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Mosaic analyses using marked activation and deletion clones dissect Arabidopsis SCARECROW action in asymmetric cell division

Department of Molecular Cell Biology, Utrecht University, 3584 CH Utrecht, The Netherlands

	Abstract

Top Abstract Results and Discussion Materials and methods Acknowledgments References

 
In the Arabidopsis root meristem, ground tissue stem cell daughters perform an asymmetric division to form endodermis and cortex. The putative transcription factors SCARECROW (SCR) and SHORTROOT (SHR) regulate this radial patterning event, and the mixed cell fate in scr mutants suggests an atypical role of the SCR gene in asymmetric cell division. Here we use a newly developed site-specific gene activation/deletion system in which induced clones are positively marked with green fluorescent protein (GFP). Using this system, we show that SCR acts cell-autonomously to control asymmetric cell division within the ground tissue. We provide evidence that SCR gene expression is under autoregulatory control, that SCR limits SHR movement, and that transient SCR action is sufficient to separate endodermis and cortex fates by asymmetric cell division.

[Keywords: Asymmetric cell division; CRE/lox; meristem; pattern formation]

Received April 13, 2004; revised version accepted June 17, 2004.

View larger version (60K): [in this window] [in a new window]   Figure 1. Site-specific SCR gene activation and deletion to investigate alternative possibilities for SCR function in asymmetric division. (a) Schematic representation of cell types present in the Arabidopsis root meristem. Radially organized are the stele (St), endodermis (En), cortex (Cor), epidermis (Epi), and lateral root cap (Lrc). In the proximal-distal plane, quiescent center (QC) and columella (Col). (gtsc) Ground tissue stem cell; (scd) stem cell daughter. (b) Possibilities for SCR function in establishing asymmetry during periclinal ground tissue cell division. SCR is required for the execution of the periclinal division (1,2,3). (1) SCR and SHR are required to maintain endodermis fate; C determines cortex fate. (2) SCR plays no part in division asymmetry, only external factors determine endodermal and cortex fate. (3) During periclinal division, SCR separates endodermis and cortex fates. (c) Two possible signaling pathways allowing periclinal cell division in the ground tissue stem cell daughters. (1) Mature cells act as a patterning template and reinforce periclinal cell division. (2) QC signaling prevents differentiation and periclinal division in the stem cell. (d) Clonal SCR gene activation in scr-4 using vectors pCB1 and pG7HSCRE-USCR. Heat-shock activation of CRE recombinase mediates excision of the sequences between the direct repeat lox recombination sites. The 35S constitutive promoter then drives GAL4VP16 expression, resulting in transactivation of SCR expression and GFPER, thereby marking the cells with recombination events. (e) Clonal deletion of SCR using pCB1-SCR complemented scr-4 and pG7HSCRE. Heat-shock activation of CRE recombinase mediates excision of SCR, resulting in the 35S-driven GAL4VP16 and transactivation of GFPER expression, thereby marking the scr-4 mutant cells. Color-filled objects represent active promoters (green), transcribed genes (blue, green, orange, yellow), and terminators (red).

The role of SCR in the asymmetry of the periclinal ground tissue division and endodermis specification can be addressed by analyzing how cells respond shortly after local induction or elimination of SCR expression. Here we study the effects of clonal activation and deletion of the SCR gene. For this purpose, we have developed a CRE/lox-based site-specific recombination system consisting of two vectors, in which recombination events are positively marked with green fluorescent protein (GFP) expression. Our results demonstrate a transient role for SCR in initiating and stabilizing the asymmetry of cell division, as well as a role for SCR in restraining SHR movement, which represents a noncanonical mechanism for asymmetric cell division.

	Results and Discussion

Top Abstract Results and Discussion Materials and methods Acknowledgments References

 

Clonal activation reveals SCR involvement in division asymmetry

SCR induces a periclinal division in the daughter of the ground tissue stem cell only, but ectopic expression of SHR results in multiple ground tissue layers indicating that limiting SHR expression is a mechanism to prevent continued activation of SCR and additional periclinal ground tissue divisions. Yet SHR and SCR are present in the entire endodermal ground tissue layer (Helariutta et al. 2000; Nakajima et al. 2001). To test whether only certain ground tissue cells are able to perform the periclinal division, we investigated their competence to respond to induced SCR gene expression in the scr-4 null-mutant background.

We designed a set of two vectors that can be used to generate both activation and deletion clones while positively marking the cells in which recombination has taken place with endoplasmic reticulum (ER)-localized GFP (GFP_ER; Fig. 1d,e). We combined the CRE/lox recombination system with the GAL4/UAS transactivation system. The pCB1 binary vector contains the recombination cassette consisting of the CRT1 resistance gene flanked by two direct repeat lox recombination sites. This construction separates and prohibits the constitutive 35S promoter from inducing GAL4VP16 transcription and transactivating GFP_ER. The pG7HSCRE construct harbors the CRE recombinase driven by Arabidopsis HSP18.2 heat-shock promoter. To study activation clones (Fig. 1d), the SCR gene is placed under control of the UAS promoter (USCR) in the pG7HSCRE vector. scr-4 plants harboring a single-copy CB1 insertion were crossed with scr-4,G7HSCRE-USCR plants, and the resulting F1 seedlings were used to generate GFP_ER-marked gene activation clones upon heat-shock induction, which can be recorded in the living organism.

The earliest time point of GFP_ER expression, mainly in the columella and root cap tissues, was observed after -8 h. Up to 16 h after heat shock (has), newly induced clones expressing GFP_ER appeared. GFP_ER-positive (GFP_ER⁺) clones were only observed in seedlings subjected to heat-shock induction (data not shown). Activation of SCR expression in all meristematic scr-4 mutant ground tissue cells can induce a periclinal division (Fig. 2a-c,e,f). No effects of SCR activation were detected in other tissues, nor did SCR activation in cells neighboring the mutant ground tissue have any effect (Fig. 2g,h). In addition, heat shock alone did not induce any divisions in the ground tissue in scr-4 plants alone or in scr-4 plants harboring either construct (data not shown). These results show that in the absence of SCR, all ground tissue cells are competent to perform a periclinal division as long as they reside in the meristematic zone, indicating the necessity for an active mechanism to restrict periclinal division to stem cell daughters.

View larger version (162K): [in this window] [in a new window]   Figure 2. Induction of periclinal cell division by SCR activation clones. (a) Root tip showing GFPER-marked clones with SCR expression 16 has. (b) Close-up of section depicted in a, showing ground tissue clone. (c) Ground tissue clone from a and b has divided periclinally 24 has. (d) Additional periclinal ground tissue divisions (arrowhead) in scr-2 roots marked by SCR promoter-driven GFPER. (e) GFPER-marked SCR activation clone at the border of the meristem shows a periclinally divided ground tissue cell flanked by undivided proximal cells (arrowheads, 16 has). (f) At 24 has, the GFPER-marked cells have elongated and not divided again indicating their displacement from the meristem. (g,h) Vascular and epidermal clones do not induce periclinal divisions in the neighboring ground tissue. (i) SHR promoter-driven GFP:SHR expression in wild-type roots. GFP:SHR protein is localized to the nucleus in the endodermis, ground tissue stem cells, and QC. (j) Expression of pSCR::YFPH2B in endodermis, ground tissue stem cells, and QC in a wild-type root. (k) pSCR::YFPH2B is absent from the QC and low in scr-4 mutant ground tissue. (l,m) pSCR::YFPH2B is present in both ground tissue layers after periclinal divisions in scr-4 roots. (n) GFP:SHR is present in both ground tissue layers after periclinal divisions in scr-4 roots. Brackets indicate ground tissue. Internal tissues are to the left.

SHR protein can translocate from the stele to the single ground tissue layer in scr mutants, indicating that SHR movement from the stele does not require SCR activity (Helariutta et al. 2000; Wysocka-Diller et al. 2000; Nakajima et al. 2001). However, ectopically expressed SHR:GFP moves from the epidermis to the ground tissue in a scr mutant background but not in wild type, which suggests a role for SCR in restricting SHR localization (Sena et al. 2004). Indeed, SHR promoter-driven GFP: SHR fusion protein is present at low levels and is maintained in both ground tissue layers on periclinal divisions observed in scr-4 (Fig. 2i,n), demonstrating that symmetric division and SHR movement or perdurance beyond a single cell layer occurs in the absence of functional SCR.

To determine the asymmetry of the induced periclinal ground tissue divisions in activation clones, we again used the pSCR::YFP_H2B marker. The lines were analyzed using two different confocal microscope settings (see Materials and Methods). In the GFP + YFP mode, fluorescence from both GFP and YFP are detected, whereas in the YFP mode, only YFP is detected. After induction of SCR, pSCR::YFP_H2B is induced in cells marked by clonally activated GFP_ER and is equally divided over the inner and outer cells on periclinal division at 16 has (Fig. 3a,b). By 40 has, pSCR::YFP_H2B disappears from the outer cell while being strongly maintained in the inner cell (Fig. 3c,d), matching SCR regulation in ground tissue stem cell daughters (Wysocka-Diller et al. 2000).

View larger version (102K): [in this window] [in a new window]   Figure 3. Activation clones reveal cell-autonomous SCR function in asymmetric division. (a-d) pSCR::YFPH2B is induced in a SCR activation clone and divided over the inner and outer ground tissue cells on periclinal division at 16 has (a,b). Later, pSCR::YFPH2B separates asymmetrically to the inner cells. Induced periclinal ground tissue divisions observed in cells flanking the clone (arrows) exhibit low levels of pSCR::YFPH2B that is divided equally over both cells (c,d; 40 has). (e,f) GFPER-marked ground tissue SCR activation clone (e; 16 has) induces periclinal division in a flanking GFPER- cell (f; arrow; 24 has). (g,h) GFPER- ground tissue cells flanking a periclinal GFPER-marked SCR activation G2-clone (g, arrows, 16 has) are nonautonomously induced to perform periclinal divisions (h; arrows; 24 has). (i-k) Periclinal division in GFPER- ground tissue cells flanking a SCR:GFP activation clone in the same (i) and adjacent (j) cell file 40 has. (k) Optical cross-section of the root in i and j, revealing two nonautonomously induced periclinal ground tissue divisions in cell files flanking the SCR:GFP activation clone (arrows). Nuclear SCR:GFP strictly colocalizes with the GFPER-marked activation clone. (l-o) pSCR::YFPH2B is divided over both ground tissue layers following periclinal division in a SCR activation clone (l,m; 16 has). At 24 has, functional SCR gene expression marked by GFPER expression throughout the cells localizes to the outer cells in the periclinal G2-clone (n; arrow), whereas nuclear pSCR::YFPH2B still separates asymmetrically to the inner cells (o). (a,c,l,n) GFPER and YFPH2B are visualized simultaneously in the GFP mode (see Materials and Methods). Brackets indicate ground tissue. Internal tissues are to the left.

To examine whether these apparently nonautonomous divisions were caused by SCR movement, we replaced SCR with a fully functional SCR:GFP fusion gene. SCR:GFP was never observed in nonautonomously induced periclinally divided cells neither before nor following the observed division, and hence we found no evidence for SCR movement (Fig. 3i-k; data not shown). In nonautonomously induced periclinal cell divisions (induced before 24 has; data not shown), the SCR promoter is not activated, and the low background pSCR::YFP_H2B expression is distributed evenly, indicating that these periclinal cell divisions are symmetric (Fig. 3c,d; arrows). Cells may respond by periclinal division because of artificially high expression of SCR from the 35S promoter or by movement of the highly expressed GAL4VP16 protein in the activation clones, and therefore a final conclusion on SCR cell autonomy requires the analysis of deletion clones (see below). A similar observation was made in flowers, where ML1-driven high expression of AP1 induced a more extensive rescue of the ap1 mutant phenotype compared with AP1 clones in mosaic plants, suggesting that higher levels of AP1 in L1 had limited nonautonomous effects (Sessions et al. 2000).

We next examined the dynamics of pSCR::YFP_H2B activity in periclinal G2 clones to determine whether SCR is permanently or transiently required to maintain the asymmetry of the division (Fig. 1b, 1 vs. 3). Heat-shock activation of SCR expression results in pSCR::YFP_H2B induction in ground tissue cells that divide periclinally even before GFP_ER is detected in the GFP + YFP mode (Fig. 3l,m). After the division, SCR expression marked by GFP_ER fluorescence throughout the cells is separated to the outer cells shown in the GFP + YFP mode (Fig. 3n). The YFP detection mode shows that the nuclear pSCR::YFP_H2B marker still becomes asymmetrically expressed in inner ground tissue cells that no longer transcribe functional SCR (Fig. 3o).

Our results suggest that ground tissue cells divide asymmetrically only if SCR is present in these cells. Importantly, SCR is only transiently required to promote asymmetry indicating rapid separation of cell fates. Our data show that SCR is not exclusively promoting cell division plane rotation in the ground tissue. Symmetric periclinal divisions observed in scr mutants show that periclinal division per se is not dependent on SCR presence, but the maintenance of GFP:SHR in both layers suggests that one role of SCR is to restrict SHR to a single tissue layer that prevents additional periclinal cell divisions and specification of endodermal layers as observed in SHR ectopic expression studies (Helariutta et al. 2000; Nakajima et al. 2001; Sena et al. 2004).

Deletion clones reveal cell autonomy of SCR action, feedback regulation, and early fate determination

To further examine the autonomy of SCR action, we tested SCR deletion clones initiated in the ground tissue stem cell whose surrounding cells have near wild-type levels of SCR expression. For clonal deletion experiments, the pCB1 vector was used to complement the scr-4 mutant by cloning the SCR gene expressed from its own promoter within the recombination cassette (pCB1-SCR, Fig. 1e) and selecting transformants with a single copy insert. Subsequent introduction of G7HSCRE by crossing reveals the effects of deleting SCR gene activity in heat-shock-induced GFP_ER-marked clones in a phenotypically wild-type plant (Fig. 1e).

Three types of clones were observed, consisting of mutant ground tissue derived from scr^-/- stem cells attached to either wild-type endodermis and cortex or one of the two layers being scr^-/-. Optical cross-sections also revealed wild-type ground tissue files flanking the deletion clones. None of these configurations rescued periclinal divisions in daughters of scr mutant stem cells (Fig. 4a,b,e; data not shown). Thus, deletion of SCR from ground tissue stem cells invariably results in a single layered ground tissue typical for the scr mutant phenotype, strongly suggesting that SCR at wild-type levels acts strictly cell autonomously in periclinal ground tissue division. Although the cell autonomy eliminates SCR as a possible top-down signal, its ability to induce asymmetric periclinal divisions in meristematic ground tissue cells in the absence of mature endodermis and cortex acting as a patterning template effectively rules out the need for top-down signaling (Fig. 1c, 1) to pattern the ground tissue.

View larger version (141K): [in this window] [in a new window]   Figure 4. Cell autonomy, autoregulation, and ground tissue determination revealed by SCR deletion clones. (a,b,e) GFPER-marked single-layered ground tissue SCR deletion clones (arrowheads) originating from a scr-/- stem cell are not induced to divide periclinally by neighboring cells expressing wild-type SCR levels. (e) Optical cross-section of a root containing a GFPER-marked SCR deletion clone circumpherentially flanked by wild-type ground tissue. (c,f) QC, ground tissue stem cells, and their daughters rapidly lose pSCR::YFPH2B when SCR expression is eliminated (arrowheads), whereas pSCR::YFPH2B is maintained in the already formed endodermis 40 has. (d,g) In a different root at 72 has, pSCR::YFPH2B is reduced to background levels in the already formed endodermis within a SCR deletion clone (open arrowheads). pSCR::YFPH2B remains absent in the single ground tissue layer originating from the mutant stem cell (arrowheads). (h) pCo2::YFPH2B marker expression in the cortex of wild-type roots is excluded from QC, ground tissue stem cells, and their single-layered daughters. (i) pCo2::YFPH2B expression in the single-layered ground tissue and QC (arrow) in scr-4 roots. (j,k) Massive GFPER marked the SCR deletion clone, including the ground tissue that contains a pile of single-layered cells (arrowheads, 48 has). pCo2::YFPH2B remains present in the cortex and is also present in the single-layered ground tissue (k, arrows). (l) pEn7::YFPH2B expression in the endodermis of wild-type roots is only excluded from the QC cells. (m) pEn7::YFPH2B expression in the single layered ground tissue in scr-4 roots. (n,o) Massive GFPER-marked SCR deletion clone, including the ground tissue that contains a pile of single layered cells (arrowheads, 48 has). (o) pEn7::YFPH2B remains present in the endodermis (arrows) and is also present in the single-layered ground tissue. Brackets indicate ground tissue. (e) Endodermis; (c) cortex. (a,b,h,i,l,m) Internal tissues are to the left.

To examine the effect of SCR deletion on asymmetric fate specification, we studied the expression of the independent endodermis and cortex specific transcripts En7 and Co2. The promoters of both genes were fused to YFP_H2B. pCo2::YFP_H2B is highly expressed in the cortex but excluded from the QC, the ground tissue stem cells, and their undivided daughters in wild type, whereas it is expressed in the entire single-layered mutant ground tissue and QC in scr-4 roots (Fig. 4h,i). pEn7::YFP_H2B is highly expressed in the endodermis and is excluded from the QC in wild type, whereas it is expressed in the mutant ground tissue and QC in scr-4 roots (Fig. 4l,m; data not shown). These markers confirm previous data on the mixed identity of the ground tissue layer in scr mutants (Di Laurenzio et al. 1996) and reveal a role for SCR in inhibiting En7 and Co2 expression in QC and QC plus ground tissue stem cells, respectively. Surprisingly, both markers are maintained in their respective ground tissue layer in clones containing cells that underwent asymmetric division before SCR deletion (Fig. 4j,k,n,o, arrows). pCo2::YFP_H2B expression is induced in the single-layered ground tissue originating from the scr^-/- stem cells (Fig. 4j,k).

The endodermis and cortex markers indicate that the SCR-mediated asymmetric cell division leads to immediate and stable separation of cell fates. This is in agreement with the transient requirement of SCR for cell fate separation on periclinal ground tissue division observed in activation clones. In analogy with animal systems, we speculate that such a "locking" mechanism may be caused by chromatin-mediated processes (Orlando 2003; Rasmussen 2003).

Our results support a model in which SCR functions cell autonomously to induce rotation of cell division plane and asymmetry of division in the ground tissue (Fig. 5). One aspect of the model is the strong autoregulatory SCR expression in QC and ground tissue stem cells versus the maintained postdivision expression of SCR in the maturing endodermis. SCR expression is induced by SHR in the QC and elevated in the ground tissue, and thereafter, autoinduction of expression becomes the main source of gene regulation upon which the SCR promoter appears to be desensitized to SHR. SCR in the QC is required to specify QC fate and to maintain the surrounding stem cells. In the ground tissue stem cell daughters, SCR induces the asymmetric periclinal division. The active QC prevents this division in the ground tissue stem cells. Upon periclinal division SCR causes a rapid separation of endodermis and cortex gene expression patterns and locks the cells in their respective fates. SCR and SHR expression in the outer cortex cell is rapidly reduced to ensure a single periclinal ground tissue division. We postulate that during separation of cell fates, additional factors required for the execution of the periclinal division are segregated or degraded from the SHR and SCR expressing endodermal cells, thus preventing repeated periclinal divisions. The function of SCR in the endodermis is to sequester SHR and prevent movement beyond a single cell file, thereby preventing the renewed induction of SCR in the cortex, which would lead to additional asymmetric divisions. This mechanism effectively limits asymmetric division to ground tissue stem cell daughters.

View larger version (47K): [in this window] [in a new window]   Figure 5. SCR function in QC and ground tissue. SHR moves from the stele to the QC and ground tissue cells. In the QC and ground tissue stem cells, SCR expression is induced by SHR and maintained by autoregulation. The inductive capacity of SHR is lost on SCR expression. The QC prevents SCR induced periclinal cell division in the ground tissue stem cell. SCR induces the periclinal division in the ground tissue stem cell daughter. SCR mediates rapid endodermal (SHR) and cortical (C) fate separation and segregation of factors required for execution of the periclinal division. Residual SHR and SCR in the outer cell is degraded. In the endodermis, SCR prevents SHR movement to the neighboring cortex cell file, thereby preventing additional periclinal divisions.

	Materials and methods

Top Abstract Results and Discussion Materials and methods Acknowledgments References

 
Additional details on growth conditions, number of plants and clones analyzed, and cloning strategies are provided in the Supplemental Material.

Heat shock and image analysis of clones

Heat shocks were applied to seedlings grown on vertical plates by incubation at 37°C for 18 min to 1 h, thereby generating increasingly larger clones. Imaging and analysis of clones was performed using a Leica SP2 inverted confocal microscope and the accompanying software. Root cell walls were stained with propidium iodine. In the GFP channel, GFP and YFP are visualized simultaneously by excitation at 488 nm and by collection at 498-523 nm. In the YFP channel, only YFP is visualized at excitation at 514 nm and collection at 530-560 nm.

	Acknowledgments

Top Abstract Results and Discussion Materials and methods Acknowledgments References

 
We are indebted to Keiji Nakajima and Philip Benfey for providing mutants and constructs and to the Benfey lab, and in particular Kim Gallagher, for valuable discussions and suggestions.

The publication costs of this article were defrayed in part by payment of page charges. This article must therefore be hereby marked "advertisement" in accordance with 18 USC section 1734 solely to indicate this fact.

	Footnotes

 
Supplemental material is available at http://www.genesdev.org.

Article and publication are at http://www.genesdev.org/cgi/doi/10.1101/gad.305504.

¹ Corresponding author.
E-MAIL r.heidstra{at}bio.uu.nl; FAX 31-30-2532837.

	References

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