Highlights in gibberellin research: A tale of the dwarf and the slender

Abstract It has been almost a century since biologically active gibberellin (GA) was isolated. Here, we give a historical overview of the early efforts in establishing the GA biosynthesis and catabolism pathway, characterizing the enzymes for GA metabolism, and elucidating their corresponding genes. We then highlight more recent studies that have identified the GA receptors and early GA signaling components (DELLA repressors and F-box activators), determined the molecular mechanism of DELLA-mediated transcription reprograming, and revealed how DELLAs integrate multiple signaling pathways to regulate plant vegetative and reproductive development in response to internal and external cues. Finally, we discuss the GA transporters and their roles in GA-mediated plant development.


Introduction
The gibberellins (GAs) were named for the phytopathogenic fungus Gibberella fujikuroi, whose secretions caused abnormal growth and sterility in infected rice (Oryza sativa) plants (Kurosawa 1926).The biologically active factor was isolated in impure form from fungal cultures in the 1930s in Japan and named gibberellin A (Yabuta and Sumiki 1938), but this research was not widely known outside of Japan until the late 1940s.The main active component was identified in the 1950s in the UK, USA, and Japan, where it was named gibberellic acid, gibberellin-X, and gibberellin A 3 (GA 3 ), respectively (Curtis and Cross 1954;Stodola et al. 1955;Takahashi et al. 1955).The structure of gibberellic acid, the name agreed upon by the UK and US groups, or GA 3 , was proposed in the late 1950s by chemists working at the ICI Ackers Laboratory, Welwyn, UK (reviewed by Grove 1961).The remarkable effect of this substance on plants stimulated interest in fungal gibberellins (GAs).GAs promote plant growth, particularly to rescue the growth of dwarf mutants of pea (Pisum sativum) and maize (Zea mays) (Brian et al. 1954;Phinney 1956) and to induce bolting in long-day (LD) rosette species (Lang 1956;Wittwer et al. 1957), prompting the suggestion that they may be endogenous plant hormones (Stowe and Yamaki 1957).Plant extracts promoted the growth of mutants in a similar manner to GA 3, reinforcing this hypothesis, which was confirmed by the isolation of 2 mg of GA 1 from 87.3 kg of immature seeds of runner bean (Phaseolus coccineus) (Macmillan and Suter 1958).The identity of the isolated bioactive compound was determined by comparing its infra-red spectrum with that of authentic GA 1 from G. fujikuroi.Thus, GA was established as the second endogenous growth regulator (plant hormone) after auxin.The role of GA in plant growth regulation is illustrated in Fig. 1, which compares wild-type and mutant wheat (Triticum aestivum) plants with compromised GA-biosynthesis (GA-responsive) or signaling (GA-unresponsive) without or with treatment with GA 3 .While GA 3 was the first GA to be discovered, it is a minor form in plants, whereas the major bioactive forms are GA 1 or GA 4 (see Fig. 2).GA 3 differs from GA 1 by the presence of a double bond that prevents inactivation by 2β-hydroxylation.
The identification of GA 1 and other GAs in bean seeds was followed by the isolation of other GAs from many plant species.Their structures were determined by conversion to compounds of known structure and/or nuclear magnetic resonance spectroscopy profiles.Later, the development of combined gas chromatography-mass spectrometry for GA analysis allowed them to be identified in plant tissues without the need to obtain pure compounds (Binks et al. 1969).This technique, and later liquid chromatographymass spectrometry (LC-MS), has enabled GA identification and quantitation to become routine and not just the purview of chemists.The high sensitivity and resolution of ultra high performance LC-MS-MS now allow GAs to be measured in low (mg) amounts of plant tissues.
Following their discovery, there was initially steady but slow progress in elucidating the biosynthetic pathways for GAs in G. fujikuroi (the rice pathogen is now reclassified as Fusarium fujikuroi) and in plants.In addition, although there was considerable information on the physiological action of GAs on plants, advances in understanding their molecular modes of action were sluggish.By contrast, the application of GAs in agriculture and horticulture developed rapidly with their availability from fungal cultures, with major uses in the production of seedless grapes, to improve skin finish in apples, and many other applications (Rademacher 2015).Furthermore, inhibitors of GA biosynthesis found important applications as plant growth retardants (Rademacher 2000), while semidwarf varieties of major crop species that were key contributors to the Green Revolution were later shown to be defective in GA biosynthesis or action (Phillips 2016).In the last 30 years, with the use of mutants and developments in molecular genetics and genomics, progress in our understanding of both GA metabolism and signaling has accelerated, with details emerging on the biosynthetic reactions, enzymes, genes, and their regulation as well as GA perception and signal transduction.The movement of GAs between cells or over longer distances between organs

ADVANCES
• The use of biosensors, gene reporters, single-cell RNA-sequencing, and tissue-specific manipulation of GA metabolism is revealing the cellular distribution of GA biosynthesis and accumulation, and its relevance in plant development.
• The GA signaling repressors DELLAs function as master growth regulators by interacting with regulators in many cellular pathways in response to internal and external cues.
• The movement of GA precursors provides an additional layer of regulation for bioactive GA contents at responding tissues, which is particularly crucial for long-distance communication in coordinating plant growth and development.
is an important factor in their function, and recent progress in understanding their transport and transporters is a major development.This review highlights the advances that have contributed to our current understanding of GA metabolism, signaling, and transport and their role in plant development.

Establishing the GA-biosynthetic pathways
The diterpenoid nature of GAs was demonstrated in the fungus F. fujikuroi by the incorporation of 14 C-labeled mevalonic acid (MVA) into GA 3 (Birch et al. 1958).Subsequently, the GA-biosynthetic and catabolic pathways were established in plants, primarily using cell-free systems from developing seeds (Graebe et al. 1965;Dennis and West 1967;Graebe et al. 1972Graebe et al. , 1974a, b;, b;Kamiya and Graebe 1983) and in the fungus using liquid cultures (Cross et al. 1964;Bearder et al. 1975;Evans and Hanson 1975).The GA metabolism pathway in plants is summarized in Fig. 2, and details can be found in a recent review (Hedden 2020).The diterpene precursor trans-geranylgeranyl diphosphate (GGPP), which is formed from MVA in the fungus and mainly via the methylerythritol phosphate (MEP) pathway in plants, is converted in two steps to the tetracyclic diterpene ent-kaurene via ent-copalyl diphosphate (CPP).ent-Kaurene is oxidized to ent-kaurenoic acid and then to GA 12 via several intermediates by two multifunctional cytochrome P450 (CYP450) monooxygenases, ent-kaurene oxidase (KO) and ent-kaurenoic acid oxidase (KAO), respectively.A third CYP450 converts GA 12 to GA 53 by hydroxylation on C-13.These C 20 intermediates are converted in parallel pathways by soluble dioxygenases to the C 19 -GAs GA 9 and GA 20 , respectively, and then to the bioactive phytohormones GA 4 and GA 1 .The loss of a C atom (C-20) in the formation of C 19 -GAs occurs from an aldehyde intermediate (Kamiya and Graebe 1983).In contrast to plants, in which 13-hydroxylation (in GA 53 formation) occurs early in the pathway and 3β-hydroxylation is the final step, in F. fujikuroi, 3β-hydroxylation occurs earlier, while 13-hydroxylation is the last step in the formation of GA 3 (Bearder et al. 1975;Evans and Hanson 1975).Further metabolism of inactive products is critical to the regulation of GA concentration.The most important inactivation process is 2-oxidation, which can occur on the bioactive GAs and their immediate C 19 precursors, as well as on earlier C 20 intermediates.Oxidation of C 19 -GAs to 2β-hydroxy products is especially strong in late-developing legume seeds, including pea seeds, in which further oxidation on C-2 to GA-catabolites was noted (Sponsel 1983).

GA-biosynthesis mutants
GA-responsive dwarf mutants with lesions in the GAbiosynthetic pathway (Fig. 1) proved extremely useful in understanding GA physiology, identifying the underlying enzymes, and isolating the corresponding genes.Collections of single gene mutants of maize and peas were assembled by Phinney at University of California, Los Angeles (UCLA) and Murfet at Hobart, Tasmania, respectively, and the application of precursors revealed the positions of the lesions in the pathway.Such experiments established that GA 1 , but not its biosynthetic precursors, had biological activity in maize (Phinney and Spray 1982) and that DWARF-1 in maize and LE in pea encode 3β-hydroxylases that convert GA 20 to GA 1 (Ingram et al. 1984;Spray et al. 1984).The le mutation corresponded to one of the traits, the difference in stem length, used in Mendel's classical experiments.Once the gene was identified, the mutation was shown to cause an amino acid substitution close to the Fe binding site that reduced enzyme activity (Lester et al. 1997;Martin et al. 1997).The dwarf-5 mutation alters the activity of ent-kaurene synthase (KS) to produce mainly ent-isokaurene, as shown in a cell-free system from maize seedlings (Hedden and Phinney 1979).The slender (sln) pea mutant illustrates the importance of GA inactivation in regulating GA concentration.The mutation is associated with excessive seedling growth, which decreases later in development (Reid et al. 1992;Ross et al. 1995).The gene, which encodes a GA 2-oxidase, is highly expressed in developing seeds, particularly in the testae (Lester et al. 1999;Martin et al. 1999).Mature pea seeds contain high levels of inactivation products oxidized on C-2 (Sponsel 1983), but sln seeds accumulate the precursor GA 20 , which upon germination is converted to GA 1 , causing the overgrowth symptoms (Reid et al. 1992).
In addition, Koornneef and van der Veen (1980) produced 56 independent GA-sensitive Arabidopsis (Arabidopsis thaliana) mutants, representing 5 loci, through irradiation-or EMS-induced mutagenesis.Mutations at three loci, named ga1, ga2, and ga3, prevented germination and caused severe dwarfism.By contrast, the other 2 mutations, ga4 and ga5, allowed germination without GA treatment and produced only mild dwarfism.It was later shown that GA1, GA2, and GA3, which encode CPP synthase (CPS), KS, and KO, respectively, are single-copy genes, while the mild phenotypes of ga4 and ga5, with impaired GA 3-oxidation and GA 20-oxidation, respectively, are due to gene redundancy (see below).

Characterizing the enzymes of GA metabolism
Work in Charles West's laboratory at UCLA with cell-free preparations from Marah macrocarpus endosperm and F. fujikuroi mycelia led to the characterization of the enzymes involved in the conversion of GGPP to ent-kaurene.Using the F. fujikuroi system, Shechter and West (1969) showed that the conversion occurred in two steps, with CPP as an intermediate.The 2 activities, named activity A for conversion of GGPP to CPP and activity B for conversion of CPP to ent-kaurene, were found (after purification) to be present in a single polypeptide (Fall and West 1971).However, they are separate enzymes in M. macrocarpus but probably function in association (Duncan and West 1981).Activity A was renamed as the type II terpene cyclase CPS, while activity B, a type I cyclase, was renamed KS (MacMillan 1997).Early indications that these activities were present in plastids (Simcox et al. 1975) were later confirmed (Aach et al. 1995) and further substantiated by the presence of plastidtargeting leader sequences in CPS and KS (Sun and Kamiya 1994;Yamaguchi et al. 1996) and by the plastid localization of enzyme fusions with green fluorescent protein (GFP) (Helliwell et al. 2001b).
The enzyme activities responsible for the middle section of GA biosynthesis, from ent-kaurene to GA 12 and GA 53 in plants and to GA 14 (3β-hydroxy GA 12 ) in F. fujikuroi, were present in microsomes from cell-free systems from M. macrocarpus, pumpkin (Cucurbita maxima) endosperm, developing pea cotyledons, and the fungal mycelia and required NADPH (West 1973;Hasson and West 1976;Ropers et al. 1978;Graebe et al. 1980).These enzymes have the properties of CYP450s, which was confirmed when cDNAs encoding the enzymes were isolated (see below).By contrast, the final reactions in the pathway are catalyzed by soluble oxidases requiring Fe 2+ and are therefore different from the monooxygenases responsible for earlier steps.The pumpkin enzymes were shown to require a small molecule whose identification as 2-oxoglutarate established the enzymes catalyzing GA 12 -aldehyde 7-oxidation, GA 20-oxidation, 3β-hydroxylation, and 2β-hydroxylation as 2-oxoglutarate-dependent dioxygenases (2-ODDs) (Hedden and Graebe 1982).The soluble 7-oxidase has restricted distribution between plant families, with most plants employing only a monooxygenase for this reaction, while in pumpkin endosperm, this reaction is catalyzed by both monooxygenase and dioxygenase enzymes.
Although work with cell-free homogenates demonstrated the efficient conversion of MVA into GAs, the application of 13 C-labeled substrates to Arabidopsis seedlings indicated that ent-kaurene and GA 12 were synthesized mainly from the MEP pathway with a small contribution from the MVA pathway (Kasahara et al. 2002).The extent of cross-over between these pathways, which is dependent on the movement of isoprenoid intermediates into and out of the plastid, may vary among tissues and developmental stages.

Identification of genes encoding GA-metabolic enzymes
The isolation of transcripts and genes encoding the GA-biosynthetic enzymes were major developments that advanced our understanding of the regulation of GA metabolism.Sun et al. (1992) took advantage of the large deletion in the ga1-3 Arabidopsis mutant to isolate the GA1 gene by genomic subtraction.Expression of its cDNA in Escherichia coli demonstrated that it encodes CPS (Sun and Kamiya 1994).The maize gene ANTHER EAR1 (AN1), which also encodes CPS, was isolated by tagging with the Mutator transposon shortly thereafter (Bensen et al. 1995).After purifying a GA 20-oxidase from pumpkin endosperm and partial amino acid sequencing (Lange 1994), the use of antibodies raised against synthetic peptides led to the isolation of its cDNA from an expression library (Lange et al. 1994).Expression in E. coli confirmed its enzymatic activity as oxidizing C-20 mainly to the carboxylic acid.Based on the nucleotide sequence of the pumpkin transcript, three GA20ox cDNAs were isolated from Arabidopsis and shown (by expression in E. coli) to encode enzymes that convert GA 12 to the C 19 -GA, GA 9 (Phillips et al. 1995).The tissue-specific expression patterns of the genes differed, but these genes showed partial redundancy, explaining the mild phenotype of the ga5 mutant (Rieu et al. 2008b).Their expression was downregulated by GA, confirming feedback regulation, which had been proposed earlier (Hedden and Croker 1992).A similar approach was used to clone one of these genes, AtGA20ox1, which corresponds to GA5 (Xu et al. 1995).Arabidopsis contains five GA20ox genes, but only three of these, AtGA20ox1,2, and 3, play major roles in plant development (Plackett et al. 2012).
The cloning of other GA-biosynthetic genes quickly followed.The Arabidopsis GA4 gene was cloned by T-DNA tagging (Chiang et al. 1995) and confirmed (by heterologous expression) to encode a GA3ox (Williams et al. 1998).Of the four Arabidopsis GA3ox genes, two genes, AtGA3ox1 and AtGA3ox2, regulate vegetative growth (Mitchum et al. 2006).Like AtGA20ox1,2, and 3, AtGA3ox1 is down-regulated by GA signaling as part of GA homeostasis (Cowling et al. 1998).KS was cloned from pumpkin following the purification of KS protein from cotyledons (Yamaguchi et al. 1996).This led to the isolation of KS cDNA from Arabidopsis and the finding (by mutant complementation) that it corresponded to GA2 (Yamaguchi et al. 1998).Helliwell et al. (1998) demonstrated that GA3 encodes KO based on the accumulation of ent-kaurene in the ga3-1 mutant and its inability to respond to ent-kaurene application.The authors used map-based cloning and random sequencing to isolate GA3, which encodes a CYP450, and confirmed its identity by mutant complementation and by demonstrating KO activity after expression in yeast.KAO was cloned from barley (Hordeum vulgare) in which it corresponds to GA-RESPONSIVE DWARF5 (GRD5), whose mutants accumulate ent-kaurenoic acid (Helliwell et al. 2001a).GRD5 and 2 Arabidopsis homologs encode CYP88A family members, which, after expression in yeast, were shown to catalyze the 3-step conversion of ent-kaurenoic acid to GA 12 via ent-7α-hydroxykaurenoic acid and GA 12 -aldehyde (Helliwell et al. 2001a).The equivalent enzyme in F. fujikuroi (CYP68A) also has 3β-hydroxylase activity and produces GA 14 (Rojas et al. 2001).The two AtKAO genes share fully redundant functions, with the double mutant being severely dwarfed (Regnault et al. 2014).Thus, two enzymes, KO and KAO, are required to convert ent-kaurene to GA 12 in plants, with a third CYP enzyme catalyzes the 13-hydroxylation of GA 12 to GA 53 (see below).Fusions of AtKO and AtKAO with GFP localized to the outer chloroplast envelope and endoplasmic reticulum (ER), respectively, provide a mechanism for the transit of ent-kaurene from plastids to the ER (Helliwell et al. 2001b).
The first cloning of a GA2ox cDNA took advantage of the very high GA2ox activity in late-developing P. coccineus seeds by functional screening of a cDNA expression library for release of 3 H from [2β, 3β-3 H 2 ]GA 9 (Thomas et al. 1999).The functions of the P. coccineus cDNA and three homologous Arabidopsis cDNAs identified in genomic databases were determined by expression in E. coli.The enzymes converted C 19 -GAs to their 2β-hydroxy analogs and, depending on the substrate and paralog, catalyzed further oxidation to GA-catabolites.GA promoted the expression of two of the Arabidopsis GA2ox genes, whereas it had the opposite effect on GA20ox and GA3ox gene expression.Like GA20ox and GA3ox, the C 19 -GA2oxs form a gene family with five functional members in Arabidopsis (Rieu et al. 2008a).Soon after, similar approaches were used to clone GA2ox cDNAs from developing pea seeds, one of which, PsGA2ox1, corresponds to SLN (Lester et al. 1999;Martin et al. 1999).A second clade of GA2ox genes with 2 members was identified from Arabidopsis by activation tagging, encoding enzymes that act on C 20 -GAs (Schomburg et al. 2003).Two additional members of this clade were identified in Arabidopsis recently (Lange et al. 2020).Apart from the GA7ox genes with restricted distribution, angiosperms contain four families of 2-ODDs, GA20ox, GA3ox, C 19 -GA2ox, and C 20 -GA2ox, while this last clade is absent from gymnosperms (Yoshida et al. 2020).The C 19 -GA2ox gene family is the largest in most species, with some tissue-specific expression but considerable redundancy.
GA 13-hydroxylase genes were first identified in rice.The encoded monooxygenases CYP714B1 and CYP714B2 converted GA 12 to GA 53 following expression in yeast (Magome et al. 2013).Overexpression of these genes in Arabidopsis caused a slight reduction in height, suggesting that 13-hydroxylation is a mild inactivation reaction.Other members of the CYP714 family oxidize 13-deoxy GAs and/or ent-kaurenoic acid on C-13 or adjacent C atoms and are also inactivating.Mutation of the rice enzyme CYP714D1, known as ELONGATED UPPERMOST INTERNODE (EUI), which oxidizes the 16,17-double bond to the epoxide, is utilized in hybrid rice production to promote panicle emergence in male-sterile cultivars (Zhu et al. 2006).Arabidopsis, which produces low amounts of 13-hydroxy GAs, except in the seed, contains two CYP714 genes, CYP714A1 and CYP714A2.Overexpression of CYP714A1, which converts GA 12 to 16α-carboxy-17-norGA 12 , causes extreme dwarfism, while CYP714A2 functions mainly as a 12α-hydroxylase, with only low 13-hydroxylase activity, and causes mild dwarfism when overexpressed (Nomura et al. 2013).Notably, AtCYP72A9 was found to 13-hydroxylate GA 12 , GA 9, and GA 4 (following expression in yeast) and may be the main source of 13-hydroxy GAs in Arabidopsis seeds (He et al. 2019).Its overexpression resulted in dwarfism.

Regulation of GA metabolism
GA biosynthesis and inactivation are tightly regulated by developmental and environmental cues (Yamaguchi and Kamiya 2000;Sun 2008;Yamaguchi 2008;Hedden and Thomas 2012;Hedden 2020;Bouré and Arnaud 2023).Following the identification of genes encoding the metabolic enzymes, there have been numerous reports of their transcriptional regulation, particularly for the 2-ODDs, which limit the production of bioactive GAs.As discussed under GA perception and signaling, their expression is modified by other hormones as well as by numerous environmental factors, including stress (Fig. 3).While there is some evidence for post-transcriptional regulation (Lee and Zeevaart 2007), this process has been little studied for practical reasons.Reports of altered GA levels in GA-response mutants were early indications that GA-metabolism was regulated via GA signaling (reviewed in Hedden and Sponsel 2015).These observations highlighted 20-oxidation as a potential site of regulation by GA action, which was confirmed by experiment (Hedden and Croker 1992).Subsequently, as noted above, expression of some GA20ox and GA3ox genes was found to be repressed by GA, while GA2ox expression was upregulated (Thomas et al. 1999).Furthermore, down-regulation of GA INSENSITIVE DWARF1 (GID1) receptor genes by GA extended homeostasis to GA signaling (Griffiths et al. 2006).The involvement of the DELLA GA-signaling component in this process is discussed below.A nontranscriptional homeostatic mechanism was revealed from the X-ray crystal structure of OsGA2ox3 (Takehara et al. 2020).In the presence of its substrate GA 4 , the enzyme forms a tetramer, thereby increasing its catalytic efficiency.

GA biosynthesis in nonseed plants, fungi, and bacteria
In the evolution of land plants, DELLA-mediated signaling predates its regulation by GA-GID1 (Hernandez-Garcia et al. 2021).The evolution of GA biosynthesis was discussed in detail recently (Yoshida et al. 2020).The bryophyte Physcomitrium patens produces ent-kaurenoic acid derivatives but not GAs (Miyazaki et al. 2018), whereas the lycophyte Selaginella moellendorffii and the fern Lycodium japonicum produce GA 4 using 2-ODDs for 20ox and 3ox activities and possess the GA-GID1-DELLA signaling system (Hernandez-Garcia et al. 2019;Yoshida et al. 2020).Notably, while P. patens and L. japonicum have bifunctional CPS/KS enzymes, S. moellendorffi has separate CPS and KS enzymes for ent-kaurene synthesis, as in seed plants.GA-inactivation by 2-oxidation is not present in nonseed plants and was acquired just before the establishment of gymnosperms (Yoshida et al. 2020).GA 2β-hydroxylation is also absent from GA-producing fungi and bacteria, whose genes for GA-biosynthesis are clustered in operons and were acquired independently of plants and each other (Hedden et al. 2001;Nett et al. 2017b).The members of both kingdoms employ CYP450s rather than 2-ODDs for 3and 20-oxidation, while F. fujikuroi uses a 2-ODD to convert GA 4 to GA 7 in GA 3 biosynthesis (Bhattacharya et al. 2012).Bacteria have separate CPS and KS enzymes, whereas fungi contain a bifunctional CPS/KS (Morrone et al. 2009).The capacity to produce bioactive GAs appears to be related to pathogenicity.Most symbiotic N-fixing bacteria produce GA 9 , allowing the plant to regulate GA 4 production, while the phytopathogenic species Xanthomonas oryzae contains an extra gene encoding a 3β-hydroxylase (CYP115) and produces GA 4 (Nagel and Peters 2017;Nett et al. 2017a).

Dwarf and slender mutants with reduced or elevated GA responses
Genetic analyses of mutants displaying altered GA responses and molecular cloning of their corresponding genes have been instrumental in unveiling the long-sought GA receptor (GID1) and its immediate downstream repressors (DELLAs) and activators (F-box proteins GID2/SLEEPY1 [SLY1]).GA-unresponsive recessive mutants exhibit a dark-green, dwarf phenotype that mimics GA biosynthesis mutants, but their growth cannot be restored by GA treatment (Fig. 1).Plants with defects in genes encoding the GA receptor GID1 or the F-box protein GID2/SLY1 belong to this mutant class (McGinnis et al. 2003;Sasaki et al. 2003;Ueguchi-Tanaka et al. 2005).Gain-of-function DELLA mutants are dominant GA-unresponsive dwarves, e.g.GA insensitive (gai) in Arabidopsis (Koornneef et al. 1985) and Reduced height (Rht) varieties in wheat (Fig. 1), which were major contributors to the "Green Revolution" by increasing grain yield in the 1960s to 1970s (Börner et al. 1996;Peng et al. 1999).Conversely, "slender" mutants with elevated GA responses (e.g.la cry in pea and slender (sln) in barley) are recessive and display a tall and thin stem phenotype, which resembles wild-type plants that have been overdosed with GA (Brian 1957;Foster 1977).
Besides genetic analysis, cereal aleurone was also used extensively to study GA signaling (Lovegrove and Hooley 2000;Sun and Gubler 2004).During seed germination, aleurone cells produce hydrolytic enzymes in response to GA (diffused from the embryo) to degrade the starchy endosperm.Using this aleurone system, pharmacological assays have identified GA-induced genes and GAMYB, the transcription factor responsible for this transcriptional induction.

GA-GID1 induces SCF SLY1/GID2 -mediated DELLA degradation
With the development of Arabidopsis as a model system for plant research in the 1980s, the gai-1 mutant and repressor of ga1-3 (rga) mutants in Arabidopsis were isolated by screening for GA-unresponsive dwarves (Koornneef et al. 1985) or suppressors of the dwarf phenotype of ga1-3 (Silverstone et al. 1997b), respectively.Intragenic suppressors of the semidominant gai-1 mutant were generated by Ds transposon insertion mutagenesis (Peng and Harberd 1993), which guided the cloning of GAI (Peng et al. 1997).Suppressor mutants of ga1-3 generated by fast-neutron mutagenesis contained large deletions in the RGA locus, which facilitated the cloning of RGA by genomic subtraction (Silverstone et al. 1998).The Arabidopsis genome contains Interaction network between the GA-GID1-DELLA signaling module and various internal and external cues.Signals that increase bioactive GA levels are labeled in blue, while signals that decrease GA levels are shown in red.GA-GID1 triggers DELLA degradation via SCF SLY1/GID2 -mediated polyubiquitination.GA-GID1 also induces OsNGR5 degradation in a SCF GID2 -dependent manner to inhibit nitrogen-induced shoot branching in rice.DELLAs interact antagonistically or additively with a myriad of transcription factors (TFs), transcription regulators (TRs), CRC, and PREFOLDINs (PFDs) to modulate specific developmental processes.Most of the DELLA interactors are Arabidopsis proteins, except those that are labeled (Os, Oryza sativa; Mt, Medicago truncatula; Lj, Lotus japonicus).See Boxes 1 and 2 for details.PD, protein degradation; PPI, protein-protein interaction; TC, transcription; SAM, shoot apical meristem; MT, microtubule; GA, gibberellin; ABA, abscisic acid.
five DELLA genes, RGA, GAI, RGA-LIKE1 (RGL1), RGL2, and RGL3, which belong to a subfamily of GRAS (for GAI, RGA and SCARECROW) transcription regulators.The N-terminal DELLA domain is unique to the DELLA subfamily, whereas the C-terminal GRAS domain is shared among all GRAS family members (Pysh et al. 1999;Sun and Gubler 2004).Further characterization of orthologs in other species showed that DELLA genes are conserved in plants, including Rht in wheat (Peng et al. 1999), SLENDER RICE1 (SLR1) in rice (Ikeda et al. 2001), SLN1 in barley (Chandler et al. 2002), D8 and D9 in maize (Peng et al. 1999;Lawit et al. 2010), PROCERA in tomato (Solanum lycopersicum) (Jasinski et al. 2008), and LA and CRY in pea (Weston et al. 2008).
How are DELLA proteins regulated by the GA signal?The la cry slender mutant phenotype resembles the effects of GA overdose, leading to the idea that LA and CRY control the production of inhibitors (for GA-induced growth) and suggesting that GAs may function as "inhibitors of inhibitors" to promote growth (Brian 1957).Importantly, an examination of RGA protein levels by immunoblot analysis and confocal microscopy revealed that RGA protein levels in planta rapidly decreased in response to GA treatment (Silverstone et al. 2001).Furthermore, the gai-1 Arabidopsis mutant encodes a mutant protein with a 17-amino acid deletion within the DELLA motif, suggesting that this mutation turns the GAI protein into a constitutive repressor of GA signaling (Peng et al. 1997).Indeed, deletion of the identical DELLA motif in RGA (rga-Δ17) abolished GA-induced degradation and conferred a GA-unresponsive dwarf phenotype, indicating that the DELLA motif is required for its proteolysis in response to GA (Dill et al. 2001).Notably, the semidwarf varieties of wheat and maize were found to be caused by deletion mutations in the DELLA domain of Rht and D8, respectively (Peng et al. 1999).Further studies of the recessive GA-unresponsive dwarf mutants Arabidopsis sly1 and rice gid2 led to the identification of F-box proteins and associated Skp, Cullin, F-box (SCF) ubiquitin E3 ligase complexes (SCF SLY1/GID2 ) that are responsible for polyubiquitination of DELLA and degradation by the 26S proteasome (Steber et al. 1998;McGinnis et al. 2003;Sasaki et al. 2003).
Although Arabidopsis research led to the breakthrough discoveries of the DELLA repressors and SLY1 (F-box) activators of GA signaling, the GA receptor remained elusive despite the efforts of multiple mutant screens.Eventually, aided by the completion of the rice genome sequence (Goff et al. 2002;Yu et al. 2002), the GA receptor was unveiled by positional cloning of GA-insensitive dwarf1 (gid1) mutants in rice (Ueguchi- Tanaka et al. 2005).Notably, the smaller genome of Arabidopsis contains three GID1 orthologs (GID1A, GID1B, and GID1C), whose functional redundancy explains why genetic screens failed to identify GA receptors in Arabidopsis (Griffiths et al. 2006;Nakajima et al. 2006).GID1 is localized to both the cytoplasm and nucleus and belongs to the hormone-sensitive lipase (HSL) family, although it lacks one of three key catalytic residues for lipase activity.Yeast two-hybrid (Y2H) and in vitro pull-down assays show that GA binding to GID1 promotes GID1-DELLA interactions (Ueguchi- Tanaka et al. 2005) and that the DELLA domain (including DELLA, LEXLE and VHYNP motifs) is essential for its interaction with GID1 (Griffiths et al. 2006;Willige et al. 2007).Molecular details of the GA-AtGID1A-DELLA domain (GAI) complex and GA-OsGID1 determined by X-ray crystallography revealed that bioactive GA is an allosteric inducer of its receptor GID1 (Murase et al. 2008;Shimada et al. 2008).The carboxyterminal core domain of GID1 forms a GA-binding pocket, and the amino-terminal extension (N-Ex) domain acts as a lid.GA binding induces a conformational switch of its N-Ex to close the GA-binding pocket and creates hydrophobic surfaces for DELLA binding (Fig. 2).
How does GA-GID1-DELLA promote SLY1/GID2 recognition?Mutant and Y2H analyses indicated that SLY1/GID2 interacts with the GRAS domain of the DELLA protein (Dill et al. 2004;Hirano et al. 2010).Yeast 3-hybrid assays further demonstrated that GA-bound GID1 enhances the RGA-SLY1 interaction, suggesting that the GA/GID1-DELLA domain interaction triggers conformational changes in the GRAS domain for SLY1 recognition (Griffiths et al. 2006).Moreover, the GRAS domain of SLR1 was shown to interact with GID1 after the binding of the DELLA domain to further stabilize the GID1-SLR1 complex, which allows efficient recognition by the F-box protein GID2 (Hirano et al. 2010).

Mechanism of DELLA action: transcriptional reprograming via protein-protein interactions with hundreds of transcription factors
DELLAs are nucleus-localized transcription regulators.Transcriptome studies on early GA-and DELLA-responsive genes showed that DELLAs can activate or repress transcription, depending on the target genes (Zentella et al. 2007;Hou et al. 2008).DELLAs do not contain any canonical DNA binding motifs and have not been shown to bind DNA directly.Importantly, chromatin immunoprecipitation (ChIP)-qPCR analysis demonstrated an association of RGA with its target chromatin (Zentella et al. 2007).ChIP-sequencing (seq) analysis identified genome-wide RGA binding sites: 421 associated genes in Arabidopsis seedlings and 2,327 associated genes in the inflorescence meristem (Marin-de la Rosa et al. 2015;Serrano-Mislata et al. 2017).Abundant evidence indicates that DELLAs regulate transcription via antagonistic or additive interactions with a myriad of transcription factors/regulators (Figs. 2 and 3 and Boxes 1 and 2) (Sun 2011;Daviere and Achard 2016;Van De Velde et al. 2017).PHYTOCHROME INTERACTING FACTORS (PIFs), PIF3, and PIF4 were the first reported DELLA-interacting transcription factors (TFs) (de Lucas et al. 2008;Feng et al. 2008).PIF3 and PIF4 are light-responsive bHLH TFs that promote hypocotyl elongation.Genetic analysis and ChIP-qPCR showed that the DELLA-PIF3/4 interaction sequesters PIFs from binding to the promoters of growth-related genes, revealing molecular crosstalk between light and GA signaling.Extensive studies in the last 15 years have identified 370 potential DELLA-interacting proteins in Arabidopsis by Y2H screens, and over 40 of them have been verified by co-IP and/or genetic analyses (Marin-de la Rosa et al. 2014;Van De Velde et al. 2017;Lantzouni et al. 2020).

BOX 2. DELLA INTERACTORS: TRANSCRIPTION REPRESSORS AND OTHERS
(1) DELLA-repressed transcription repressors include the jasmonate (JA) signaling repressors JAZs, which promote JA-induced defense responses against herbivory and necrotrophs (Hou et al. 2010).Moreover, the JAZ-DELLA interaction inhibits DELLA-PIF3 to promote plant growth, revealing the role of JAZ/DELLA/PIF in balancing plant defense and growth (Yang et al. 2012).DELLAs also inhibit SCL3 (a GRAS protein) activity by interacting and competing with SCL3 for binding to IDDs (Zhang et al. 2011;Yoshida et al. 2014).SCL3 is an activator of GA signaling whose transcription is induced by DELLA but repressed by itself.In addition, DELLAs inhibit the activity of GRFs in promoting the expression of cold-induced genes (Lantzouni et al. 2020).
analyses showed that RGA binding peaks are enriched near cis-elements for several DELLA-interacting TFs (Marin-de la Rosa et al. 2015;Serrano-Mislata et al. 2017), supporting the notion that DELLAs are recruited to target promoters by their interacting TFs.

Multiple signaling pathways regulate DELLA-mediated plant responses to internal and environmental cues
DELLAs were initially identified as GA signaling repressors, and GA promotes rapid DELLA proteolysis mediated by GID1 and SCF SLY1/GID2 (Sun and Gubler 2004).Notably, DELLAs also play a key role in feedback regulation to help maintain GA homeostasis by inducing the transcription of genes encoding GA biosynthetic enzymes and GID1s (Fig. 3) (Zentella et al. 2007).However, extensive studies of DELLA interactors and DELLA-regulated processes in the last 15 years have unveiled a much broader function of DELLAs as master growth regulators that integrate the activities of many signaling pathways in response to developmental and external cues, including biotic and abiotic stress (Thomas et al. 2016;Van De Velde et al. 2017).Boxes 1 and 2, and Fig. 3 highlight the diverse processes regulated by DELLAs and their interactors.Importantly, DELLA activity can be regulated by several mechanisms: (i) altered DELLA stability (GA-GID1 dependent) by modulating GA metabolism; (ii) altered DELLA activity by interacting with TFs/ TRs/chromatin-remodeling complexes (CRC); (iii) GA-GID1independent polyubiquitination and degradation; (iv) other post-translational modifications (PTMs); and (v) transcriptional induction of RGL3 by JA signaling.
(1) Altered DELLA stability (GA-GID1 dependent) by modulating GA metabolism Factors that decrease bioactive GA levels to increase DELLA accumulation include other phytohormones (ABA, cytokinin, and ethylene), external cues (e.g.light, abiotic stresses [cold, salt, and drought], and biotic stress [biotrophic pathogens]) (Fig. 3).Conversely, factors that increase bioactive GA levels to decrease DELLA accumulation include auxin, and external cues (e.g.nitrogen, light, abiotic stresses [warmth, shade, submergence], and biotic stress [necrotrophic pathogens]).Most of these findings have been discussed in previous reviews (Sun 2011;Colebrook et al. 2014), except for two recent studies showing that drought inhibits GA biosynthesis in the leaf base of wheat seedlings (Ptošková et al. 2022) and that nitrate (a major nitrogen sources) induces root growth by increasing GA biosynthesis, resulting in reduced DELLA protein accumulation in Arabidopsis and wheat (Camut et al. 2021).Recent studies on the semidwarf Green Revolution varieties (GRVs) of wheat (Rht alleles encoding dominant DELLAs) and rice (semi-dwarf1 [sd1], defective in GA20ox2) demonstrated that nitrogen use efficiency (NUE) is regulated by the GA signaling pathway (Wang et al. 2021;Liu et al. 2022).The GRVs dramatically increase crop yields, although they exhibit low NUE because SLR1 inhibits nitrogen and carbon metabolism, nitrogen uptake, and assimilation by disrupting the interaction between the key TF OsGRF4 and its coactivator OsGIF1 (Li et al. 2018) (Fig. 3).Notably, elevated DELLA activities in GRVs promote nitrogen-induced tillering (shoot branching).It turns out that GID1 and DELLA can interact with NITROGEN MEDIATED TILLER GROWTH RESPONSE 5 (NGR5), a transcription factor that represses the expression of genes that inhibit tillering (Wu et al. 2020).GA-GID1 promotes NGR5 degradation by the SCF GID2 -mediated ubiquitin-proteasome pathway (Fig. 3), while DELLA competes with GID1-NGR5 interaction to stabilize NGR5.
CONSTITUTIVE PHOTOMORPHOGENIC1 (COP1) mediates DELLA degradation in response to warm temperatures and shade: Shade-or warm temperature-induced hypocotyl elongation correlates with elevated bioactive GA levels and a reduction in DELLA protein levels (Djakovic-Petrovic et al. 2007;Stavang et al. 2009;Arana et al. 2011).Surprisingly, the abundance of the GA-resistant rga-Δ17 protein is also reduced by these environmental cues, suggesting the presence of a GA/GID1-independent mechanism for DELLA degradation (Blanco-Tourinan et al. 2020a).Biochemical and genetic analyses showed that the E3 ubiquitin ligase COP1 and its interacting protein SUPPRESSOR OF phyA-105 proteins (SPAs) play a direct role in the rapid proteolysis of DELLA prior to changes in GA content in the shade or under warm conditions.As the liverwort (Marchantia polymorpha) genome contains putative orthologs of COP1 and DELLA genes, COP1-mediated DELLA degradation may serve to regulate DELLA activity prior to the GA/GID1-mediated mechanism, which appears later in lycophytes.
FLAVIN-BINDING KELCH REPEAT F-BOX 1 (FKF1) mediates DELLA degradation to promote flowering in LD conditions: FKF1 promotes flowering under long-day (LD) conditions.The fkf1 mutant is late flowering and has elevated RGA protein levels even in the GA-deficient background (Yan et al. 2020).co-IP assays in Nicotiana benthamiana and in vitro assays showed that FKF1 directly binds to DELLAs and promotes their ubiquitination and degradation.It was proposed that FKF1 regulates the cyclical degradation of DELLA in LDs, but this remains to be verified.
Strigolactone (SL)-D14 mediates DELLA degradation in response to low nitrogen conditions: As described above, GA reduces NUE by promoting NGR5 degradation.Conversely, SL increases NUE.D53 is a repressor of SL signaling that inhibits the expression of GRF4-induced genes for N metabolism.Low nitrogen conditions induce the biosynthesis of SL, which binds to its receptor D14 and promotes the D14-D53 interaction and subsequent SCF D3 -mediated ubiquitination and degradation of D53.Notably, SL also promotes the interaction of D14 with SLR1 (rice DELLA) (Nakamura et al. 2013), which leads to SLR1 degradation mediated by SCF D3 (Sun et al. 2023).D53 competes with SLR1 for binding to D14, adding another layer of regulation for DELLA degradation.Under salt-stress conditions, DELLA SUMOylation is induced due to increased degradation of the SUMO proteases OVERLY TOLERANT TO SALT 1 and 2 (OTS1 OTS2) (Conti et al. 2014).SUMOylated DELLA binds to and sequesters GID1 independently of GA, thereby promoting the accumulation of non-SUMO-DELLA and restricting plant growth.Under nonstress conditions, OTS-mediated de-SUMOylation of DELLA promotes the growth of stamen filaments (Campanaro et al. 2016).The role of phosphorylation in DELLA function is not well understood.An early study reported that GA-induced SLR1 degradation in rice occurs independently of phosphorylation (Itoh et al. 2005).However, another study suggested that the phosphorylation of SLR1 by the casein kinase I EARLIER FLOWERING1 (EL1) increases its stability (Dai and Xue 2010).The el1 mutant displays elevated GA response and early flowering phenotypes, and the SLR1-YFP (yellow fluorescent protein) protein in 35S: SLR1-YFP el1 transgenic rice was degraded more rapidly after GA treatment than in the wild-type background.These findings suggest that EL1 may inhibit GA signaling by enhancing DELLA stability, although SLR1 phosphorylation by EL1 was only shown in vitro.
The discovery of the role of O-glycosylation in regulating DELLA activity came from the characterization of the Arabidopsis spindly (spy) mutants, which partially rescue the GA-deficient dwarf phenotype caused by a GA biosynthesis inhibitor (paclobutrazol) or a mutation (ga1), indicating that SPY is a repressor of GA signaling (Jacobsen and Olszewski 1993;Jacobsen et al. 1996;Silverstone et al. 1997bSilverstone et al. , 2007)).Both SPY and its paralog SECRET AGENT (SEC) in Arabidopsis were predicted to be O-GlcNAc transferases (OGTs) based on sequence analysis (Olszewski et al. 2010).Both SPY and SEC contain a tetratricopeptide-repeat (TPR) domain and a putative OGT catalytic domain.Surprisingly, electron transfer dissociation (ETD)-MS/MS and in vitro enzyme assays showed that SPY O-fucosylates DELLAs and that SEC O-GlcNAcylates DELLAs (Zentella et al. 2016(Zentella et al. , 2017)).Genetic analysis and pulldown assays further showed that O-fucosylation of DELLA by SPY enhances DELLA binding to TFs (e.g.BZR1 and PIFs), while O-GlcNAcylation of DELLA by SEC reduces DELLA activity.As OGT serves as a nutrient sensor in metazoans (Hart 2019), it was proposed that O-Fuc and O-GlcNAc modifications might modulate DELLA activity and plant growth in response to nutrient availability.
(5) Transcriptional induction of RGL3 by JA signaling RGL3 transcription is rapidly induced by MYC2, which is a JA signaling activator (Wild et al. 2012).As RGL3 binds to and sequesters the JA signaling repressors JAZs, elevated expression of RGL3 in response to the JA signal enhances MYC2 activity to promote JA-mediated resistance to necrotrophic pathogens.

DELLA-independent GA responses
Although DELLAs control almost all GA-regulated processes, a few DELLA-independent GA responses have been reported.SPATULA (SPT), a bHLH TF that is unrelated to DELLAs, also inhibits GA-induced cotyledon expansion and fruit growth (Josse et al. 2011;Fuentes et al. 2012).The SPT-repressed cotyledon expansion is independent of light conditions, which is in contrast to DELLA, whose stability is reduced by red light-induced GA biosynthesis.Notably, DELLAs negatively regulate SPT transcript accumulation, which provides a balance between the two classes of repressors (Josse et al. 2011).Another DELLA-independent GA response is GAinduced increases in cytosolic Ca 2+ levels, although it remains to be determined whether this GA response is mediated by GID1 in the cytoplasm (Okada et al. 2017).

Long-distance GA transport
Nearly half a century ago, initial findings were reported on the movement of GA in plants (Zweig et al. 1961;Chin and Lockhart 1965;Hoad and Bowen 1968).These studies confirmed the presence of GA in the phloem sap and its ability to travel through this medium.Since then, ongoing efforts have been made to understand and measure the movement of GA in plants (Hedden and Sponsel 2015;Binenbaum et al. 2018).GA moves within the plant in both upward (acropetal) and downward (basipetal) directions (Proebsting et al. 1992;Bjorklund et al. 2007;Regnault et al. 2015;Lacombe and Achard 2016).The movement of GA is crucial for various developmental processes in plants (Anfang and Shani 2021;Zhang et al. 2023).
Several studies have attempted to identify the mobile form of GA by perturbing GA biosynthesis at different stages of the pathway.In peas, grafting mutant plants deficient in GA biosynthetic enzymes onto wild-type plants led to an increase in GA content in the shoots compared to non-grafted mutant plants.GA analysis revealed that GA 20 was the major mobile form in pea plants (Proebsting et al. 1992).Similarly, in Arabidopsis, grafting experiments with mutant plants at different stages of GA biosynthesis identified GA 12 as the major form transported over long distances through the vasculature (Regnault et al. 2015) (Fig. 5).GA 12 moves through the xylem from roots to shoots and through the phloem from shoots to roots to regulate plant growth (Regnault et al. 2015).The transport activity is most evident in plants that fail to synthesize GA locally.It was furthermore demonstrated that GA 12 derived in the roots plays a role in regulating the growth of shoots in response to temperature changes in Arabidopsis (Camut et al. 2019).Most recently, it was reported that two GA and ABA transporters (NPF2.12 and NPF2.13) are required for shoot-to-root GA 12 translocation to regulate endodermal root suberization (summarized below) (Binenbaum et al. 2023).

GA movement and localization
The synthesis of active GA is a complex and multistep process involving various intermediate compounds (Fig. 2).This complexity makes it challenging to identify the specific tissues or organs where GAs are produced and localized.Analysis of GA biosynthesis reporter lines indicated that while some tissues show colocalization of GA biosynthesis genes and GA perception genes, there are cases where these two groups of genes do not overlap.For example, GA biosynthesis genes are not expressed in the aleurone cells of the rice endosperm, but GA signaling genes are (Kaneko et al. 2003).This spatial separation suggests the need for GA movement within the plant.In addition, the expression levels of genes involved in the GA biosynthesis pathway itself do not always align.For instance, the expression of the late-stage GA biosynthesis genes AtGA3ox1 and AtGA3ox2 in germinating embryos differs spatially from that of the early GA biosynthesis .12 and NPF2.13 are found in the phloem of the shoot and play vital roles in transporting GA 12 over long distances from shoot to root.NPF2.12 is active in the membranes of root pericycle cells and facilitates the movement of ABA and GA from the vasculature to the pericycle region.Once inside the pericycle's cytoplasm, NPF2.14 transports these hormones into the vacuole, where they are possibly stored as a reserve for future use.As the root elongates over time and these cells mature, the stored hormones are released from the pericycle vacuole and taken up by the endodermis through the action of NPF3.1.This uptake triggers suberization, a process that forms a protective barrier in the endodermis.In addition, GA 12 derived in the root, plays a role in regulating the shoot growth in response to ambient temperatures (28°C) in Arabidopsis.PCC, phloem companion cell; PS, phloem sieve; Pe, pericycle; End, endodermis; Vac, vacuole; GA, gibberellin; ABA, abscisic acid.
gene AtCPS (Silverstone et al. 1997a;Yamaguchi et al. 2001).Similar patterns are found in different root cell types (Barker et al. 2021).Such differences indicate that the location and movement of GA precursors could play a vital role in regulating GA responses.An interesting example of GA precursor translocation was found in the fern L. japonicum, where GA movement is involved in the sex-determining mechanism.The study proposed a model in which different stages of prothalli in a colony express different GA-biosynthetic genes, producing specific forms of GA that regulate the formation of reproductive structures (Tanaka et al. 2014).In the future, there is a need to measure GA contents (including bioactive GAs and precursors) in different tissues and cell types at the single-cell level to shed light on the GA map with respect to its dynamic movement.
Long and short-distance movement of different GA forms are crucial for plant development (Rizza and Jones 2019;Wexler et al. 2019;Anfang and Shani 2021).For example, one of the functions of GA is to induce xylem differentiation in the hypocotyl following the floral transition in Arabidopsis.GA3ox1 mRNA levels increase in the shoot but not the hypocotyl after flowering, suggesting GA movement.Mutant plants lacking GA biosynthesis, such as the ga1-3 mutant, exhibit reduced hypocotyl xylem expansion after the flowering stage (Ragni et al. 2011).However, xylem expansion was restored when the mutant plants were grafted onto wild-type rootstocks.This suggests that GA acts as a mobile signal derived from the shoot that triggers xylem expansion in the hypocotyl (Ragni et al. 2011).Similar effects were observed in tobacco (Nicotiana tabacum) plants when defoliation occurred, resulting in reduced GA content and growth abnormalities in the stem (Dayan et al. 2012).
Additional reports have described the dependency of certain organs on external sources of GA.For example, GA movement from the embryo scutellum to the aleurone in cereal grains plays a pivotal role in regulating seed germination (Paleg 1960).Upon imbibition, during germination, the scutellum synthesizes GAs, which move to the aleurone layer (Hayashi 1940).In the aleurone, GA triggers the activation of hydrolytic enzymes that break down the stored starch and proteins in the endosperm into simpler forms, providing essential nutrients for the developing embryo (Lovegrove and Hooley 2000;Sun and Gubler 2004).This coordinated GA-mediated movement and response from scutellum to aleurone are fundamental for successful germination and early seedling growth in cereal grains.
In addition, petals rely on anthers as a source of GA for their growth and development (Hu et al. 2008).Studies in Arabidopsis, petunia (Petunia hybrida), tobacco, and rice demonstrated that GA produced in the anthers is crucial for petal development (Weiss and Halevy 1989;Itoh et al. 1999Itoh et al. , 2001;;Hu et al. 2008).These pieces of evidence support the idea that GA acts as a mobile plant hormone and that its movement is necessary for various processes involved in plant growth and development.
In cucumber flowers, specific forms of GA were found to be localized to different floral parts, suggesting their involvement in localized growth regulation.Experiments using deuterated GA provided quantitative support for the production and movement of GA from ovaries to sepals and petals, where it is converted to a bioactive form to regulate organ growth (Lange and Lange 2016).A study characterizing GA biosynthesis sites in roots at the cellular level, coupled with cell-type-specific GA synthesis rescue experiments, indicated GA movement between root cell-files (Barker et al. 2021).Analysis of photocaged bioactive GA 4 released endogenously in Arabidopsis roots allowed the kinetic parameters of its flow to be measured, such as decay length and velocity (Wexler et al. 2019).More comprehensive studies are needed to explore additional developmental stages where GA movement plays a fundamental role by correlating the expression patterns of GA biosynthetic genes with direct measurements of GA levels.

GA transporters
The first evidence of bioactive and regulated GA transport came with the identification of GA transporters from the NPF (Chiba et al. 2015;Saito et al. 2015;David et al. 2016;Tal et al. 2016;Anfang and Shani 2021;Kanstrup and Nour-Eldin 2022).Several NPF transporter proteins, including NPF2.3, NPF2.4,NPF2.5, NPF2.7,NPF2.10, and NPF3.1 have been identified as potential GA transporters using yeastmodified 2-hybrid systems and further confirmed in Xenopus oocytes (Chiba et al. 2015;Saito et al. 2015;Wulff et al. 2019).However, the physiological importance of most of these transporters in plants remains to be fully understood.The main challenge in characterizing GA transporters and their physiological function is the lack of apparent GA-mediated phenotypes in the respective mutants.Genetic redundancy plays a substantial role in this shortcoming, as most, if not all, transporter proteins belong to large and robust gene families.Thus, the knockout of one putative GA transporter is compensated for by another family member (Zhang et al. 2023).
Recent research has revealed that a subset of NPF proteins is required for the mechanisms behind long-distance GA transport from shoot to root and its developmental importance (Binenbaum et al. 2023).GA transport plays a critical role in suberin formation in the root.NPF2.12 and NPF2.13 (2 recently identified GA and ABA importers), along with NPF2.14 (a tonoplast importer), coordinate the regulation of suberin formation (Binenbaum et al. 2023).NPF2.12 and NPF2.13 are membrane-localized proteins expressed in leaf phloem companion cells that facilitate the transport of GA 12 from shoot to root (Fig. 5).Once reaching the root, GA 12 is converted to GA 4 by the enzymes GA20ox and GA3ox.It is speculated that the bioactive GA and ABA exit the phloem at the phloem unloading zone (Robe and Barberon 2023) located around the root elongation zone (Binenbaum et al. 2023).NPF2.12 is then able to import GA 4 and ABA into the pericycle, and subsequently, the pericycle-specific transporter NPF2.14 transports these phytohormones into the vacuole (Fig. 5) GA and ABA accumulate in the vacuole within the phloem unloading zone located around the root elongation zone, where they are stored during root maturation and differentiation.Only later in development are these plant hormones released from the vacuole by an unknown mechanism and are able to be taken into the endodermis by NPF3 to promote suberization.NPF3 is localized to the plasma membrane and imports GAs in a pH-dependent manner (David et al. 2016;Tal et al. 2016) (Fig. 5).These findings indicate that GA and ABA can work in a nonantagonistic manner to regulate plant development.This mechanism highlights the importance of long-distance shoot-to-root movement of GA 12 and the accumulation of bioactive GA 4 and ABA in the endodermis for regulating endodermal suberization (Binenbaum et al. 2023;Zhang et al. 2023).
In Arabidopsis, the Sugars Will Eventually Be Exported Transporters (SWEET) family members SWEET13 and SWEET14 have been identified as GA transporters (Kanno et al. 2016;Morii et al. 2020).These transporters import GAs, as demonstrated in yeast and oocyte transport assays (Kanno et al. 2016).SWEET13 and SWEET14 function redundantly to regulate anther development, and the application of exogenous GAs to the sweet13 sweet14 double mutant rescues the anther's dehiscence defect (Kanno et al. 2016).In rice, OsSWEET3a acts as both a sugar transporter and a GA transporter, playing roles in seed germination and early shoot development (Morii et al. 2020).

GA biosensors and markers
Studies utilizing GA biosensors have provided insights into the transport and localization of GAs, indicating that GAs are highly mobile (Rizza and Jones 2019).Specifically, analysis using the GA perception biosensor GA Perception Sensor 1 (GPS1) revealed that, in the root, the concentration of bioactive GA is highest in the root elongation zone (Rizza et al. 2017).GPS1 represents a pioneering biosensor that utilizes Förster resonance energy transfer (FRET) to detect and track cellular GA levels in planta.This biosensor contains AtGID1C and the N-terminal domain of AtGAI, which are linked to two fluorescent proteins that produce FRET when GA binding to GID1C triggers an intramolecular conformational change.The assessment of a fluorescence emission ratio of nuclear localized-GPS1 (nlsGPS1) enables the precise mapping of endogenous and externally administered GA gradients within various tissue structures at the cellular level.The use of nlsGPS1 live imaging, combined with comprehensive modeling, revealed that a disparity in GA biosynthesis along the roots is accountable for shaping the distribution of GA (Rizza et al. 2021).Another biosensor based on the DELLA protein RGA, named qmRGA (pRPS5a::RGAmPFYR-VENUS), provided in planta information on changes in GA responses at the cellular level in the shoot apical meristem, with GA signaling found primarily in cells located between organ primordia (Shi et al. 2021).
Furthermore, experiments involving fluorescently labeled bioactive GAs demonstrated the exclusive accumulation of GAs in the root elongation zone (Shani et al. 2013) and in leaf mesophyll cells (Matias-Hernandez et al. 2016), suggesting that GAs move from one tissue to another.The latter process is regulated by two transcription factors, TEMPRANILLO1 (TEM1) and TEM2, which negatively regulate the expression of genes encoding specific GA transporters (GLUCOSINOLATE TRANSPORTER1 (GTR1), NPF3, and NPF2.3) belonging to the NPF family, leading to variable GA accumulation and distribution in mesophyll cells that regulate trichome initiation in the epidermis (Matias-Hernandez et al. 2016).
While the GPS1 FRET biosensor (Rizza et al. 2021) and the qmRGA ratiometric GA signaling biosensor (Shi et al. 2021) report on GA localization based on perception mechanisms, limited progress has been made in generating GA biosensors that are based on transcriptional reporters.Such transcriptional reporters have been widely used in other phytohormone research based on promoters of endogenous phytohormone-induced genes or synthetic transcriptional reporters (Ulmasov et al. 1997;Muller and Sheen 2008;Kim et al. 2011;Okamoto et al. 2013;Liao et al. 2015;Wu et al. 2018).Dayan et al. generated several β-glucuronidase reporters based on the GA-induced promoters of EXP1, MYB34, and GA2OX2 and a synthetic GA-responsive promoter (FK) containing known GA-response cis-elements found in promoters of α-amylase genes from cereal crops (Dayan et al. 2012).However, constructing a universal GA reporter that reflects the broad range of transcriptional regulation (Fig. 3), remains challenging.Such a reporter would need to respond specifically to endogenous GA levels in all tissues and cell types, with an appropriate reporter turnover rate.It may be difficult to design GA reporters that respond to both DELLA-dependent and -independent pathways.
Despite the progress made, several open questions remain regarding GA transport (see Outstanding questions).One unanswered question is whether there are GA exporters capable of transporting GAs from the cytosol to the apoplast.Currently, no proteins with this function have been identified, but it is believed that such proteins must exist to overcome the GA ion-trapping mechanism.In addition, considering the recent findings regarding GA accumulation in the pericycle vacuole, one could speculate that GA is actively transported out of the vacuole and pericycle cells to reach the endodermis.However, the specific transporters responsible for this process have not yet been identified.Furthermore, the relevance of movement of GA through plasmodesmata and the apoplast remains unclear.A recent discovery demonstrated that the plant hormone ABA travels radially through the plasmodesmata in the root to regulate lateral root branching in response to water stress (air gaps in the soil) (Mehra et al. 2022).Investigating whether a similar mechanism applies to GA in various developmental and environmental responses would be intriguing.Further research is required to fully understand the transport and localization of GAs in plants.

Concluding remarks
In the last three decades, substantial progress has been made in elucidating the regulation of GA metabolism and the molecular mechanism of GA perception and early GA signaling.The central role of DELLAs as integrators of multiple signaling pathways has clearly been demonstrated, although the specificity of these key growth regulators in distinct tissue/celltype requires further investigation (see Outstanding Questions).Recently identified GA transporters and the development of GA biosensors are important advances toward understanding how GA regulates plant growth and development in response to internal and external cues (see Outstanding Questions).The development of methods for analyzing GA content at the single-cell level in combination with existing molecular/genomics/proteomics tools will allow us to achieve this goal in the future.

OUTSTANDING QUESTIONS
• How are GA metabolism, transport, and signaling activities regulated in different cell/tissue types to coordinate plant growth and development?
• What is the role of post-transcriptional regulation of GA-metabolic enzymes in determining GA concentration?
• How do DELLAs interact with a myriad of distinct classes of TFs/transcriptional regulators (TRs), and does the tissue/cell-type specific expression of DELLAs and their interacting TFs/TRs determine the selective regulation of a subset of target genes?
• Do GA exporters exist and, if so, what are their developmental roles and specificity?

Figure 1 .
Figure 1.GA regulates plant growth and development.Shown are 12-wk-old GA-unresponsive vs -responsive mutants in wheat.All the mutant lines are in cv.Cadenza background.The gain-of-function Rht-D1b and Rht-B1c (DELLA) alleles were introduced into Cadenza from cvs Avalon and Mercia, respectively (Van De Velde et al. 2021).The hypomorphic gid1 and loss-of-function ga3ox2 and rht-1 plants were produced by TILLING after EMS-induced mutagenesis (A.L.Phillips and S.G.Thomas, unpublished data).All plants were untreated (-) or treated (+) twice-weekly with 10 µM GA 3 .Rht and gid1 mutants are unresponsive to GA treatment, whereas GA completely rescued the GA-biosynthesis mutant ga3ox2.Scale bar = 40 cm.

Figure 2 .
Figure2.GA metabolism, transport, perception, and signaling in plant cells.GA biosynthesis takes place in three cellular compartments: ent-Kaurene is synthesized from GGPP by CPS and KS in the plastid; ent-Kaurene is converted to ent-kaurenoic acid by KO on the outer plastid membrane, which is connected to the ER; ent-Kaurenoic acid is converted to GA 12 by KAO and GA 12 to GA 53 by GA13ox in the ER; GA 12 and GA 53 are converted to bioactive GA 4 and GA 1 , respectively, by GA20ox and GA3ox in the cytoplasm.GA 4 and GA 1 as well as their immediate precursors GA 9 and GA 20 , respectively, are oxidized on C-2 by C 19 -GA2ox, resulting in inactivation, while C 20 -GA2ox acts on earlier C 20 -GA precursors.In addition to de novo biosynthesis, GA can be imported into the cell by GA transporters nitrate and peptide transporter families (NPFs) and SWEETs or transported into the vacuole as labeled.GA perception and signaling occur in the nucleus where GA binding to its receptor GID1 (+GA) promotes DELLA degradation via Skp, Cullin, F-box (SCF) SLY1/GID2 -mediated polyubiquitination and subsequent proteolysis by the 26S proteasome.When GA levels are low (− GA), DELLAs accumulate to high levels.Three distinct modes of DELLA action are shown: (i) DELLA represses transcription by blocking DNA binding and sequestering transcription factors (TF in blue) from target promoters; (ii) DELLA induces transcription by recruiting TFs (in pink); and (iii) DELLA induces transcription by sequestering transcription repressors (TR in green) from target promoters.GGPP, trans-geranylgeranyl diphosphate; CPP, ent-copalyl diphosphate; CPS, ent-copalyl diphosphate synthase; KS, ent-kaurene synthase; KO, ent-kaurene oxidase; KAO, ent-kaurenoic acid oxidase; GA13ox, GA 13-oxidase; GA20ox, GA 20-oxidase; GA3ox, GA 3-oxidase; GA2ox, GA 2-oxidase.GA biosynthesis enzymes are labeled in blue, and the deactivation enzymes are labeled in red.GA, gibberellin; TF, transcription factor; TR, transcription repressors; ER, endoplasmic reticulum.
Figure3.Interaction network between the GA-GID1-DELLA signaling module and various internal and external cues.Signals that increase bioactive GA levels are labeled in blue, while signals that decrease GA levels are shown in red.GA-GID1 triggers DELLA degradation via SCF SLY1/GID2 -mediated polyubiquitination.GA-GID1 also induces OsNGR5 degradation in a SCF GID2 -dependent manner to inhibit nitrogen-induced shoot branching in rice.DELLAs interact antagonistically or additively with a myriad of transcription factors (TFs), transcription regulators (TRs), CRC, and PREFOLDINs (PFDs) to modulate specific developmental processes.Most of the DELLA interactors are Arabidopsis proteins, except those that are labeled (Os, Oryza sativa; Mt, Medicago truncatula; Lj, Lotus japonicus).See Boxes 1 and 2 for details.PD, protein degradation; PPI, protein-protein interaction; TC, transcription; SAM, shoot apical meristem; MT, microtubule; GA, gibberellin; ABA, abscisic acid.

Figure 4 .
Figure 4. GA/GID1-dependent versus GA/GID1-independent DELLA degradation.GA/GID1-dependent proteolysis of DELLA is mediated by SCF SLY1/GID2 .DELLA can be destabilized by signals including warmth, shade, LD light, and low nitrogen conditions.COP1 and its associated CUL4-DDB COP1 ubiquitin E3 ligase complex mediate warmth-and shade-induced DELLA degradation in Arabidopsis.The SCF FKF1 ubiquitin E3 ligase complex mediates LD-induced DELLA proteolysis in Arabidopsis.Low nitrogen conditions induce the biosynthesis of SL in rice, which binds to its receptor D14 and promotes the D14-DELLA interaction and DELLA degradation mediated by SCF D3 .GA, gibberellin; Ub, ubiquitin.

Figure 5 .
Figure5.Model of the role of NPF2s activity in regulating shoot-to-root translocation of GA 12 to promote endodermal suberin deposition.NPF2.12 and NPF2.13 are found in the phloem of the shoot and play vital roles in transporting GA 12 over long distances from shoot to root.NPF2.12 is active in the membranes of root pericycle cells and facilitates the movement of ABA and GA from the vasculature to the pericycle region.Once inside the pericycle's cytoplasm, NPF2.14 transports these hormones into the vacuole, where they are possibly stored as a reserve for future use.As the root elongates over time and these cells mature, the stored hormones are released from the pericycle vacuole and taken up by the endodermis through the action of NPF3.1.This uptake triggers suberization, a process that forms a protective barrier in the endodermis.In addition, GA 12 derived in the root, plays a role in regulating the shoot growth in response to ambient temperatures (28°C) in Arabidopsis.PCC, phloem companion cell; PS, phloem sieve; Pe, pericycle; End, endodermis; Vac, vacuole; GA, gibberellin; ABA, abscisic acid.