Seed development in angiosperms demands the tightly coordinated development of three genetically distinct structures. The embryo is surrounded by the endosperm, which is in turn enclosed within the maternally derived seed coat. In Arabidopsis, final seed size is determined by early expansion of the coenocytic endosperm, which then cellularises and subsequently undergoes developmental programmed cell death, breaking down as the embryo grows. Endosperm breakdown requires the endosperm-specific basic helix-loop-helix transcription factor ZHOUPI. However, to date, the mechanism underlying the Arabidopsis endosperm breakdown process has not been elucidated. Here, we provide evidence that ZHOUPI does not induce the developmental programmed cell death of the endosperm directly. Instead ZHOUPI indirectly triggers cell death by regulating the expression of cell wall-modifying enzymes, thus altering the physical properties of the endosperm to condition a mechanical environment permitting the compression of the cellularised endosperm by the developing embryo.
The ‘Russian doll-like’ organisation of the angiosperm seed coat, endosperm and embryo implies that growth in one compartment must have direct consequences for neighbouring tissues. In Arabidopsis, growth of the expanding coenocytic endosperm during early post-fertilisation development drives seed expansion, which is in turn controlled by the seed coat in order to achieve a genetically determined final seed size and shape (Garcia et al., 2005, 2003; Ingram, 2010). More recently, it has been shown that seed coat expansion is regulated by a specific cell layer, the adaxial epidermis of the outer integument, at least in part in response to mechanical tension imposed by the growing endosperm (Creff et al., 2015).
After the initial phase of rapid expansion, the endosperm cellularises; a process that initiates in the micropylar zone surrounding the developing embryo and progresses towards the chalazal pole of the seed (Sørensen et al., 2002). Embryo growth, and a poorly characterised concurrent process involving progressive endosperm breakdown in the zone surrounding the growing embryo, closely follow cellularisation. In mature Arabidopsis seeds, only a single specialised layer of cellularised endosperm remains surrounding the mature embryo. Embryo size in Arabidopsis is thus strongly influenced by the size of the endosperm prior to breakdown. This relationship is dramatically altered in zhoupi (zou) mutants, in which endosperm breakdown does not occur. ZOU encodes a unique basic helix-loop-helix (bHLH) transcription factor that is expressed exclusively in the developing endosperm and acts as a heterodimer with another bHLH protein, ICE1, to mediate endosperm breakdown (Denay et al., 2014; Kondou et al., 2008; Xing et al., 2013; Yang et al., 2008). In zou mutants, the presence of a persistent endosperm has consequences both for embryo development and for the testa. Embryo growth is dramatically reduced in zou mutants, owing to an apparent inability of the embryo to expand into the persistent endosperm (Yang et al., 2008). The idea that the embryo is physically constrained in this background is supported by the fact that the testa in zou mutants is under greater tension than that in wild-type plants after endosperm cellularisation (Creff et al., 2015), suggesting that the expanding embryo and the abnormally persistent endosperm compete for space within the seed cavity.
The mechanism underlying endosperm breakdown remains very poorly understood. The genetically controlled elimination of unwanted cells is a common occurrence during both animal and plant development. The term developmental programmed cell death (dPCD) has been used to describe such processes (Olvera-Carrillo et al., 2015). Although in animals, the molecular control of dPCD pathways is well characterised and relatively conserved (recently reviewed by Suzanne and Steller, 2013), almost every reported instance of plant dPCD seems to involve unique molecular players, with the triggers of plant dPCD being particularly diverse (recently reviewed by Van Hautegem et al., 2015). Interestingly, however, a conserved set of indicator genes expressed prior to multiple plant dPCD processes has recently been defined (Olvera-Carrillo et al., 2015). These include the aspartate protease-encoding PASPA3 gene, which has no known function, but is a very early marker of cells destined for dPCD, and the bifunctional nuclease-encoding BFN1 gene, expression of which has been shown to pave the way for nuclear corpse clearance during lateral root cap cell death (Fendrych et al., 2014; Van Durme and Nowack, 2016). Here, we have combined biophysical and compositional analysis with expression analysis of both of these pre-dPCD markers and direct ZOU targets, to investigate the processes involved in the breakdown of the Arabidopsis endosperm.
Cell death markers show ZOU-dependent expression in the developing endosperm during seed development
Cell death in the developing Arabidopsis seed is not restricted to the endosperm, and is also known to occur in the developing seed coat (Andeme Ondzighi et al., 2008; Nakaune et al., 2005) and the embryonic suspensor (Blanvillain et al., 2011). To identify cell death markers with relative specificity for the endosperm, we therefore interrogated available in silico resources and the literature. We identified two genes expressed prior to cell death in the lateral root cap as potentially useful pre-cell death markers in endosperm: PASPA3 and BFN1 (Olvera-Carrillo et al., 2015; Fendrych et al., 2014). In silico expression profiles (Le et al., 2010; Winter et al., 2007) for these genes are shown in Fig. S1. We characterised the expression of these genes during seed development by in situ hybridisation and found that their expression profiles closely matched those shown in available in silico and published data. PASPA3 expression was detected in the endosperm from the late heart stage (Fig. 1A, first three panels) whereas BFN1 expression was first detected only from the late torpedo stage onwards (Fig. 1A shows expression at the bent cotyledon stage). We then analysed the expression of PASPA3 and BFN1 in zou-4 seeds, and found that expression of both genes was strongly reduced (Fig. 1A). This reduction was confirmed by Q-RT-PCR analysis of whole siliques from wild-type plants and homozygous zou-4 mutants (Fig. 1B). It should be noted that both PASPA3 and BFN1 also show expression in the testa (Fig. S1), which might explain residual expression in Q-RT-PCR experiments. The developing Arabidopsis endosperm thus shows ZOU-dependent expression of both an early and a late pre-dPCD marker.
ZOU activity leads to cell wall modifications in the developing endosperm
We previously identified a set of genes strongly downregulated in zou-4 mutants at the early heart stage and early torpedo stages of embryo development (Xing et al., 2013). Interestingly, none of the genes identified in this analysis as strongly downregulated (>10×) at the heart stage was annotated as being implicated in cell death, whereas several of the most strongly downregulated genes were annotated as potentially involved in the modification of cell wall proteins and polysaccharides. We have previously shown that one of these genes, RGP3, encoding a member of a small protein family shown involved in plant cell wall biosynthesis through the metabolism of arabinose (Rautengarten et al., 2011), is a direct target of activation by ZOU (Denay et al., 2014). We confirmed the ZOU-dependent expression of five more strongly regulated genes by Q-RT-PCR (Fig. 2), and confirmed their expression patterns in the developing endosperm by in situ hybridisation (Fig. S2). Downregulation of these genes in zou-4 mutants could already be detected at the early heart stage of development (Fig. 2). To compare the relative spatiotemporal expression pattern of a direct ZOU target (RGP3) and the earliest pre-dPCD marker, PASPA3, we undertook an analysis using serial sections of the same seed, probed with either an RGP3 or a PASPA3 probe. Convincing signals were first observed for RGP3 expression at the early heart stage, whereas PASPA3 transcript levels were only detected at the late heart/early torpedo stages (Fig. 2).
In light of the regulation of cell wall modifier-encoding genes by ZOU, we explored cell wall composition in the endosperm of zou-4 mutant and wild-type seeds using antibodies against a variety of cell wall epitopes. These experiments showed that (1-5)-α-L-arabinan epitopes, labelled with the LM6 antibody (Willats et al., 1998), were more abundant in the endosperm of zou-4 mutants than that of wild-type embryos. In particular, the relative staining with LM6 in the endosperm immediately adjacent to the embryo compared with that in more chalazal regions is considerably stronger in zou mutants compared with wild type, and in later stages translates as a delineation of the embryo with LM6 signal, which is not observed in wild-type seeds (Fig. 2).
The endosperm of zou mutants is physically stiffer than that of wild-type seeds post-cellularisation
In a previous study, we showed that the presence of a persistent endosperm in zou-4 mutants leads to an abnormal increase in seed size post-endosperm-cellularisation, and causes increased tension in the developing seed coat (Creff et al., 2015). Both observations suggest that the mechanical properties of the endosperm are altered in zou-4 mutants. To investigate this, we measured the apparent stiffness of developing seeds during development using a nano-indenter system. This equipment allows the measurement of the force necessary to carry out tissue indentations of known amplitude using a geometrically defined probe. We carried out 30 µm indentations of immobilised seeds using a flat, circular probe with a diameter of 100 µm as described by Beauzamy et al. (2016). Slopes of force-displacement curves for the extend- and retract-phases of indentation are shown in Fig. 3 and Fig. S3, respectively (methodology described in Beauzamy et al., 2016).
Indentations were carried out on staged seeds from wild-type and zou-4 mutant plants from the onset of endosperm cellularisation (heart stage) to bent-cotyledon stage. At the early heart stage of development, we found no difference in the apparent stiffness of wild-type and zou-4 mutant seeds. However, at the early torpedo stage, when embryo elongation and endosperm breakdown is initiated in wild-type seeds, we found that the seeds of zou-4 mutants were up to three times as stiff as those of wild-type plants at the same developmental stage. Plasmolysis of seeds significantly reduced the difference in stiffness between the two genotypes, indicating that this difference can be attributed to increased endosperm turgor, consistent with previous indentation experiments (Creff et al., 2015). The lower stiffness of plasmolysed seeds of zou-4 mutants at the latest stage can be ascribed to arrested embryo growth in this background.
Endosperm breakdown requires embryo growth
Our observation that endosperm turgidity increases in the zou-4 mutant seed, combined with the observation that regulation of cell wall composition, rather than cell death, appears to be the primary function of ZOU, led us to ask whether endosperm death could also be dependent upon physical crushing/bursting of endosperm cells by the expanding embryo during wild-type seed development. To explore this possibility, we investigated the morphology of the endosperm in mutants in which embryo development arrests early, but endosperm growth/cellularisation has not been described to be abnormal. In the first instance, we chose two mutant backgrounds. The first is homozygous for dek1-3, a null allele of the DEFECTIVE KERNEL 1 gene in which embryo development arrests at the globular stage, but endosperm proliferation and cellularisation occur normally (Johnson et al., 2005; Lid et al., 2005). Because dek1 mutants have been shown to have a partially disrupted organisation of the outer endosperm cell layer (Lid et al., 2005), we also investigated a line homozygous for the null allele of homeodomain protein-encoding gene ATML1 (atml1-3), and segregating a null allele of the closely related PDF2 gene (pdf2-2). Double atml1-3 pdf2-2 mutants again arrest at the globular stage of development with no reported defects in endosperm development (San-Bento et al., 2014). For both backgrounds, we fixed and resin-embedded seed populations from single self-fertilised siliques at a late developmental stage when seeds containing either a dek1-3 mutant or an atml1-3 pdf2-2 zygotic compartment could be easily distinguished, but before seeds started to desiccate (at which point seeds with a mutant zygotic complement abort in both genotypes). In both backgrounds, in phenotypically wild-type seeds, the endosperm had been eliminated. However, in each case, when a seed containing an arrested embryo was sectioned, the endosperm was intact, although cells had a slightly rounded aspect as if they had separated (Fig. 4; Fig. S4).
To eliminate the possibility that ZOU is not expressed in mutants in which embryo development is abnormal, we analysed the expression of ZOU, and the direct ZOU target gene RGP3 in seeds containing a dek1-3 zygotic compartment, and in phenotypically wild-type siblings, by in situ hybridisation. We found that both genes were expressed in the endosperm of seeds containing mutant embryos. Finally, we visually compared the endosperm phenotypes of seeds containing a dek1-3 zygotic compartment in either a ZOU+ or a zou− mutant background. We found that the endosperm cell walls of seeds containing a dek1-3 zygotic compartment in a ZOU+ background resembled those of wild-type seeds undergoing endosperm breakdown, in that they were relatively weakly stained with Toluidine Blue and additionally showed evidence of cell wall separation (Fig. 4). A similar phenotype is observed in atml1-3 pdf2-2 endosperm (Fig. S4). By contrast, the endosperm cell walls of seeds with a zou-4 or a dek1-3 zou-4 zygotic compartment looked visually more robust, were more strongly stained, and showed no signs of cell separation.
Interestingly, we found that in siliques segregating for dek1-3 seeds, by the bent torpedo stage of embryo development, the endosperm of seeds with a dek1-3 zygotic compartment showed a strong, uniform expression of both PASPA3 and BFN1, suggesting that the expression of these genes may be triggered in the dek1-3 endosperm independently of the imposition of mechanical stress by the embryo (Fig. S4).
Our results strongly support the hypothesis that the loss of endosperm cells in the embryo-surrounding endosperm is a process dependent upon alterations in the biochemical and physical properties of endosperm cell walls, which permit the growing embryo to expand and exert physical stresses on endosperm cells. Our analysis of pre-cell-death marker expression suggests that these physical stresses combined with embryo growth could be a trigger for a dPCD process. This does not occur in zou mutants owing to loss of endosperm cell wall modifications. Consistent with this idea, our indentation and plasmolysis experiments, taken together with our analyses of endosperm cell wall structure and composition suggest that the cell wall modifications mediated by ZOU may affect the capacity of endosperm cells to resist an increased turgor pressure caused by endosperm compression by the growing embryo. We propose that in wild-type seeds the function of ZOU may be to render endosperm cell walls fragile enough to allow deformation, physical stress, and ultimately bursting upon compression by the growing embryo. In zou mutants, the presence of more robust cell walls allows endosperm cells to remain intact and unstressed in the face of these compressive forces. In mutant seeds, the maintenance of (1-5)-α-L-arabinan epitopes, which have previously been detected in the endosperm of Arabidopsis and tobacco, and shown to be most likely associated with rhamnogalacturonan-1 pectins in these tissues (Willats et al., 2001; Lee et al., 2012, 2013), suggests that ZOU could act to remove or modify pectins in endosperm cell walls.
Our analysis of the dek1-3 mutant indicates that the expression of ZOU and ZOU-dependent genes in the endosperm is not dependent upon embryo growth. In addition, ZOU-dependent endosperm cell wall thinning appears to occur normally in seeds containing a dek1-3 zygotic compartment. ZOU-dependent endosperm modifications are thus likely to be an autonomous feature of endosperm development, although an influence from arrested embryos cannot be excluded. Intriguingly, we show that the expression of known pre-cell-death markers in the endosperm, which is absent in the zou-4 mutant, is not lost in seeds containing a dek1-3 zygotic compartment. ZOU-mediated cell wall modifications may therefore impose a physiological stress upon endosperm cells, which ultimately leads to the expression of these markers even in the absence of embryo-mediated compression. The timing of this expression in comparison with that in wild-type siblings was difficult to ascertain and it could therefore be an early consequence of the onset of abortion. However, the fact that the cells in dek1-3 endosperms are capable of active gene expression indicates that they are still alive at the late-torpedo stage, when much of the endosperm in sibling seeds has been eliminated, underlining the requirement for physical stresses imposed by the embryo in cell elimination.
Cell wall weakening and subsequent cell rupture due to the behaviour of neighbouring cells may be a common feature involved in sensitising or conditioning plant cells for dPCD during cell elimination. For example, death in the lateral root cap (lrc) cells is preceded by cell extension driven by the expansion of underlying tissues (Fendrych et al., 2014). Sensitivity to this extension is conditioned by expression of the transcription factor SOMBRERO (Fendrych et al., 2014), in a mechanism that could be functionally similar to that mediated by ZOU. More detailed biophysical analysis as well as detailed cell structure analysis will help to clarify whether molecular pathways are shared between these processes and with other dPCD events in plants, but may be hampered by the relative inaccessibility of the developing endosperm.
MATERIALS AND METHODS
All genotypes used in this work have been previously described and published. Seeds were plated on Murashige and Skoog (MS) media, vernalised for 3 days at 4°C, germinated under short day conditions (8 h light) at 18°C. Plantlets were transferred to soil in identical growth room conditions for 3 weeks and finally placed under continuous light at 16°C. To ensure synchronicity between plants, flowers were labelled and dated at anthesis.
Resin embedding and immunolocalisation experiments
In situ hybridisation experiments
RNA extraction and Q-RT-PCR experiments
Nano indentation of developing seeds and analysis of indentation curves
Indentation experiments and statistical analysis were carried out using a TI 950 TriboIndenter (Hysitron) exactly as described by Beauzamy et al. (2016). Slopes were taken from the region of the extend force-displacement curve ranging from 75 to 100% of the maximum force.
We would like to thank Nelly Dubrulle for help with statistical analysis, and the plant culture, logistics and secretarial teams at the RDP (ENS de Lyon) for their support.
L.B., C.F., S.C. and A.C. carried out experiments, analysed results and prepared figures. All authors participated in experimental design and manuscript preparation. G.I. planned and directed the project.
This work was funded by a fellowship from AgreenSkills (CESETAB project) and Institut National de la Recherche Agronomique (to C.F.); a ‘Chaire d'excellence’ from l’Agence Nationale de la Recherche, France [ANR-10-CHEX-0011: mécanograine to G.I.]; and a European Research Council Starting Grant [Phymorph #307387 to A.B.].
The authors declare no competing or financial interests.