In mitochondria, H 2 S is generated during cyanide detoxification through the catalysis of β-CAS. The functional mitochondria isoform of CAS is CYS-C1 (At3g61440), which catalyzes the conversion of cysteine and cyanide into hydrogen sulfide and β-CAS and maintains optimum levels of cyanide to prevent phytotoxicity [27]. This yielded H 2 S is converted back into cysteine via mitochondrial OASTL (OAS-C, At3g59760), which will again be used in the detoxification of cyanide. This process is considered a cyclic pathway of cysteine generation via H 2 S consumption in mitochondria [28]. Under stress conditions, excess accumulation of H 2 S raises the pH of mitochondria, leading to the conversion of H 2 S into hydrosulfide ions (HS − ). Excess accumulation of H 2 S also prevents the loss of H 2 S from mitochondrial membranes and maintains H 2 S homeostasis ( Figure 2). The environmental cues also modulate the endogenous H 2 S biosynthesis by stimulating desulfhydrase activities in plant cells [18].
In plastids, the reduction of sulfate to sulfide and its incorporation into the OAS is executed as an entry point of reduced sulfur to plant metabolism for growth and development via a photosynthetic sulfate assimilation pathway [18,29]. The OAS interaction with serine acetyltransferase (SAT) forms a cysteine synthase complex (CSC), which generates demand-driven synthesis of cystine in plant cells [30,31]. Subsequently, the breakdown of cysteine in the chloroplast generates H 2 S due to the catalysis of DES1 and L/D-cysteine desulfhydrase ( Figure 2). The generation of H 2 S in chloroplasts acts as a signaling molecule because it substantially impacts cellular metabolism by limiting the rate of photosynthesis.
The peroxisome is an essential single membrane-bound organelle involved in the metabolism of reactive nitrogen species (RNS), including H 2 S [26,32,33]. Recent studies demonstrated the presence of H 2 S in plant peroxisomes [34]. Some studies speculated that peroxisomes have the capacity to transform sulfite to sulfate under the catalysis of Sulfite oxidase (At3g01910) in A. thaliana. Presently, no enzymatic source for H 2 S metabolism has been observed in the peroxisome of Arabidopsis, and tomato [34][35][36]; the mechanism of H 2 S production in peroxisome is still obscure. The H 2 S characterization study in Solanum lycopersicum showed the localization of OASTL9 in the peroxisome, which exhibited upregulation under different developmental stages and pathogenic bacterial treatments [36].
In the plant, several additional enzymes are also involved in H 2 S synthesis, and most of the H 2 S in the cell is produced during the necessary consumption of cysteine. For example, At5g28030 encodes a cysteine synthase (CS)-like protein that degrades L-cysteine and produces H 2 S [28]. This protein is also localized in the cytoplasm as AtDES1 (desulfhydrase). The homolog of this protein in Brassica napus (BnDES) is also involved in the breakdown of cysteine [37]. However, AtDES1 homolog in rice (OsLCD2) exhibits cysteine biosynthesis activity [38]. The Arabidopsis nitrogen fixation-like 1 and 2 (At5g65720; At1g08490) also use L-cysteine as a substrate and produce H 2 S during the synthesis of L-alanine in the cytosol [20,28,39]. This diversity in enzymatic functioning and discrepancies in their substrates' catalyzation may allow the plants to calibrate endogenous H 2 S levels according to their requirements and external prompts.

Application of H2S in Plant Drought Responses
During osmotic stress, improved water status of plants is a vital survival strategy that is achieved via accumulating osmolytes to maintain normal hydration levels. Exposure to drought stress or PEG-induced osmotic stress in plants enhances the accumulation of osmolytes such as proline and glycine betaine to maintain normal water status in stressed plants. However, sometimes the accumulation of these osmolytes fails to maintain adequate water status due to the severity of osmotic stress [50,52]. The endogenous stimulation of H2S regulates the proline synthesizing enzyme via stimulating the expression of 1pyrroline-5-carboxylate synthetase, and by inhibiting the activity of the proline-degrading enzyme. On the other hand, H2S also triggers the activity of glycine betaine biosynthesis enzymes (aldehyde dehydrogenase), which reduce the osmotic stress and assist the plants in enhancing osmotic pressures to improve water uptake and relative water content in vital tissues [57,58]. The pre-exposure of SO2 to drought-stressed wheat plants showed a pronounced increase in endogenous H2S. This inflation may be caused by the conversion of SO2 into the SO3 2− and decomposition of L-/D-Cys, which generates enough H2S to initiate drought adaptive responses in the stressed seedling. However, when hypotaurine (HT; H2S scavenger) was applied on SO2-pretreated seedlings, reduced content of H2S and severe symptoms of drought toxicity appeared in seedlings. In addition, endogenous generation of H2S via pretreatment of SO2/NaHS, fully activated the antioxidant enzymes (SOD, CAT, and POD) and reduced the production of H2O2 and MDA content in drought-

Application of H 2 S in Plant Drought Responses
During osmotic stress, improved water status of plants is a vital survival strategy that is achieved via accumulating osmolytes to maintain normal hydration levels. Exposure to drought stress or PEG-induced osmotic stress in plants enhances the accumulation of osmolytes such as proline and glycine betaine to maintain normal water status in stressed plants. However, sometimes the accumulation of these osmolytes fails to maintain adequate water status due to the severity of osmotic stress [50,52]. The endogenous stimulation of H 2 S regulates the proline synthesizing enzyme via stimulating the expression of 1-pyrroline-5-carboxylate synthetase, and by inhibiting the activity of the proline-degrading enzyme. On the other hand, H 2 S also triggers the activity of glycine betaine biosynthesis enzymes (aldehyde dehydrogenase), which reduce the osmotic stress and assist the plants in enhancing osmotic pressures to improve water uptake and relative water content in vital tissues [57,58]. The pre-exposure of SO 2 to drought-stressed wheat plants showed a pronounced increase in endogenous H 2 S. This inflation may be caused by the conversion of SO 2 into the SO 3 2− and decomposition of L-/D-Cys, which generates enough H 2 S to initiate drought adaptive responses in the stressed seedling. However, when hypotaurine (HT; H 2 S scavenger) was applied on SO 2 -pretreated seedlings, reduced content of H 2 S and severe symptoms of drought toxicity appeared in seedlings. In addition, endogenous generation of H 2 S via pretreatment of SO 2 /NaHS, fully activated the antioxidant enzymes (SOD, CAT, and POD) and reduced the production of H 2 O 2 and MDA content in drought-stressed plants [41,47,59,60]. The endogenous H 2 S modulation in plants also activated the expression of transcription factors (TFs) such as ERF1, NAC69, and MYB30 [41,61]. The findings of several studies indicated that TF NAC69 could confer resistance in drought-stressed plants via the H 2 S mediated ABA signaling pathway.
Additionally, the upregulation of TFs such as ERF1 and MYB30 may activate signal transduction pathways and regulate stress-responsive gene expression profiling under drought stress conditions [62][63][64]. Since the application of H 2 S scavengers inhibited the transcript abundance of ERF1, NAC69, and MYB30 in wheat plants under drought stress conditions, there must be direct involvement of H 2 S in the regulation of stress-related TFs in response to drought stress [61,65,66]. Some studies also recognized that H 2 S signaling in response to drought stress influences the functioning of ABA biosynthesis genes such as NCED2, NCED3, and NCED5 and suppresses the ABA catabolic genes (ABA8ox1, ABA8ox2, and ABA8ox3), which is consistent with ABA accumulation in drought-stressed plants [47,50].

Role of H 2 S in the Alleviation of Metal Stress
Under metal toxicity, plants modulate several metal/metalloid ions from toxic to less toxic forms, such as reduction of arsenate (AsV) to arsenite (ASIII), and hexavalent chromium (Cr (VI) ) to less toxic trivalent Cr (III) , and sequester these metal ions via thiols (GSH) and phytochelatins (PCs) ligands [64]. These metabolites (GSH and PCs) actively participate in the intracellular redox balance and metal tolerance capacity of crop plants and prevent the cells from entering programmed cell death or necrosis phases [67,68]. Due to metal-induced oxidative stress, the intracellular redox becomes oxidized, decreasing levels of reduced molecules such as NADH/NADPH and allowing apoptosis or necrosis to be initiated. The endogenous production of H 2 S or exogenous application of H 2 S donors assists in maintaining the levels of GSH and phytochelatins in the plant to sustain optimum redox balance and the sequestration of toxic metal ions into the vacuoles [41,69]. The GSH and PCs are sulfur enriched compounds, whereas, in sulfur metabolism, metabolites such as sulfite, H 2 S, cysteine, and GSH are highly interconnected, and depletion of GSH during metal toxicity could potentially accelerate cysteine breakdown and ultimately enhance the GSH and H 2 S supply to the cell [16,67]. In several published studies, it is observed that the mitigation effects of H 2 S under different abiotic stresses and metal excess conditions are related to the upregulation or superior maintenance of redox-active compounds such as ASA-, GSH, and PCs [40,67,69,70]. This finding of these studies provides compelling evidence that modulation of endogenous H 2 S during stressful conditions could help the plant to maintain or reduce the loss of intracellular glutathione, which supports the overall redox positive state of the cell and verifies that H 2 S has an important influence on cell functions under stressful conditions [41,70,71].
H 2 S not only overcomes ROS-induced toxicity in metal exposed plants but also plays an effective role in the inhibition of metal transport and absorption. H 2 S has the ability to alter chemical forms of metal ions into insoluble phosphate compounds, which decreases metal toxicity and movements [72]. However, the metal reduction capacity of H 2 S is much lower than GSH, cysteine, phytochelatins, and metallothioneins [73]. H 2 S mediated reduction in metal transport/immobilization is usually associated with downregulation of metal transporters or secretion of chelating compounds to prevent the further translocation of metal ions to the sensitive tissues or uptake from the root zone. For example, in several crop plants, exogenous application of H 2 S intensifies the citrate secretion and expression of citrate transporters, so the non-toxic complexes of citrate with Al 3+ could be formed in the rhizosphere [74][75][76]. Similarly, H 2 S also suppresses pectin methyl esterase activity, which suppresses Al 3+ binding sites by reducing negative charge in root cells, which has direct implications for Al 3+ tolerance [77,78]. In the case of Cd metal, H 2 S triggers the expression of phytochelatin synthase (PCS) and the Cd-ATPase gene to effectively chelate and transport metal ions into the vacuoles through the help of HMT transmembrane transporter channels [79]. The L-DC-mediated H 2 S accumulation modulates root pectin content with a lower degree of methylation to facilitate the binding of Cd 2+ to the cell wall, which ultimately diminishes its further translocation from root to shoot and toxicity symptoms in exposed plants [80]. In Arabidopsis, exogenous application of H 2 S activated the generation of Cr 6+ binding peptides, such as phytochelatins and metallothioneins, to carry toxic Cr 6+ to insensitive regions mediated by compartmentalization [81,82]. Based on these studies, we infer that H 2 S plays a pivotal role in the chelation of heavy metals for inactivation and later sequesters them into the vacuole to increase the metal stress tolerance of plants.

Effect of H 2 S on Plant Salt Tolerance
Salinity is a major constraint limiting agriculture productivity due to poor irrigation practices and continuous climate fluctuations [83]. Saline stress imposes both osmotic stress and ionic toxicity, which retard plant growth and productivity. The unregulated accumulation of sodium (Na + ) hinders water and nutrient uptake and induces water deficit conditions for plants. Furthermore, an excessive amount of Na + and chloride (Cl − ) accumulation in plants disturbs ionic homeostasis. The depolarization of membranes leads to the loss of potential stress mitigating ions such as K + and Ca 2+ and induces changes in transpiration rate, photosynthesis, oxidative stress, etc. [84][85][86]. Saline stress in plants reinforces several physiological, molecular, and metabolic disorders that completely inhibit plant growth [87][88][89]. The maintenance of ionic homeostasis and a lower cytosolic Na + /K + ratio is critical for salt adaptation and tolerance. It is observed that several Na + /K + ion transporters and stress-responsive gene activation pathways are interconnected with plant hormones because stress and growth hormones are spatially involved in mediating saltstress signaling and maintaining the balance between stress responses and growth in plants [83,87,88]. In this regard, H 2 S biosynthesis and signaling are implicated in saline stress tolerance in plants. [90][91][92][93]. Several studies demonstrated that exogenous application of H 2 S reduces the uptake of Na + and increases the accumulation of K + that untimely preserves an optimal Na + /K + ratio for the plant's vital functioning. [90][91][92][93]. It is proven via pharmacological studies that when H 2 S scavengers were applied to the salt-stressed plants, the depletion of endogenous H 2 S aggravated the saline stress symptoms and increased the Na + /K + ratio and cytosolic concentration of Na + in studied plants. These studies also highlighted that H 2 S application significantly maintains K + homeostasis in plants by preventing K + leakage by reducing oxidative stress-mediated lipid peroxidation and membrane depolarization. [90][91][92][93]. At the molecular level, it was observed that H 2 S regulated the activity of SKOR (outward rectifying K + channel) by inhibiting its expression and preventing the loss of K + into the xylem under saline stress conditions. However, when H 2 S scavengers (DL-propargylglycine or HT) were applied to the plants, SKOR expression was not compromised. [90][91][92][93]. Similarly, the K + retention during saline stress conditions normalizes H + -ATPase, because H + gradient-mediated H + -ATPase activity repolarizes the PM to accelerate potassium influx and sodium efflux [90][91][92][93]. This repolarization occurs because H 2 S is involved in the stimulation of gene expression and phosphorylationmediated upregulation of H + -ATPase activity under salinity [94,95]. This observation suggests that H 2 S shows the implication of K + uptake and its homeostasis via upregulating the K + /Na + antiport system through modulating H + -ATPase activity [42,91,92,95]. Besides this, AKT1 (inward rectifying potassium channels) is located in root epidermal tissue [96], and HAK5 (potassium transporter) gene is located in the tonoplast and the PM [96]. These genes are also coupled with maintaining K + and plant resistance to salt. The exogenous application of H 2 S donors improved the transcript expression of AKT1 and HAK5 and total K content in the salt-challenged Brassica napus plant [97]. Similarly, NaHS induced H 2 S promoted the expression of HvAKT1 and HvHAK5 in roots of barley seedlings under salinity [8]. All these findings advocate that the potential increase in H 2 S and its signaling is a positive regulator of K + homeostasis and maintenance of the Na + /K + ratio during saline stress in plants [8,95,98,99].
The (SOS) pathway is critical for the exclusion of Na + under saline stress conditions. SOS1 is involved in the long-distance transport of Na + from roots to shoots [95,100]. The increase in transcript abundance of SOS1 favors the accumulation of SOS1 proteins in the PM, which triggers the exclusion of Na + from cells and minizines the Na + load in the cytosol [60]. The H 2 S application under alkaline and normal salt stress conditions stabilizes the mRNA level of SOS1, which leads to the reduced Na + content in the roots of cultivated apple plants [101]. SOS1 is regulated by the H + gradient provided by PM H + -ATPase. Several studies identified that H 2 S positively influences the gene expression and phosphorylation of PM H + -ATPase under salinity [102]. In pharmacological experiments where endogenous H 2 S production was inhibited, the expression level of SOS1 and related Na + antiporters were downregulated, and salinity tolerance of plants was compromised due to unregulated accumulation of Na + in sensitive tissues [100]. The PM H + -ATPase on the membranes of vacuoles also regulates the expression and activation of the Na + /H + antiporter, because the compartmentalization of Na + ions into the vacuoles is an alternative solution to decrease the Na + induced toxicity in cells [42,103]. The H 2 S application greatly induces the transcript accumulation of NHX2 and VHA-β genes (Na + /H + antiporter) in salt-exposed plants. This finding also advocates that Na + caging in vacuoles is influenced by H 2 S signaling [8,85]. Meanwhile, for the regulation of Na + /K + homeostasis, H 2 S also controls the H 2 O 2 mediated activity of PM-bound NADPH oxidases [104]. For instance, PM NADPH oxidase inhibitor (diphenyleneiodonium chloride) suppressed the H 2 S mediated increase in H 2 O 2 in the root of Arabidopsis under salinity. The application of ROS scavenger (N,N'-Dimethylthiourea) abolished the H 2 S mediated H 2 O 2 production in salt stress plants due to the Na + uptake being high in salt-stressed plants from the absence of H 2 S mediated activation of NADPH oxidase [104]. This conclusion indicates that H 2 O 2 might act as a downstream signal for H 2 S-mediated Na + /K + homeostasis [85,104,105]. The findings of these studies demonstrate that H 2 S regulated signaling influences the activity of H + -ATPase and the expression of PM Na + /H + antiporter that enhances the salt tolerance by maintaining Na + /K + homeostasis in plants [85,106].

Crosstalk of H 2 S with Signaling/Phytohormones under Changing Environmental Conditions
Phytohormones, or plant growth regulators (PGRs), are the most significant signaling molecules, synthesized in specific locations within plants, and can be translocated to different parts to regulate stress responses [106]. PGR such as abscisic acid (ABA), auxins (IAA), brassinosteroids (BRs), cytokinins (CK), gibberellins (GA), jasmonic acid (JA), and salicylic acid (SA) help the plants to overcome numerous biotic/abiotic adversities by triggering physiological and molecular responses [107,108]. H 2 S, which acts as an endogenous gasotransmitter, is recognized in relevance with other signaling molecules such as NO [109], ROS [110], H 2 O 2 [111], CO [112], and plant hormones such as ABA [113], JA [114], GA [115] and ethylene. H 2 S in plants exhibits a dual role, either disseminated as pernicious cellular repercussion or as credible signaling molecules depending upon stress conditions. A study discovered that H 2 S operates downstream of NO and helps decrease oxidative stress during salt stress in tomatoes. H 2 S helps minimize postharvest ripening and senescence in bananas because it inhibits ethylene signaling as well as mitigating oxidative stress [115]. Additional studies revealed that H 2 S regulates NADPH oxidase (RBOH) activity, leading to ROS accumulation [116]. Simultaneously, the concentration of phosphatidic acid generated via phospholipase D [117,118] is also modulated by H 2 S, which helps further to inhibit the cellular signaling pathway [1]. In Arabidopsis, H 2 S operates upstream of the MAPKs pathway, and both of these work parallelly under cold stress conditions [119]. Various developmental processes such as organogenesis, seed germination, and the advent of senescence are spurred by H 2 S produced from sodium hydrosulfide (NaHS) and morpholin-4-ium 4-methoxyphenyl (morpholino) phosphinodithiolate (GYY4137) [119,120]. As a signaling molecule, H 2 S participates in several cross-talk networks amid H 2 O 2 , NO, CO, and phytohormone ABA during different stress conditions [121]. It is evident that signaling molecules such as H 2 S interplay an essential role in several stages of plant development because of the interaction between H 2 S and numerous phytohormones. In the future, genes involved in governing the new signaling molecules such as H 2 S could be targeted to develop a genetically improved crop.

Crosstalk of H 2 S and Abscisic Acid (ABA)
Plants modify ABA levels continually in response to changing physiological and environmental conditions, while bioactive ABA levels are sustained through a fine balance between generation and catabolism [45,86,87]. Several ABA receptors are involved in signal perception and transduction [45]. Earlier studies revealed that the interaction of H 2 S with ABA receptor genes implied that H 2 S regulates ABA signaling via influencing ABA receptors [45,122,123]. H 2 S application in drought-stressed plants upregulated the expression of potential ABA receptors such as RCAR (The regulatory component of ABA), ABAR (abscisic acid receptor), PYR1 (pyrabactin resistant protein), GTG1 (GPCR-type G proteins), and CHLH (H subunit of the Mg-chelatase) [45,124]. Some studies point out that ABA regulates many physiological processes, and H 2 S sometimes regulates these responses in a similar way [45,113,124]. Exogenous application of ABA triggers the endogenous production of H 2 S, suggesting complex crosstalk between two signaling molecules exists under drought stress conditions [45]. Similarly, under heat stress, ABA could trigger the accumulation of endogenous H 2 S and act as a new downstream gaseous signaling molecule that regulates ABA-induced stress responses in heat-stressed plants [45].
In plants, stomatal closure or opening is regulated by guard cells. The plant hormone ABA regulates the function of several ion channels in an ABA-dependent manner to control stomatal closure and opening [124][125][126][127][128]. A wealth of literature provides ample evidence that H 2 S regulates stomatal aperture in various plant species, and it may have implications for ABA-dependent stomatal closures in plants under stressful conditions [124]. The earlier study of Wang et al. [129] illuminated this underlying mechanism and revealed that exogenous application of H 2 S activates the S-type anion currents in guard cells of Arabidopsis. Concurrently, the elevated level of free Ca 2+ is a prerequisite for its activation [129]. H 2 S triggers Ca 2+ waves in guard cells. In guard cells, Ca 2+ sensing is perceived by a heterotrimeric G-protein β-subunit (AGB1) that collaborates in Ca 2+ induced stomatal closure in Arabidopsis [130]. Ca 2+ ions also activate SLAC1 by stimulating CPK (calcium-dependent protein kinase) activity. It was observed that lower concentrations of ABA partially impaired stomatal closure in CPK quadruple mutant plants; however, higher concentrations of ABA effectively close stomata. The application of Ca 2+ chelator (1,2-bis(o-aminophenoxy) ethane-N,N,N,N-tetraacetic acid (BAPTA) completely inhibited the ABA-mediated activation of anion channel in guard cells and prevented the ABAinduced stomatal closure [131,132]. These studies showed that H 2 S and ABA are signaling components in stomatal closure in plants.
A recent study demonstrated that H 2 S mediated persulfidation of SnRK2.6/OST1 in response to ABA signaling initiated stomatal closure ( Figure 4). In guard cells, SnRK2.6/OST1 acts as a core component of ABA signaling that controls stomatal movements, and its function is tightly regulated by H 2 S-mediated PTMs. Under certain physiological conditions, ABA induces the generation of H 2 S by activating DES1 in the guard cell. The accumulation of H 2 S persulfidates SnRK2.6 on Cyc131 and Cys137, which are close to the catalytic loop and near to Ser175 residues, which is vital for the phosphorylation of SnRK2.6 [133][134][135][136][137]. The Cys137 can also undergo S-nitrosylation and could inhibit the activity of SnRK2.6 [9,136]. However, persulfidation promotes SnRK2.6 activity, and it is believed that persulfidation occurs earlier than S-nitrosylation [9,137]. Due to Cyc131/137 persulfidation induced changes, Ser175 affinity for ATP-γ-phosphate proton acceptor site (Asp140) increases, which leads to the robust autophosphorylation of Ser175 and triggers efficient interaction of SnRK2.6 with its target. This observation confirms that H 2 S-mediated persulfidation positively impacts the function of SnRK2.6 in ABA-mediated stomatal closure in guard cells [9,135]. Likewise, Shen et al. [138] reported that during drought stress, ABA signaling in guard cells is promoted by H 2 S interaction with ABA. The drought stress mediates the accumulation of ABA, which stimulates persulfidation of DES1 in a redoxdependent manner. At the physiological level, enhanced accumulation of H 2 S in the guard cell leads to the persulfidation of H 2 O 2 producing enzymes, such as NADPH oxidase, which triggers the generation of H 2 O 2 in the guard cell that reinforces ABA signaling and the closure of stomata [138]. Another study revealed that abscisic acid insensitive 4 (ABI4) is involved in the facilitation of ABA and H 2 S crosstalk at the transcriptional level ( Figure 4). ABI4 is a vital TF in the ABA signaling cascade, and little was known about the PTMs that regulate its activity in response to ABA/H 2 S interaction in plants. The ABA accumulation triggers a massive generation of H 2 S that leads to the persulfidation of ABI4, which allows the binding of ABI4 to the E1 motif of the MAPKKK18 (mitogen-activated protein kinase kinase kinase 18) promoter to activate DES1 transcription to close stomata under the ABA-dependent signaling cascade [43]. This study provides compelling evidence that the DES1/H 2 S-ABI4 module acts downstream of ABA signaling to regulate stomatal closure [43,139] (Figure 4). The drought stress mediates the accumulation of ABA, which stimulates persulfidation of DES1 in a redox-dependent manner. At the physiological level, enhanced accumulation of H2S in the guard cell leads to the persulfidation of H2O2 producing enzymes, such as NADPH oxidase, which triggers the generation of H2O2 in the guard cell that reinforces ABA signaling and the closure of stomata [138]. Another study revealed that abscisic acid insensitive 4 (ABI4) is involved in the facilitation of ABA and H2S crosstalk at the transcriptional level (Figure 4). ABI4 is a vital TF in the ABA signaling cascade, and little was known about the PTMs that regulate its activity in response to ABA/H2S interaction in plants. The ABA accumulation triggers a massive generation of H2S that leads to the persulfidation of ABI4, which allows the binding of ABI4 to the E1 motif of the MAPKKK18 (mitogen-activated protein kinase kinase kinase 18) promoter to activate DES1 transcription to close stomata under the ABA-dependent signaling cascade [43]. This study provides compelling evidence that the DES1/H2S-ABI4 module acts downstream of ABA signaling to regulate stomatal closure [43,139] (Figure 4).  wave alongside strong persulfidation of SnRK2.6. The persulfidated SnRK2.6 robustly phosphorylates SALAC1 and NADPH oxidase to produce a long-lasting burst of ROS to modulate water efflux in guard cells to close stomata, similarly to the way that ABA induces stomatal closure.
In some of the recently published reports, it was also revealed that H 2 S might be involved in the biosynthesis of ABA in guard cells [140]. The H 2 S promotes the synthesis of cysteine, which is a substrate of ABA3 (molybdenum cofactor sulfurase) enzymes that regulate the activation of AAO3 (abscisic aldehyde oxidase 3) [141]. The higher accumulation of cysteine stimulates the activity of AAO (in vivo) and favors the synthesis of ABA [39] by stimulating the transcript abundance of NCED3 (9-cis-epoxycarotenoid dioxygenase 3). It was revealed that H 2 S could boost ABA synthesis, because in a cysteinebiosynthesis-depleted mutant with the disrupted ABA biosynthesis, the H 2 S was unable to induce stomatal closure [135,136]. All these studies point out the involvement/crosstalk of H 2 S with SnRK2.6, CPK6, MAPKKK18, ABI1, NADPH oxidase, Ca 2+ , and ROS in ABA-mediated signaling for stomatal movements in plants [135][136][137].

Nitric Oxide (NO) and H 2 S: Two Interacting Gaseous Molecules Essential for Plant Functioning
Nitric oxide (NO) is also a lipophilic gaseous hormone that could diffuse into interor intra cellular spaces without the need for any carrier or transport channel. NO is also involved in PTMs via tyrosine nitration, metal nitrosylation, and S-nitrosylation, whereas H 2 S mediated-PTM is associated with persulfidation. However, all these reactions led to the modification of structure, localization, and function of target proteins. Several studies have shown that H 2 S interacts with NO and other signaling molecules to modulate plant development and stress responses [7,26,32,34,142]. Earlier reports indicate that the interaction of H 2 S towards NO is complementary or inhibitory [55,[143][144][145][146]. The positive or negative interaction of these two gaseous signaling molecules may be dependent upon the dosage of exogenous H 2 S or NO application. For instance, the level of NO was reduced in plant tissues that were treated with H 2 S modulator (NaSH) [126,147]. However, crosstalk of NO-H 2 S showed synergistic interaction during abiotic stresses and inhibition of ethylene-induced fruit ripening, whereas antagonistic interaction of H 2 S-NO-ethylene is also reported [16,[148][149][150]. The discrepancy in H 2 S and NO interaction may depend upon the specific location of these gaseous molecules in the cell that deicide their signaling behavior [151]. There is also a possibility that both gaseous molecules may compete for the same targeting protein in the cell. For example, SnRK2.6 is a target of both NO and H 2 S biomolecules, and S-nitrosylation of SnRK2.6 via NO inhibits its activity while persulfidation enhances its activity and mediate stomatal movements [135,137]. Additionally, H 2 S and NO could react among themselves to produce nitrosothiol compounds that are also involved in signaling responses. The crosstalk of ROS with H 2 S-NO cascades also modulates their interactions in positive or negative ways [152]. Taken together, the nature of the interaction between NO and H 2 S may vary for different physiological functions based upon their location and concentration in the cell.
NO and H 2 S belong to the family of reactive nitrogen and sulfur species (RNS and RSS), and their positive combinations regulate various important physiological and molecular processes in plants. For example, the interaction of H 2 S with NO and Ca 2+ regulate lateral root (LR) formation in tomato plants. The exogenous application of NO triggers the accumulation of H 2 S in tomato roots due to the upregulation of H 2 S biosynthesis enzymes, which induce later root formation [6]. However, when H 2 S inhibitor/scavengers were applied, LRs' formation was partially arrested. These findings indicate that NO-induced H 2 S synthesis governs the later root formation [6,153].
Stomatal movements are regulated by many endogenous signaling molecules; among them, H 2 S and NO crosstalk are also responsible for stomatal closure. In a recent study, with the employment of pharmacological, spectrophotographic, and fluorescence microscope techniques, the coordinated action of H 2 S and NO in the presence of 2,4-epibrassinolide (EBR) was involved in stomatal regulation [154,155]. The authors demonstrated the application of EBR-induced stomatal closure in a dose and time-dependent manner via modifying the levels of NO, and H 2 S in Vicia faba. The application of EBR upregulated the activity of L-/D-cysteine desulfhydrase and enhanced the endogenous levels of H 2 S together with H 2 O 2 and NO generation in guard cells. The application of the H 2 S in-hibitor significantly reduced L-/D-cysteine desulfhydrase activity and H 2 S endogenous production, which in turn abolished the EBR mediated stomatal closure effect [154]. The H 2 S scavengers/inhibitors did not affect the NO and H 2 O 2 levels in guard cells. However, the application of NO and H 2 O 2 inhibitors/modulators significantly affected the endogenous production of H 2 S and its biosynthesis enzymes and compromised the EBRinduced stomatal closure [154]. Similarly, Jing et al. [156] found that H 2 S may function downstream of NO in ethylene-induced stomatal closure in V. faba. These results indicate that H 2 S and NO participate in EBR-mediated stomatal closure response and H 2 S signifies an essential constituent downstream of H 2 O 2 and NO in EBR-induced stomatal closure in V. faba [154,157]. Previous studies demonstrated that H 2 S inhibits ABA-mediated NO generation in Arabidopsis and Capsicum annuum guard cells. Conversely, H 2 S increased NO levels in alfalfa seedlings [55,147], while H 2 S induces NO generation in Arabidopsis guard cells. Conversely, NO scavenger inhibited H 2 S-induced stomatal closure [145]. However, investigation of H 2 S-mediated guard cell signaling in Arabidopsis revealed that the H 2 S induced signaling cascade for stomatal closure is NO-dependent [128], and both H 2 S and NO equally contribute to the production of 8-mercapto-cGMP, which triggers stomatal closure. In the same way, H 2 S and NO collaborate in ethylene induce stomatal closure responses in Arabidopsis plants, and H 2 S generation is mediated by NO, which suggests that H 2 S acts as a downstream signaling agent in ethylene induce stomatal closure [158].
The crosstalk of H 2 S and NO in the alleviation of metal toxicity is also reported, but these studies focused more on stress physiology and lacked underlying molecular mechanisms of crosstalk [159]. The exogenous application of H 2 S donor alleviated Cd stress in alfalfa plants by triggering the synthesis of NO. The interaction mechanism between H 2 S and NO improved the Cd stress tolerance by reducing Cd accumulation and lowering the lipid peroxidation in stressed plants [136]. Another study, where H 2 S and NO scavenger and inhibitor were applied to Cd stressed bermudagrass plants, revealed that depletion of NO makes them more vulnerable to metal toxicity. Furthermore, through pharmacological experiments, it was demonstrated that NO-activated H 2 S was essential for cadmium stress responses in bermudagrass [160]. In Pisum sativum, positive interaction of NO and H 2 S was also explored under arsenate stress [109]. The application of H 2 S donor triggered endogenous H 2 S and NO accumulation in P. sativum, which led to the strengthening of the antioxidant defense system, reduced arsenate accumulation, and maintained the redox balance of P. sativum plant under metal toxicity [109]. Similarly, the crosstalk of NO and H 2 S reduced oxidative stress and increased salinity tolerance in alfalfa, while barley seedlings under H 2 S application regulate ion homeostasis under salinity via maintaining the NO signaling pathway [8,146]. Most of the published studies on the interaction of NO and H 2 S in the context of metal toxicity/salinity proposed that crosstalk of these gaseous molecules ameliorates stress-induced toxicity in exposed plants via (i) improving the antioxidant defense to prevent oxidative stress, (ii) reducing the metal uptake, and (iii) by modulating the expression of associated metal transporter genes [159].
In short, H 2 S and NO are both gaseous biomolecules with common signaling pathways, and it seems that one pathway controls the functions of the other [159]. The persulfidation promoted by H 2 S reacts with thiol groups in the same way as NO does in modification through S-nitrosation [159,161]. However, there is still a need to investigate the interaction of H 2 S and NO in different plant species, tissues, and diverse environmental conditions to unveil the regulatory mechanism of the NO-H 2 S signaling cascade in plants.

H 2 S-Mediated Manipulation of Auxin Signaling in Plants
The development of roots, including lateral and adventitious roots, is incredibly important for normal plant growth and the successful completion of the life cycle. Plant root architecture is mainly based on the LR that is generated from pericycle founder cells [155]. The plant hormone auxin and environmental factors (i.e., water and nutrient availability) are key influencers in lateral root formation [162,163]. Since auxin is a master regulator of root development in plants, there have always been complex crosstalks of auxin with other signaling agents in the root development [162,164,165].
Several studies have reported that H 2 S and auxin interact with each other to regulate root growth; however, mechanistic insight remains to be elucidated [120,154,166]. The earlier studies demonstrated that the application of exogenous H 2 S on the sweet potato seedling stimulated the numbers and length of adventitious roots by modulating the IAA levels in a dose-dependent manner [154]. It was also noted that pretreatment of H 2 S donor upregulated the transcript abundance of the auxin-dependent Cyclin-Dependent Kinases gene (CDKA1) and a cell cycle regulatory gene (CYCA2) [153,165]. The activity of both of these genes was inhibited either by auxin blocker or H 2 S inhibitor, which illustrated that H 2 S mediated LR development is dependent upon the IAA signaling via influencing the regulation of CDKA1 and CYCA2 [153,165]. Similarly, when higher doses of H 2 S donor (1 mM) were applied, the RBOH1 (respiration burst oxidase homologous) transcript was significantly upregulated and ROS accumulation triggered the later root formation [115] ( Figure 5). The pharmacological studies revealed that H 2 S triggered the expression activity of RBOH1, which stimulated an H 2 O 2 -mediated increase in IAA signaling via regulation of CDKA1, CYCA2, and Kip-Related Protein 2 (KRP2), to activate LR formation [115]. A transcriptomic study revealed that exogenous application of H 2 S impacted the regulation of various auxin pathway-related genes. The accumulation of auxin biosynthesis genes (TAA1 and UGT74B1) was correlated with the increase in auxin levels in roots. The genes involved in auxin polar subcellular distribution, such as PIN2, ABCB1, ABCB19, PILS3, and PILS7, were differentially expressed, while PIN1c appeared as a hub gene on the basis of WGCNA analysis. This study provides sufficient evidence that H 2 S induced root development emanates from regulating the genes involved in transcriptional control and synthesis of auxin [166] (Figure 5).  In some studies, the application of higher dosages of H2S showed changes in root development and inhibition of auxin transport due to the alteration in the polar subcellular distribution of the PIN proteins [166]. The polar subcellular movement of auxin in root cells is an actin-dependent process, and H2S is involved in the regulation of actin dynamics due to the persulfidation and depolymerization of F actin [167]. Furthermore, during root hair development, the H2S fine-tuned polar auxin transport via persulfidation and actin filament growth [167,168]. In the root developmental process, actin-binding proteins In some studies, the application of higher dosages of H 2 S showed changes in root development and inhibition of auxin transport due to the alteration in the polar subcellular distribution of the PIN proteins [166]. The polar subcellular movement of auxin in root cells is an actin-dependent process, and H 2 S is involved in the regulation of actin dynamics due to the persulfidation and depolymerization of F actin [167]. Furthermore, during root hair development, the H 2 S fine-tuned polar auxin transport via persulfidation and actin filament growth [167,168]. In the root developmental process, actin-binding proteins work downstream of the H 2 S signal transduction pathway because actin-binding proteins are involved in the depolymerization of F-actin in root cells, which regulate the distribution and transport of auxin [168]. Auxin affects the patterning and organization of the actin cytoskeleton in root cells during cellular growth [169,170]. Conversely, the actin cytoskeleton modulates the directional transport of auxin by altering auxin efflux carriers [171,172]. This finding indicates that overproduction of H 2 S significantly increases the S-sulfhydration level of actin-2 and decreases the distribution of actin cytoskeleton in root cells, thereby reducing auxin's polar transport, which restricts the LR and the root hair growth [44,167,168].
The exposure of plants to CH 4 strongly induces H 2 S production and affects the root growth, adventitious root numbers, and root length in cucumber explants [106,173]. At the transcriptional level, it was observed that H 2 S modulated auxin-signaling genes (Aux22D-like and Aux22B-like) reinforce the CH 4 -induced cucumber adventitious rooting network [111,[173][174][175]. Similarly, in tomato plants, LRs formation was also triggered by the CH 4 -mediated H 2 S signaling cascade. It was hypothesized that the possible involvement of auxin transport and auxin signaling in CH 4 -induced LR formation is involved [176]. However, more biochemical and genetic investigations are required to analyze the detailed targets and their functions in root organogenesis under CH 4 -H 2 S-Auxin crosstalks [173,176].
The signaling pathways of H 2 S and auxin interaction under the chilling stress were recently explored in cucumber plants [177][178][179] (Figure 6). The study demonstrated that chilling stress in cucumber arrested photosynthesis and induced oxidative stress; however, deleterious effects were alleviated due to exogenous application of H 2 S donor or IAA application [179]. The expression of YUCCA2 (auxin biosynthesis gene) and auxin contents were very high in chilling-exposed cucumber seedlings. This result may be due to the inhibition of polar transport of IAA in long-term chilling stress, which increases auxin concentration in leaves and inhibits plant growth. The complex interaction of H 2 S and IAA under chilling stress improved the activities and gene expression of key enzymes of the Calvin-Benson cycle (Ribulose-1,5-bisphosphatecarboxylase, fructose bisphosphatase, sedoheptulose-1,7-bisphosphatase, fructose-1,6-bisphosphate aldolase, and transketolase) and strengthened the photosynthetic carbon assimilation capacity [179] (Figure 6). The results also indicated that auxin is a downstream signal for the protective effects induced by H 2 S under chilling-induced tolerance in cucumber plants [179]. Furthermore, the overexpression of auxin response factor 5 (ARF5) in cucumber unveiled the molecular mechanism of cold tolerance. In transgenic plants overexpressing ARF5 under cold stress, ARF5 directly activates the expression of dehydration-responsive element-binding protein 3 (DREB3) for the reinforcement of auxin signaling to improve cold stress tolerance in cucumber in response to H 2 S application [180] (Figure 6). Previously, it was observed that auxin response factors (ARFs) and miR390 formed an auxin-responsive regulatory network (miR390-TAS3-ARF2/ARF3/ARF4) that strengthens auxin signaling in plants [181].
the overexpression of auxin response factor 5 (ARF5) in cucumber unveiled the molecular mechanism of cold tolerance. In transgenic plants overexpressing ARF5 under cold stress, ARF5 directly activates the expression of dehydration-responsive element-binding protein 3 (DREB3) for the reinforcement of auxin signaling to improve cold stress tolerance in cucumber in response to H2S application [180] (Figure 6). Previously, it was observed that auxin response factors (ARFs) and miR390 formed an auxin-responsive regulatory network (miR390-TAS3-ARF2/ARF3/ARF4) that strengthens auxin signaling in plants [181].

Interaction between H 2 S and Gibberellic Acid
Gibberellic acid (GA) is a phytohormone that substantially influences the seed germination and growth of seedlings. Imbibition of barley grains in 0.25 mM NaHS solution caused an upsurge in antioxidant enzymes such as CAT, POD, APX, and SOD in the aleurone layer [182]. In tomato plants, boron stress reduced dry weight, photosynthetic rate, water content, chlorophyll content, and increased H 2 O 2 , MDA, and endogenous H 2 S. GA foliar spray reduced the harmful effects of boron by raising endogenous H 2 S, Ca 2+ , and K + , as well as lowering the levels of H 2 O 2 , MDA, and boron, as well as membrane leakage. Surprisingly, NaHS further increased GA-induced boron tolerance, whereas H 2 S scavengers prevented it (HT). These findings indicate that H 2 S plays a signaling role downstream of GA in the development of boron stress tolerance in tomato plants. During cadmium stress, the NaHS treatment stimulated the activities of amylase and antioxidant enzymes in cucumber hypocotyls and radicles, which might be connected to H 2 S-induced Cd stress tolerance.
Moreover, GA can cause programmed cell death (PCD); however, NaHS application can prevent PCD by lowering L-cysteine desulfhydrase (LCD) activity and accumulating endogenous H 2 S in wheat aleurone layers [49]. GA-induced PCD is reduced in the aleurone layer in the NaHS-treated seeds by diminishing the endogenous GSH levels. H 2 S concentration regulates the GSH levels, which upsurges expression of the HEME OXYGENASE-1 (HO-1) gene, resulting in the alleviation of apoptosis in the aleurone layer and an overall decrease in PCD. Hence, in the aleurone layer, there are regulatory interactions between GA, H 2 S, GSH, and HO-1. Intriguingly, NaHS pretreatment slowed Arabidopsis seed germination, but Arabidopsis des1 mutant seedlings were more susceptible to ABA than the wild-type. These findings suggest that H 2 S interacts with GA in plants to control seed germination under normal and stressful circumstances.

Interaction between H 2 S and Melatonin
Melatonin (N-acetyl-5-methoxytryptamine) is a multifaceted phytohormone involved in germination, ripening, flowering, photosynthesis, and defense mechanisms [183]. In plants, melatonin alters the permeability of the cell layer governed by ion transporters, which control stomatal opening and closure. Studies have shown that melatonin can increase the photosynthetic capacity of plants, which leads to greater levels of nitrogen and chlorophyll. In tomato and wheat, increased transcription of stress-responsive genes was induced by melatonin, resulting in better tolerance to high temperature [184,185]. Furthermore, melatonin cross-talks with various plant hormones and signaling molecules. It was also discovered that H 2 S and melatonin conjointly helped alleviate salt stress-induced growth reduction in tomatoes, and exogenous melatonin treatment assisted in regulating early H 2 S signaling [186]. In wheat, the heat stress-induced oxidative damage was mitigated by exogenous melatonin and further increased the H 2 S production, suggesting that melatonin-mediated H 2 S was involved in alleviating the oxidative stress. However, the melatonin function was attenuated when H 2 S was inhibited by its inhibitor, indicating that the cross-talk between H 2 S and melatonin, and possibly melatonin, regulates heat stress signaling by acting upstream of H 2 S [187].

H 2 S-Plant Hormone Cross-Talk under Pathogen Attack
In plants, the dual roles of H 2 S in interactions with phytohormones determine the biological roles of H 2 S in plant growth, development, and responses to biotic stresses. In response to biotic stresses, the crosstalk between H 2 S and phytohormones, as well as several other signaling molecules, has been studied less; however, some critical molecular insights have been found in the recent past. In the following paragraph we discuss the H 2 S-phytohormone interplay under biotic stress.

Interaction between H 2 S and Salicylic Acid
Salicylic acid (SA) is a phytohormone that triggers a defense response in plants against biotrophic and hemibiotrophic phytopathogens. SA activates a large number of defenserelated genes, especially those that encode pathogenesis-related (PR) proteins [188,189]. Susceptibility to virulent and avirulent pathogens develops as a result of mutations that impede SA production. In Nicotiana tabacum cv. Xanthi-nc, acetyl SA (aspirin) confers resistance to tobacco mosaic virus [190]. Previously, it was found that the expression of multiple WRKY transcription factors (TFs) is modulated by pathogen attack or SA treatment [191]. A subsequent study has shown that the mutation in WRKY18, WRKY40, and WRKY60 resulted in the up-regulation of LCD, DES, DCD1, and higher production of H 2 S in Arabidopsis [192]. In Arabidopsis, the expression level of a PR gene-regulating transcription factor WRKY54 was elevated in des1 mutants and decreased in oas-a1 mutants [193]. Furthermore, des1 mutants had lower levels of L-glutathione oxidation than oas-a1 mutants, and lesser intracellular redox potential was caused by higher L-Cys levels in des1 mutants, which may help boost plant resistance to pathogen invasion [193]. Later, Alvarez et al. [194] demonstrated that Arabidopsis des1 mutants have increased amounts of SA and developed more resilience against Pseudomonas syringae pv. tomato (Pst) DC3000 avrRpm1, while oas-a1 mutants were more vulnerable to this pathogen [194]. The des1 mutants exhibited all the constitutive systemic acquired resistance characteristics, including high resistance against biotrophic and necrotrophic pathogens, accumulation of salicylic acid, and induction of WRKY54 and PR1 [194]. In contrast to the oas-a1 mutants, Arabidopsis cad2-1 mutants showed lower levels of L-glutathione but a non-significant change in the L-Cys levels. In cad2-1 mutants, repression of WRKY54 was also not observed, which suggests that lower expression of PR genes in oas-a1 mutants might be due to reduced L-Cys level [192]. In order to determine if L-Cys is involved in plant immunity, researchers exposed oas-a1 mutants to the bacterial pathogen Pst DC3000, which releases effectors that suppress PAMP-triggered immunity (PTI). The Arabidopsis oas-a1 mutant plants were shown to be more susceptible to infection by this pathogen [195]. Thus, the results from the previously mentioned studies suggest that higher L-Cys decreases cytoplasmic redox potential, which may play a key role in pathogen defense in Arabidopsis and other plant species. Still, more research is needed in Arabidopsis and other plant species.
Among SA-biosynthesis genes in Arabidopsis, the phytoalexin deficient (PAD) genes (PAD1, PAD2, PAD3, and PAD4) encode regulatory proteins that function against the eukaryotic biotroph Peronospora parasitica and promote resistance to downy mildew [196]. Increased sensitivity to the bacterial pathogen Pst DC3000 has been observed in the pad1, pad2, and pad4 mutants [196]. Enhanced disease susceptibility1 (EDS1) gene codes for a lipases-like protein that acts in resistance (R) gene-dependent effector-triggered immunity and contributes to basal defense in plants. EDS1 is also required for pathogen-induced PAD4 mRNA accumulation [197]. The PAD4 and EDS1 genes involved in SA biosynthesis were found to be constitutively activated in Arabidopsis plants with high H 2 S concentrations but found to be reduced in plants with low H 2 S levels ( Figure 7) [58]. NPR1 plays an essential function in SA signaling because it binds SA and initiates a SAR response [198][199][200]. Other similar molecules such as methyl salicylate (MeSA) or gentisic acid promote PR1 expression in addition to SA [201]. The deposition of SA is required for triggering the expression of SA-mediated genes, such as PRs [189]. Plants with greater H 2 S levels showed increased expression of SA-mediated PR genes, which improved pathogen resistance, and vice versa (Figure 7). Similarly, effectors also induce the biosynthesis of L-Cys. The plant cytosol contains the enzyme L-cysteine desulfhydrase (DES1), which is responsible for L-Cys decomposition and endogenous H2S production. The higher concentration of H2S triggers the upregulation of SA biosynthesis-related genes (PAD4/EDS1). The enzyme ICS1 catalyzes the conversion of chorismite into isochorismate, which is then exported to the cytosol by EDS5. The Lglutamate is converted into isochorismate-9-glutamate in the cytosol by PBS3. Subsequently, SA is produced from isochorismate-9-glutamate through spontaneous decay. By acting as an isochorismate A pyruvoyl-glutamate lyase (IPGL), EPS1 also degrades N-pyruvoyl-L-glutamate to create SA. The NPR1 gene expression is aided by SA due to the interaction of WRKY transcription factors with NPR1, which promotes the recruitment of CDK8 to the NPR1 promoter's W-box. Pathogen-induced defense signals enhance the accumulation of salicylic acid (SA) in plants by enhancing the expression of Isochorismate Synthase (ICS) genes. In addition, SA promotes redox reactions that lead to the reduction of NPR1 oligomers to monomers. The monomeric NPR1 molecules move from the cytosol to the nucleus, where they form a protein complex with transcription factor (TGA), EDS1, SA, and

Interaction between H 2 S and Jasmonic Acid
Jasmonic acid (JA) is a lipid-derived signaling molecule that plays a significant role in many biological processes in plant cells. Herbivorous insects chewing on the leaves or necrotrophic diseases trigger the JA response pathway. Plants have evolved to remember these attacks and employ this pre-conditioned situation effectively and to their benefit in a mechanism termed induced systemic resistance (ISR). Interestingly, the biological pathways of JA and SA have been reported to function antagonistically [202]. JA and SA enhance plant defense against nematodes such as M. incognita [203]. This pathogen causes plants to trigger SA pathways and prevent JA in leaves to permit successful invasion of the pathogen. Furthermore, JA showed a higher concentration in roots following the nematodic infection that is subsequently transferred to leaves, helping plants to defend themselves against pathogens [204]. In another study, when Arabidopsis was deprived of the sulfur element, it led to activation of the JA and SA metabolism; but the plant showed susceptibility to necrotrophic Botrytis cinerea [205]. This discovery suggests that the presence of sulfurcontaining compound H 2 S is essential for plant defense mechanisms through its interaction with SA and JA.
H 2 S interacts with JA to promote pathogen resistance in plants (Figure 7). The redox state of ascorbate is shown to be regulated in the leaves of A. thaliana by the interaction between H 2 S and mitogen-activated protein kinase (MEK1/2) (Figure 7) [206]. In Arabidopsis, the exogenous application of JA resulted in a significant increase in endogenous H 2 S generation, MEK1/2 phosphorylation, and a lower ascorbate to dehydroascorbate ratio (AsA/DHA) [195]. The increase in the phosphorylation level of MEK1/2, endogenous H 2 S generation, and the AsA/DHA ratio in wild-type hosts was shown to be caused by hypotaurine (HT), an H 2 S scavenger, resulting in a decrease in JA. The application of sodium hydrosulfide, which acts as an H 2 S donor in mutant A. thaliana plants, was observed to enhance these indicators. When these mutant plants were given an application of NaHS after being treated with HT and JA, the effects of hypotaurine on those JA-induced indicators were not reversed.

Interaction between H 2 S and Ethylene
Phytohormones play a critical role in the defense mechanism in plants against various pathogens. SA often controls biotrophic and hemibiotrophic pathogen defense responses, but ethylene and JA promote defense responses to necrotrophic pathogens. However, sometimes hormone signal transduction pathways that conferred resistance and vulnerability were found to be diametrically opposed. Plant resistance was shown to be associated with an increase in SA signaling, whereas susceptibility was found to be associated with an increase in the ethylene pathway and a decrease in SA and cytokinin signaling. According to Foucher et al. [207], two Phaseolus vulgaris L. genotypes (resistant and susceptible) were screened against common bacterial blight caused by Xanthomonas phaseoli pv. phaseoli. The transcriptomic study revealed that resistance was associated with an increase in the SA pathway and a decrease in photosynthetic activity as well as sugar metabolism. Susceptibility was associated with an increase in the ethylene pathway and genes that modify cell walls, as well as a decrease in the downregulation of resistance genes [207].
Pathogenic bacteria cannot form merism when exposed to exogenous NaHS, which helps plants recover from infection [208]. Fumigation with H 2 S has been shown to suppress spore germination, mycelial growth, and pathogenicity of Monilinia fructicola in peach fruit, as well as Aspergillus niger and Penicillium expansum in pear [209]. These findings show that H 2 S can promote a plant's resistance to pathogen infection, and that immunological signals and exogenous sulfide can both trigger the production of endogenous H 2 S. Exogenous H 2 S reversed the impacts of ETH by reducing the activity of enzymes involved in cell wall modification (cellulase and polygalacturonase) via transcription suppression rather than direct post-translational modification (sulfhydration) by H 2 S [210]. H 2 S also controlled the expression of SlIAA3, SlIAA4, ILR-L3, and ILR-L4 (all of which are involved in auxin signaling), which suppressed petiole abscission by controlling the amount of free auxin in tomato abscission zone cells. In rose and lily plants, similar findings were observed in floral organ abscission and anther dehiscence [210]. These findings suggest that H 2 S interacts with ethylene and auxin during plant organ abscission.
Exogenous ethylene donor (ethephon) stimulated the activities of LCD and DCD in Arabidopsis and Vicia faba plants, resulting in H 2 S production in guard cells and stomatal closure, whereas H 2 S-synthesis inhibitors (PAG) reversed ethylene-induced stomatal closure, indicating H 2 S-mediated ethylene-induced stomatal closure [211]. Furthermore, early leaf senescence was seen in Arabidopsis des1 mutants (due to reduced endogenous H 2 S content), whereas NaHS treatment reversed the senescence and extended the vase life of cut flowers by elevating endogenous H 2 S levels. In addition, by reducing ethylene synthesis, H 2 S-delayed senescence was seen in green leafy crops [212]. These findings demonstrate that ethylene promotes stomatal closure and organ senescence in plants by independently increasing and suppressing endogenous H 2 S generation.

Conclusions and Future Prospects
For a long time, H 2 S was considered an undesirable by-product of sulfur metabolism, which could adversely affect plant cells. However, this perception was altered after it was discovered that H 2 S could have signaling properties. H 2 S is involved in many plant processes and can interact with other phytohormones to mitigate stress in plants. However, most research is focused on the H 2 S interaction with phytohormones under abiotic stress.
In contrast, there is very limited research progress on the interaction of H 2 S with SA, JA, and especially, ethylene in plants under biotic stresses. The exogenous ethylene donor (ethephon) stimulated the activities of LCD and DCD in Arabidopsis and V. faba plants, resulting in H 2 S production in guard cells and stomatal closure, whereas H 2 S-synthesis inhibitors (PAG) reversed ethylene-induced stomatal closure, indicating H 2 S mediates ethylene-induced stomatal closure [211]. Since ethylene promotes stomatal closure, it might prevent the invasion of pathogens. Therefore, it is likely the crosstalk between H 2 S and ethylene plays a pivotal role in the regulation of stomatal closure during plant defense against pathogen invasion, which warrants further investigation.
In plants, the H 2 S-mediated persulfation can significantly impact protein function, altering protein conformation and regulating protein activity under stress response. According to Chen et al. [135], H 2 S positively regulates abscisic acid signaling by sulfidating SnRK2.6 in guard cells. H 2 S has also been reported to persulfidate MAPK in Arabidopsis to alleviate cold stress [213]. Numerous studies have been conducted to understand H 2 Smediated persulfation of proteins in plants under abiotic stress; however, H 2 S-mediated persulfation is not studied sufficiently in plant-pathogen interaction. H 2 S can also be involved in protein functions through trans-persulfidation and regulating cellular redox state in other unexplored H 2 S-related molecules in the plant metabolism such as glutathione persulfide (GSSH) and cysteine persulfide (CysSSH).
In future studies, more fundamental research is required to investigate the fate and regulation of endogenous H 2 S production, and its subsequent interaction with and regulation of different plant processes under laboratory as well as in field conditions. However, the exogenous application of H 2 S on plants in controlled conditions has generated plenty of experimental results that have explained at least some of the underlying mechanisms of actions driven by H 2 S molecules in plants. In the animal field, several exogenous sources of H 2 S have been utilized that can slowly release H 2 S in media (mimicking the natural generation of H 2 S). However, for plants, NaHS and inorganic sodium polysulfides (Na 2 S n ) such as Na 2 S 2 , Na 2 S 3 , and Na 2 S 4 are currently used in various research reports to study the H 2 S impacts in plants. The NaHS and related H 2 S generation compounds are usually short-lived donors and do not mimic the slow release of H 2 S in in-vivo conditions. Recently, dialkyldithiophosphate demonstrated the potential to release H 2 S slowly and enhance the maize plant biomass upon application [214]. In addition, more precise and advanced methods of H 2 S application to the plants under various growth stages and environmental stresses, and H 2 S suitable dosages for different crop species are also required.