Molecular Communication for Coordinated Seed and Fruit Development: What Can We Learn from Auxin and Sugars?

Seed development in flowering plants is a critical part of plant life for successful reproduction. The formation of viable seeds requires the synchronous growth and development of the fruit and the three seed structures: the embryo, the endosperm, the seed coat. Molecular communication between these tissues is crucial to coordinate these developmental processes. The phytohormone auxin is a significant player in embryo, seed and fruit development. Its regulated local biosynthesis and its cell-to-cell transport capacity make of auxin the perfect candidate as a signaling molecule to coordinate the growth and development of the embryo, endosperm, seed and fruit. Moreover, newly formed seeds need nutrients and form new carbon sink, generating high sugar flow from vegetative tissues to the seeds. This review will discuss how auxin and sugars may be considered as signaling molecules to coordinate seed and fruit development.


Auxin Movement within the Different Seed Structures Triggers Different Developmental Outputs
One of the examples of perfect growth coordination between fruit and seeds is the positive correlation between the number of seeds developed after fertilization and the length of the silique [1]. Current models for fruit set or fruit initiation are based on data suggesting that seeds produce auxin and GA after fertilization, which promotes the growth of the pollinated fruit [1]. This process can be mimicked by application of any of the hormones on the fruit in the absence of pollination, resulting in the formation of seedless (or parthenocarpic [fruit formed without fertilization]) fruit [37]. Therefore, following fertilization, seeds are a source of auxin and auxin is required for the growth of the fruit. Recent publications demonstrated that seed-produced auxin is of importance for the development and growth coordination of the three structures contained in the seed: embryo, endosperm, seed coat [14,15,17,38]. This recent knowledge about inter-tissular communication within the seed and the fruit will be discussed below.

Auxin Movement within the Integuments and Funiculus
Several research groups observed that fertilization of the ovule triggers an increase in auxin levels in the integuments as monitored by the auxin input reporter R2D2 and by analytic quantification [17,38], and the activation of auxin signaling as visualized by DR5-based markers [1,15,17]. Altogether these observations suggest that auxin production increases in ovule integuments following fertilization. Expression pattern analysis of seeds expressing DR5-based reporters [1,15,17] identified that auxin signaling is activated in two distinct regions of the seed integuments, at the micropyle where the embryo connects to the integuments and in the chalazal domain, where the seed is attached via the funiculus to the fruit. Besides physically attaching the seed to the silique, the funiculus plays a role of conduit between these two organs, transporting in both directions hormones, nutrients and sugars. The application of N-1-naphthylphthalamic acid (NPA), a chemical that blocks auxin transport, mimics the fertilization-induced DR5 signals [1]. The DR5 signal at the chalazal region and funiculus overlaps with the vasculature, suggesting that auxin (or auxin-derived signal) might be transported from the ovule to the fruit after pollination [1,38]. Larsson et al. (2017) [38] compared the expression pattern of genes involved in auxin biosynthesis (YUCs) and auxin transport (PINs) at different female gametophyte (FG) developmental stages (FG5-7, according to [30]) and during early seed development. The authors observed that (1) auxin accumulation at the chalazal region and funiculus marks vascular precursor cells in ovules at pre-anthesis, (2) an anther-dependent signal reduces polar localization of PIN proteins in the funiculus to limit auxin transport through the funiculus in ovules at anthesis, and (3) xylem tracheary element cell file is extended through the funiculus, and PIN-dependent auxin transport is still restricted after fertilization of the ovule. However, the increase in auxin levels in the integuments following fertilization does not appear to be due to changes in YUC expression [38] but rather to enhanced TAA1 expression levels [17]. Also, the PIN3 expression domain extends within the integuments following fertilization. Other auxin transport proteins (ABC/PGP1 ABCB/PGP19, AUX1, LAX1) are also expressed in this sporophytic tissue [17,39,40]. Together with the restriction of auxin flow through the funiculus, these could contribute to the higher auxin levels in the integuments following fertilization [17,38]. The biological relevance of these dynamic changes in auxin distribution is that auxin would be a trigger for the formation of the vascular strands within the funiculus, and the synchronous development of the ovule/seed and the gynoecium/fruit, in order to avoid the formation of parthenocarpic fruits.

Auxin Movement from the Endosperm to the Integuments
The initiation of seed development is controlled by epigenetic regulators of the Polycomb group (PcG) family. PcG proteins block the development of the endosperm in the absence of fertilization, by targeting repressive trimethylation on lysine 27 of histone H3 (H3K27me3) at target loci [41]. For female gametophyte and endosperm development, the involved PcG complex is . The FIS-PRC2 complex is repressing the development of the endosperm prior to fertilization in order to block the formation of fertilization-independent seeds, containing an endosperm but no embryo [41].
The division of the central cell nuclei, triggered by an increase in auxin levels after fertilization, marks the initiation of the endosperm development. Two YUC genes are expressed in the endosperm, YUC10 and YUC11. The latter is also present in the central cell before fertilization, co-expressed with one of the auxin-conjugating enzymes GRETCHEN HAGEN3 (GH3.5) [16,38]. Figueiredo et al. (2015) [14] showed that FIS-PRC2 represses the expression of the maternal YUC10 copy in the central cell before fertilization. The paternal YUC10 copy brought by the pollen sperm cell is expressed in the fertilized central cell and is necessary for the initiation of the endosperm proliferation. It contributes to the increase in auxin levels in the endosperm as monitored by the R2D2 reporter. In ovules of mutants lacking the FIS-PRC2 function, YUC10 expression is de-repressed, resulting in an ectopic auxin production (monitored by the R2D2 reporter line) in the central cell without fertilization [14]. Because a fertilization-dependent increase of auxin levels in the central cell is necessary for the proliferation of the endosperm, these observations would explain the autonomous endosperm development in fis2 and fie seeds. Furthermore, the authors identified the MADS-box transcription factor AGAMOUS-LIKE 62 (AGL62) as a signaling component required for this effect. AGL62 is expressed in the central cell before fertilization and in the endosperm.
Sporophytic-active PRC2 complexes also repress seed coat development before fertilization. A fertilization-derived signal activates seed coat formation by releasing the PRC2 repressing action [41]. It has been demonstrated that auxin is this signal, produced post-fertilization in the endosperm by YUC10, channeled out from the endosperm to the seed coat by AGL62-regulated ABCB/PGP10 auxin efflux proteins [14,15]. Indeed, some seeds (<30%) of mutants in auxin production (wei8/− tar1/− tar2/+), but not in auxin signaling (axr1/+ axl1/−), are smaller in size, indicating a defect in integument cell expansion. Accordingly, ectopic expression of TAA1 and YUC6 in the central cell, prior fertilization, triggers the development of a seed coat. The seeds of agl62 mutant abort 3 to 4 Days After Pollination (DAP) probably due to an early endosperm cellularization, hypothesized to be the consequence of an absence of development of a seed coat. Integuments of agl62 seeds are characterized by the absence of auxin and GA signaling responses. The activation of the DR5 promoter in agl62 endosperm would suggest that auxin is trapped in the mutant endosperm, consistent with AGL62 being a transcriptional activator of ABCB/PGP10 expression in the endosperm, and the auxin transport function of ABCB/PGP10 from the endosperm into the integuments [15]. Work from the Köhler lab initiated the characterization of the molecular components involved in the synchronization of the seed coat differentiation with the development of the endosperm following fertilization. They show that it involves the epigenetic regulation of the production and the movement of auxin from the endosperm to the integuments.

Auxin Movement from the Integuments to the Embryo
Another auxin communication flow happens shortly after fertilization between the cells at the micropyle domain and the early embryo. Above we read that auxin level increases in the integuments after fertilization [1,14,17,38]. Robert et al. (2018) [17] observed that TAA1 expression levels are enhanced in the micropyle region after fertilization, likely contributing to the enhanced auxin levels. Indeed, the presence of DR5-derived signals and the increased levels in auxin metabolites, quantified in fertilized wild-type ovules, are absent in fertilized wei8 tar1 mutant seeds. Embryos growing in seeds with reduced auxin levels within the integuments (e.g., wei8, wei8 tar1, pBAN::iaaL -a bacterial enzyme degrading auxin, expressed from the BANYULS (BAN) promoter in the integuments) display morphogenic phenotypes characterized by altered cell division patterns. TAA1 is not embryonically expressed at this stage. Noteworthy embryos from seeds with reduced auxin signaling in the integuments (pBAN::BDL, auxin-resistant version of aux/IAA12-BODENLOSS gene expressed under BAN promoter) are unimpaired despite the absence of a DR5 signal in the micropyle domain. These data, together with reciprocal backcross experiments between wild-type plants and mutant plants with reduced auxin levels, show that the auxin required for establishing a body axis in early embryos is sourced in the micropyle cells upon fertilization [17]. How auxin is transported between sporophytic and embryonic tissues, remain elusive. Expression pattern analysis of several auxin transporter proteins (PINs, AUX1, LAX1, ABCB/PGP1 and ABCB/PGP19) shows the presence of these proteins in one or both structures, but no explicit demonstration of their involvement in this transport has been presented. AUX1 and LAX1 may contribute to the micropyle-suspensor auxin transport based on their cellular localization [17,39,40]. However, genetic redundancy among other members for the protein family and defects during female gametophytic development complicate the study of sporophytic-embryonic auxin transport. Furthermore, the positional communication between sporophytic tissues facing the embryo sac and the early embryo is conserved between monocotyledonous and dicotyledonous as very similar expression behavior of the DR5 reporter is observed in maize seeds [17].

Auxin Movement from the Endosperm to the Embryo
These studies report the presence of an auxin movement within the integuments, between the endosperm and the integuments after fertilization to promote seed coat development and between the integuments and the early embryo to contribute to the formation of an apical-basal embryonic axis development. Is there any evidence for auxin transport between the endosperm and the embryo? Growth coordination within the seed structures is essential for the viable development of the seed. Therefore, one would suspect auxin to be involved as a signaling molecule for a crosstalk communication between the endosperm and the embryo. AUX1, ABCB/PGP1 and ABCB/PGP19 auxin transport proteins are localized on zygotic and early embryonic membranes at the interface with the endosperm [17,39,40,42], indicative of a possible auxin transport between the endosperm and the embryo in Arabidopsis. Expression of YUCs at various developmental stages after fertilization indicates that auxin is produced in the endosperm [14] and embryos [16]. However, there is no concrete evidence that auxin would be transported from the endosperm to the embryo (or vice versa) in Arabidopsis.
In maize, auxin levels increase in the endosperm from 8 DAP and remain high until maturation (28 DAP) [43,44]. Auxin plays a positional role for the specification and the development of the aleurone, an outer cell layer of endosperm, separating the seed coat from the starchy endosperm [43,45]. Auxin also accumulates in the ESR (Embryo Surrounding Region) and the BETL (Basal Endosperm Transfer Layer) [43]. The BETL is a specialized endosperm region that facilitates nutrient uptake from the apoplast of the chalazal region. The ESR, as its name indicates, is the layer of endosperm around the embryo. Auxin is produced in maize endosperm, synthesized locally through the IPyA pathway [44]. Expression of ZmYUC1 and three ZmTAR genes were detected, correlating with auxin accumulations [44]. Endosperms of defective endosperm18 (de18) and defective kernel18 (dek18) knockout mutants for ZmYUC1 have a low auxin content and seed (endosperm and embryo) defect phenotypes [43,44,46]. ZmPIN1a-c expression follows the same pattern as ZmYUC1, e.g., accumulation in the endosperm following fertilization [43]. In particular, the BETL and the ESR contain high levels of ZmPIN1 proteins after fertilization until the maturation phase. In BETL, ZmPIN1 is localized at membranes facing sporophytic tissues, whereas, in ESR, ZmPIN1 accumulates in the cytoplasm of cells surrounding the embryo suspensor [43]. Additionally, ZmPIN1 is present in the (epidermal) L1 cell layer of the apical region of the embryo, suggesting a possible auxin flow from the endosperm to the embryo in this region [47]. Following this hypothesis, an auxin signaling is detected using a DR5 reporter in the maize endosperm, but not in the embryo, contrary to Arabidopsis. This auxin signaling, from the endosperm, may influence the embryonic morphogenesis development in maize [47]. Interestingly no auxin signaling (DR5) signal is observed in the ESR, where PIN1 proteins localize in the cytoplasm rather than at the membranes, which may help to prevent an auxin flow between the ESR and the suspensor cells during early seed development [47]. All together these patterns would create an auxin gradient between the endosperm, the apical embryonic domain and the base of the maize embryo, involved in the directional growth and patterning of the shoot apex of the maize embryo.
In summary, within the seed, three auxin dynamics between the seed structures can be identified and trigger three different developmental responses (Figure 1). In all three cases, auxin production is activated after seed fertilization. Accumulation of auxin in the chalazal region is implicated in the differentiation of the funiculus vascular strands. The second dynamism occurs between endosperm and seed coat. An epigenetic regulation signaling pathway activates auxin production in the endosperm and its transport from the endosperm to the integuments. This transport requires ABCB/PGP10 auxin efflux proteins in the endosperm, transcriptionally regulated by AGL62. Presence of auxin within the integuments initiate its differentiation into the seed coat. The last auxin movement occurs between the micropyle and the early embryo, for the formation of the embryo body axis. Auxin transport requires an intercellular transmembrane transport, relying on transmembrane proteins. Are all cells within the seeds connected and is there any alternative molecular transport means? activated after seed fertilization. Accumulation of auxin in the chalazal region is implicated in the differentiation of the funiculus vascular strands. The second dynamism occurs between endosperm and seed coat. An epigenetic regulation signaling pathway activates auxin production in the endosperm and its transport from the endosperm to the integuments. This transport requires ABCB/PGP10 auxin efflux proteins in the endosperm, transcriptionally regulated by AGL62. Presence of auxin within the integuments initiate its differentiation into the seed coat. The last auxin movement occurs between the micropyle and the early embryo, for the formation of the embryo body axis. Auxin transport requires an intercellular transmembrane transport, relying on transmembrane proteins. Are all cells within the seeds connected and is there any alternative molecular transport means?

Symplastic Transport, as an Alternative Route of Communication Within the Seed
Symplastic molecular movement is an alternative cell-to-cell transport to transcellular transport. Transcellular transport requires the movement of signaling molecules in and out the cell, and across the apoplast, as it is the case for auxin. Symplastic transport is a direct transport between the cytoplasm of two connected cells through a plant-specific structure called plasmodesmata [48]. A Figure 1. Auxin movement between the three seed structures after fertilization. Auxin production sites are symbolized in green. Auxin in the chalazal region promotes the specification of the vasculature in the funiculus (auxin sporophytic movement symbolized by the blue arrow). Auxin at the micropyle moves to the embryo to contribute to the formation of the embryo body axis. Auxin production in the endosperm is epigenetically repressed before fertilization by FIS-PRC2 (FERTILIZATION INDEPENDENT SEED-Polycomb Repressive Complex 2) complex (red line). This auxin moves to the integuments to contribute for the differentiation of the seed coat, through ABCB/PGP10 auxin efflux proteins. Auxin movement between different seed structures are symbolized in purple (endosperm-integuments, integuments-embryo). The expression of ABCB/PGP10 is dependent on AGL62 (green arrow). No regulated auxin movement between the endosperm and the embryo has been yet demonstrated (dotted purple arrow).

Symplastic Transport, as an Alternative Route of Communication within the Seed
Symplastic molecular movement is an alternative cell-to-cell transport to transcellular transport. Transcellular transport requires the movement of signaling molecules in and out the cell, and across the apoplast, as it is the case for auxin. Symplastic transport is a direct transport between the cytoplasm of two connected cells through a plant-specific structure called plasmodesmata [48]. A symplastic domain consists of a group of cells connected through plasmodesmata. There are several symplastic domains identified in seeds (Figure 2) [49]. Their number and size evolve during seed development. Notably, there is an absence of symplastic linkage between the seed coat and the embryo for the transport of phloem-delivered nutrients from the funiculus. Within the seed coat, three symplastic domains are identified: (1) the symplastic unloading domain at the end of the funiculus in the chalazal domain, linking the developing seed to the silique, (2) the outer integuments and (3) the inner integuments [49]. Until the globular stage, the embryo is one whole symplastic domain. At the globular stage, the symplastic connectivity is restricted between the suspensor and the proembryo, which is then separated into distinct embryonic domains [49]. The symplastic connectivity between the suspensor and the embryo allows the movement of small molecules, including sucrose, hormones and small proteins as BDL/IAA12 [49][50][51][52]. Three symplastic barriers are therefore defined: (1) inner/outer integuments, (2) inner integuments/endosperm, (3) endosperm/embryo. Transport across those symplastic barriers necessitates a carrier-mediated transport, such as the sucrose transporters (SUC or SUT) or the ABCB/PGP and PIN transporters. Moreover, the presence of these symplastic barriers between the sporophytic seed coat, the triploid endosperm and the diploid embryo prevents symplastic transport to be considered as communication means for coordinated development between those three structures.
The symplastic barrier between the embryo and the endosperm is formed after deposition of a cuticle outside the proembryo around globular stage [53]. Because of the absence of a cuticle between the endosperm and the suspensor, the suspensor cells may be involved in a nutrient uptake via transmembrane transport [50]. Later during the development, suspensor cells undergo programmed cell death [54]. Therefore, after the torpedo stage, during seed maturation, uptake of nutrients may occur directly through the embryo epidermis from the endosperm, despite the presence of the cuticle membrane [54]. Outside the cuticle, at the embryo surface, is deposited an embryo sheath [55]. Involved in the organization and the integrity of the cuticle (but not its biogenesis) are peptides secreted by the endosperm: ESR-specific subtilisin protease ALE1 (ABNORMAL LEAF-SHAPE1) and embryonic epidermis-expressed receptor kinases GASSHO1 (GSO1) and GSO2 [53,55]. The genes involved in cuticle biogenesis are expressed as early as the mid-globular stage, after the formation of the protoderm [53]. The expression of these genes is GSO1-and GSO2-independent. The formation of the extra-cuticular sheath requires a signaling pathway involving the endosperm-produced peptide KERBEROS (KRS) in parallel of the ALE1/GSO1/GSO2 pathway [55]. Moreover, the endosperm-specific transcription factor ZHOUPI (ZOU) regulates the expression in the endosperm of both ALE1 and KRS [55]. The cuticle is initially deposited as patches to form a uniform layer later, resulting in the isolation of the embryo from its surrounding endosperm from early torpedo stage. As deduced from the krs mutant phenotypes the sheath appears to work as a lubricant for the growing movement of the embryo into the cellularized endosperm [55]. In an attempt to uncover downstream components of the ALE1-GSO1-GSO2 pathway, a transcriptomic approach identified a link of this pathway to genes involved in plant defence responses. By analogy, the authors studied the MAP-kinase MPK6 as a possible downstream embryonic component of the signaling pathway [53].
Symplastic transport and symplastic barriers create domains within the seed structures where molecular transport is facilitated. Furthermore, the cuticle is a clear example of endosperm-embryo cooperation for the formation of a symplastic barrier between the two structures ( Figure 2). Further studies would determine the role of this communication means for the growth coordination of the embryo, endosperm and seed coat. Symplastic barriers in the seed are illustrated (red): inner/outer integuments, inner integuments/endosperm, endosperm/embryo (cuticle). Blue arrows indicated the sucrose flow in the seed, deduced from feeding experiments in oilseed rape [56]. The expression pattern of SWEET12 (micropyle and suspensor) and SWEET15 (seed coat) is indicated in green [57]. The expression pattern of AtSUC5 in ESR is shown in purple [58].

Movement of Sucrose Within the Seed, Another Example of Molecular Communication
Sucrose is a necessary nutrient for embryo and seed development. Inflorescences, and seeds, in particular, are major carbon sinks from sucrose produced in mature leaves [59,60]. Sucrose is a sugar transported on long distance from maternal tissues, via the funicular phloem, through the seed coat and the endosperm to the embryo (Figure 2). Feeding experiment in oilseed rape identified the flow of sucrose in seeds from the integuments to the embryo via the ESR, and to the central endosperm via the chalazal endosperm [56]. It requires the help of plasma membrane sucrose transporters (SUT or SUC) and sucrose exporter (SWEET) [61,62]. In the endosperm, the sucrose is converted into hexoses (glucose and fructose) [56]. The hexose/sucrose ratio is high in the endosperm and will influence the sugar movement from maternal tissues to the seed coat and ultimately to endosperm and embryo. This sucrose flow to the embryo is crucial for seed size and viability [54,59]. A reduction in the maternal sucrose flow to the embryo by mutations in the SWEETs and (endosperm expressed) AtSUC5 induces a delay in the embryo development and a reduction in embryo and seed size, and seed weight [57,58]. The hexose concentration gradient between endosperm and embryo is in favor of endosperm nuclear division over zygote division in the initial developmental phase following fertilization [63,64]. Evidence of crosstalk between auxin and sucrose in the balance between cell elongation and cell division for seed development have been discussed by Wang and Ruan (2013) [64].
Endosperm cellularization starts from micropyle progressing towards the chalazal region after the 8th mitotic division (heart stage). This cellularization reduces the size of the endosperm vacuole, main storage pool for hexoses in the seed [56]. Therefore, a decrease of the vacuole size by cellularization decreases hexose levels in the endosperm, and thus the sink strength between the embryo and the endosperm. Indeed, endosperm cellularization correlates with a decrease in the hexose/sucrose ratio [65]. Several mutants affected in endosperm cellularization also display an arrest of embryonic development [66]. This is the case of fis2. This repressive FIS-PRC2 complex is essential Figure 2. Symplastic barriers in the seed are illustrated (red): inner/outer integuments, inner integuments/endosperm, endosperm/embryo (cuticle). Blue arrows indicated the sucrose flow in the seed, deduced from feeding experiments in oilseed rape [56]. The expression pattern of SWEET12 (micropyle and suspensor) and SWEET15 (seed coat) is indicated in green [57]. The expression pattern of AtSUC5 in ESR is shown in purple [58].

Movement of Sucrose within the Seed, Another Example of Molecular Communication
Sucrose is a necessary nutrient for embryo and seed development. Inflorescences, and seeds, in particular, are major carbon sinks from sucrose produced in mature leaves [59,60]. Sucrose is a sugar transported on long distance from maternal tissues, via the funicular phloem, through the seed coat and the endosperm to the embryo (Figure 2). Feeding experiment in oilseed rape identified the flow of sucrose in seeds from the integuments to the embryo via the ESR, and to the central endosperm via the chalazal endosperm [56]. It requires the help of plasma membrane sucrose transporters (SUT or SUC) and sucrose exporter (SWEET) [61,62]. In the endosperm, the sucrose is converted into hexoses (glucose and fructose) [56]. The hexose/sucrose ratio is high in the endosperm and will influence the sugar movement from maternal tissues to the seed coat and ultimately to endosperm and embryo. This sucrose flow to the embryo is crucial for seed size and viability [54,59]. A reduction in the maternal sucrose flow to the embryo by mutations in the SWEETs and (endosperm expressed) AtSUC5 induces a delay in the embryo development and a reduction in embryo and seed size, and seed weight [57,58]. The hexose concentration gradient between endosperm and embryo is in favor of endosperm nuclear division over zygote division in the initial developmental phase following fertilization [63,64]. Evidence of crosstalk between auxin and sucrose in the balance between cell elongation and cell division for seed development have been discussed by Wang and Ruan (2013) [64].
Endosperm cellularization starts from micropyle progressing towards the chalazal region after the 8th mitotic division (heart stage). This cellularization reduces the size of the endosperm vacuole, main storage pool for hexoses in the seed [56]. Therefore, a decrease of the vacuole size by cellularization decreases hexose levels in the endosperm, and thus the sink strength between the embryo and the endosperm. Indeed, endosperm cellularization correlates with a decrease in the hexose/sucrose ratio [65]. Several mutants affected in endosperm cellularization also display an arrest of embryonic development [66]. This is the case of fis2. This repressive FIS-PRC2 complex is essential for suppressing seed development in the absence of fertilization, as discussed above. Loss of FIS2 causes endosperm proliferation and seed abortion. In fis2, the absence of endosperm cellularization results in high hexose levels and an absence of sucrose transfer to the embryo, leading to its developmental arrest. The absence of AGL62, downstream signaling component of the FIS2 pathway, leads to early endosperm cellularization. Indeed, reducing the expression levels of AGL62 in the endosperm rescues fis2 endosperm phenotypes. In the fis2 agl62 double mutant, embryo development is delayed compared to wild-type embryos, correlating with a delayed endosperm cellularization and a reduced hexose content compared to fis2 seeds [66]. The fis2 endosperm phenotypes show the importance of endosperm cellularization for its role as a nutrient (hexose) provider for embryo growth. This is supported by the retarded embryonic growth observed in endosperm-expressed sweet mutants, impaired in sucrose transport from the endosperm to the embryo [57,66]. No direct links were so far identified between SWEET and AGL62. However, the function of FIS-PRC2 and AGL62 signaling pathway during endosperm development associates post-fertilization endosperm initiation and auxin production (for seed coat differentiation) with endosperm cellularization and endosperm-to-embryo flow of sucrose (for embryo growth).

Seed to Fruit Communication: Hormonal Crosstalk for Fruit Initiation
Coordinated seed growth alone is not enough for successful reproduction. It requires a synchronized growth with the fruit (or silique). For example, ectopic auxin production in the central cell induces fruit parthenocarpy and links ovule fertilization to fruit development [15]. Several lines of evidence suggest that fertilization-dependent auxin production and signaling in the seeds activates GA production and signaling for fruit initiation [1,[67][68][69][70]. This fertilization-dependent crosstalk is mimicked by auxin application, whereas GA application does not have any effects on auxin signaling [15]. Additionally, auxin effects on fruit initiation require unimpaired GA production and signaling pathways in Arabidopsis [70,71]. Expression analysis by RT-qPCR performed on dissected carpel valves and in ovules/seeds at anthesis and post-anthesis in unpollinated and pollinated pistils demonstrated that genes involved in GA biosynthesis are upregulated exclusively in the fertilized ovules, but not in the carpels. Validating this observation is the upregulation of GA biosynthetic genes in auxin-treated unpollinated pistils [1]. The binding of GA to its receptor, GID1 (GIBBERELLIN INSENSITIVE DWARF1) activates a GA signaling pathway involving the degradation of the transcriptional repressor DELLA proteins [72,73]. Mutant combinations in multiple DELLA proteins mimic an excess of GA, auto-activate GA responses and produce parthenocarpic fruits [70]. The DELLA protein RGA (REPRESSOR OF GA1-3) is mainly present in ovules, and weakly in carpel valves. The degradation of the RGA signals in both tissues by pollination or auxin treatments implies the activation of the GA signaling pathway in both ovules and carpel valves [1]. Alterations in GA signaling or production in tomato and Arabidopsis trigger similar results [1,70,74]. In tomato, direct crosstalk between auxin and GA has been uncovered with the interaction of SlARF7 with both SlDELLA and SlIAA9 [74]. This dual interaction antagonistically regulates the expression of genes involved in GA and auxin metabolism and synergistically regulates the expression of genes involved in growth, such as EXPANSIN5 and the ethylene production gene ACC OXIDASE4 [74]. In Arabidopsis, tomato and eggplant, downregulation of ARF7 and ARF8 proteins, by RNA interference or loss-of-function mutations, results in parthenocarpic fruits [74][75][76][77], suggesting that the IAA9/ARF7 auxin signaling pathway represses fruit growth in the absence of ovules fertilization by repressing EXPANSIN5 expression. GA (or GA-derived signal) is, therefore, a good candidate for a molecular communication component between fertilized ovules and carpel valves to promote and coordinate fruit growth and seed development [1].

Conclusions
In this review, I discussed recent advancements in our knowledge on inter-tissular molecular communication between the three seed structures (seed coat, endosperm, embryo) and the fruit. The seed is compartmentalized in symplastic domains, that isolate the three seed structures from each other's and impose a controlled transmembrane transport for communication between two symplastic domains. I emphasize the relevant role of auxin as a signaling molecule and its regulated transport between these three structures. Also, sucrose, as nutrients, is another example of small molecules involved in the communication between the seed structures. Altogether, hormones and nutrients are critical molecular components for the coordination of growth and development of the seeds and the fruit. Acknowledgments: I apologize to those colleagues whose work was not included here, due to space constraints.

Conflicts of Interest:
The author declares no conflict of interest. The funders had no role in the writing of the manuscript, or in the decision to publish the results.  /SUT SUCROSE TRANSPORTER  TAA1  TRYPTOPHAN AMINOTRANSFERASE OF ARABIDOPSIS  TAR  TAA1-related  TIR1  TRANSPORT INHIBITOR RESISTANT  Trp  tryptophan  WEI8  WEAK ETHYLENE INSENSITIVE8  YUC  YUCCA  ZOU  ZHOUPI