Drak Is Required for Actomyosin Organization During Drosophila Cellularization

The generation of force by actomyosin contraction is critical for a variety of cellular and developmental processes. Nonmuscle myosin II is the motor that drives actomyosin contraction, and its activity is largely regulated by phosphorylation of the myosin regulatory light chain. During the formation of the Drosophila cellular blastoderm, actomyosin contraction drives constriction of microfilament rings, modified cytokinesis rings. Here, we find that Drak is necessary for most of the phosphorylation of the myosin regulatory light chain during cellularization. We show that Drak is required for organization of myosin II within the microfilament rings. Proper actomyosin contraction of the microfilament rings during cellularization also requires Drak activity. Constitutive activation of myosin regulatory light chain bypasses the requirement for Drak, suggesting that actomyosin organization and contraction are mediated through Drak’s regulation of myosin activity. Drak is also involved in the maintenance of furrow canal structure and lateral plasma membrane integrity during cellularization. Together, our observations suggest that Drak is the primary regulator of actomyosin dynamics during cellularization.

Although it is clear that actomyosin dynamics are important for proper cellularization, how actomyosin is regulated during cellularization is not well understood. A few genes, such as Src64B, Btk29A, and RhoGEF2, are known to be required for actomyosin contraction during cellularization (Thomas and Wieschaus 2004;Padash Barmchi et al. 2005;Grosshans et al. 2005;. However, the products of these genes do not directly regulate myosin II, and they do not regulate the assembly or organization of myosin II in the microfilament rings. To address the question of how actomyosin dynamics are regulated during cellularization, an analysis of genes that encode direct regulators of MRLC is needed. The most likely candidates include Rok, and the proteins that contain MLCK-like kinase domains in Drosophila (Champagne et al. 2000;dos Santos et al. 2015). One of these proteins is the serine/threonine kinase Drak. It is the only Drosophila homolog of the Death-Associated Protein Kinase (DAPK) (Neubueser and Hipfner 2010). Drak functions synergistically with Rho kinase (Rok) to phosphorylate Drosophila Sqh, and to regulate epithelial tissue morphogenesis and ommatidia morphogenesis during post-embryonic development (Neubueser and Hipfner 2010;Robertson et al. 2012); however, neither study found a role for Drak independent of Rok.
Here, we analyzed the role of Drak in actomyosin regulation during cellularization, and found that Drak plays a role in the organization and function of microfilament rings through MRLC phosphorylation. We also found that Drak plays a role in the maintenance of furrow canal structure during cellularization. To our knowledge, this is the first study to show the function of a DAPK family member independently regulating actomyosin dynamics in vivo.

Fly strains
OreR was used as the wild-type strain. drak del and drak KO are lossof-function alleles that delete the entire coding region of drak, and the kinase domain of drak, respectively (Neubueser and Hipfner 2010). sqh A21 , sqh A20A21 , sqh E21 , and sqh E20E21 are phosphomimetic transgenes, and nonphosphorylatable transgenes, expressed under the control of the sqh promoter (Winter et al. 2001;Jordan and Karess 1997).

Transmission electron microscopy
Embryos were dechorionated with bleach and fixed using the n-heptane permeabilization method (McDonald et al. 2000). Embryos were hand-divitellinized, embedded in epon molds, thick-sectioned (1 mm), and stained with 1% methylene blue-azure II to determine developmental stage. Cellularization stage embryos were thin-sectioned (60-90 nm), stained with 4% uranyl acetate and Reynold's lead citrate, and examined using a Hitachi 8100 STEM electron microscope with an AMT digital camera.

Data availability
All strains and reagents are available upon request.

RESULTS
Drak is required for organization of the actomyosin cytoskeleton during cellularization To investigate the function of Drak in actomyosin regulation, we examined drak mutants for defects in the actomyosin network that spans the entire embryo during cellularization. We analyzed drak del , a complete deletion of drak, and drak KO , a deletion of the kinase domain of Drak. Homozygous drak del and drak KO mutants are viable and fertile (Neubueser and Hipfner 2010). During early cellularization, before the cellularization front has passed the nuclei, maternally and zygotically homozygous drak del and drak KO mutant embryos showed a slightly wavy cellularization front, where furrow canals have different depths ( Figure 1A and Supporting Information, Figure S1A). This defect is similar to the irregular early cellularization front defect in src64 Anillin localization in drak del mutant embryos is similar to wild-type. (B) Early cellularization microfilament rings. Anillin distribution within the microfilament rings in drak del mutant embryos is similar to wild-type. Microfilament rings are more angular in drak del mutant embryos than in wild-type embryos. (C) Late cellularization-I front. Anillin localization in drak del mutant embryos is similar to wild type. (D) Late cellularization-I microfilament rings. Anillin distribution within the microfilament rings of drak del mutant embryos is similar to Anillin distribution in wild-type. Microfilament rings are more irregular and less constricted in drak del mutant embryos than in wild-type embryos. (E) Late cellularization-II front. Anillin localization in drak del mutant embryos is similar to wild-type. (F) Late cellularization-II microfilament rings. Anillin distribution within the microfilament rings of drak del mutant embryos is similar to that in wild-type embryos. Microfilament rings are more irregular in drak del mutant embryos than in wild-type embryos. Microfilament rings are highly constricted in wild-type embryos but show less constriction in drak del mutant embryos. (G) Plot of microfilament ring circularity indices. Microfilament rings deviate more from circularity in drak del mutant embryos than in wild-type embryos. Mean 6 SD, ÃÃ P , 0.01, ÃÃÃ P , 0.001, ÃÃÃÃ P , 0.0001. Data were compared using a two-sided Mann-Whitney test. Scale bars, 20 mm. mutant embryos (Thomas and Wieschaus 2004;. Myosin II was distributed evenly in the microfilament rings at the cellularization front in wild-type embryos, whereas myosin II was distributed in clumps interspersed between regions of reduced or no myosin II in the microfilament ring network in both drak del and drak KO mutant embryos ( Figure 1B and Figure S1B). This defect is strikingly different from the microfilament ring defect of src64 mutant embryos, in which myosin II is distributed evenly throughout the microfilament rings, even though contraction is defective and microfilament ring shapes are abnormal Thomas and Wieschaus 2004;. These results suggest that Drak is involved in the organization, assembly or maintenance of myosin II in microfilament rings during cellularization.
Since drak del and drak KO caused similar defects, we conducted further phenotypic analyses with drak del . During late cellularization when the cellularization front has passed the nuclei, and the rings are undergoing basal closure, wild-type embryos had an even distribution of myosin II in microfilament rings. During late cellularization, drak del mutant embryos had myosin II organization defects, where myosin II was distributed unevenly in clumps with regions of reduced myosin II. These defects were similar to, but less severe than, those in early cellularization ( Figure 1, C-F). We divided late cellularization into an earlier part, late cellularization-I, when the cellularization front had just passed the nuclei, and a later part, late cellularization-II, when the cellularization front was near its final depth, and microfilament rings were highly constricted in wild type (Figure 1, C-F). During late cellularization-I, myosin II was distributed unevenly throughout the microfilament rings in drak del mutant embryos, but was absent in fewer regions than during early cellularization. Clumps of myosin II were observed in some regions ( Figure 1D). During late cellularization-II, some regions of the microfilament rings were missing myosin II, but these were fewer than during late cellularization-I, and there were fewer clumps of myosin II ( Figure 1F). Thus, the myosin II organization defects of drak del became less severe during later stages of cellularization. These data suggest that Drak is required for organization of myosin into contractile rings.

Sqh phosphorylation is decreased in drak mutants
Mono-phosphorylation (Serine-21) and di-phosphorylation (Serine-21 and Threonine-20) of Sqh were decreased substantially in drak mutants during cellularization ( Figure 1G and Figure S1C). Since drak del mutant embryos showed more severe defects during early cellularization than during late cellularization, we compared the phosphorylation levels of Sqh between early cellularization and late cellularization. Levels of mono-phosphorylated Sqh were reduced by 94% during early cellularization, and by 84% during late cellularization in drak del mutant embryos relative to wild-type embryos ( Figure 1H). These results suggest that Drak regulates Sqh phosphorylation during cellularization, but has a greater role during early cellularization, and that less severe defects in myosin II organization during late cellularization were due to increased phosphorylation levels of Sqh in drak del mutant embryos. By late cellularization, other kinases that phosphorylate MRLC might act synergistically with Drak. We examined Sqh phosphorylation during other stages of early embryogenesis, and found that mono-phosphorylation of Sqh was decreased substantially in drak del mutant embryos before cellularization. Sqh mono-phosphorylation was also decreased during gastrulation, but not as severely as during cellularization ( Figure S2). Thus, during embryogenesis, Drak is either the major regulator of myosin II activity or its function is required for the organization of myosin II and subsequent activity of other kinases that phosphorylate Sqh during cellularization.

Anillin localization is not dependent on Drak
Anillin is a scaffolding protein that binds septins, F-actin, and myosin II, is localized to the furrow canals, and is involved in F-actin and myosin II organization during cellularization Field and Alberts 1995;Thomas and Wieschaus 2004). To determine whether the defective organization of myosin II in drak del mutant embryos is caused by defects in the localization or organization of Anillin at the cellularization front, we stained the microfilament rings in drak del mutant embryos with anti-Anillin antibody. We found that Anillin was localized normally to the furrow canals throughout cellularization (Figure 2, A, C, and E). Anillin was distributed uniformly and organized properly in the microfilament rings of drak del mutant embryos during early cellularization ( Figure 2B). During late cellularization, Anillin distribution within the microfilament rings of drak del mutant embryos was similar to Anillin distribution in wild-type embryos (Figure 2, D and F). Therefore, Anillin localization to the cellularization front, and Anillin distribution within the microfilament rings, do not depend on Drak activity.

Actomyosin contraction requires Drak
Because, unlike myosin II, Anillin was not disorganized in drak del mutant embryos, we were able to use it as a marker for microfilament ring shape to test for defects in microfilament ring contraction. Microfilament rings in drak del mutant embryos had angular and irregular shapes during early cellularization, and had irregular shapes and showed reduced constriction during late cellularization, suggesting an actomyosin contraction defect (Figure 2, B, D, and F). To quantify the ring shape defects, we compared circularity indices of drak del microfilament rings to those of wild-type microfilament rings (Thomas and Wieschaus 2004;. drak del mutant embryos showed lower circularity indices than wild-type embryos throughout cellularization ( Figure 2G). The deviation from circularity compared to wildtype indicated that contractile activity of the microfilament rings was impaired by drak mutation. However, observation of some microfilament ring constriction indicated that actomyosin contraction was not completely abrogated by loss of drak function. These results Figure 3 Drak regulates actomyosin organization through myosin II activation. Anti-Zip antibody-stained drak del mutant embryos expressing Sqh E21 , Sqh E20E21 , Sqh A21 , or Sqh A20A21 . Throughout cellularization, myosin II is well organized within the microfilament rings of drak del ; sqh E21 and drak del ;sqh E20E21 embryos, but is disorganized within the microfilament rings of drak del ;sqh A21 and drak del ;sqh A20A21 embryos.
suggest that Drak is necessary for actomyosin contraction during cellularization.
Activated Sqh rescues the drak del phenotype To test whether MRLC phosphorylation is involved in Drak function, we expressed activated Sqh in drak del mutant embryos. Expression of either the mono-phosphorylated mimetic Sqh E21 , or the di-phosphorylated mimetic Sqh E20E21 , completely rescued defective myosin II organization during cellularization, whereas expression of nonphosphorylatable Sqh A21 or Sqh A20A21 did not. An even distribution of myosin II throughout the microfilament rings similar to wild-type embryos was observed in drak del mutant embryos expressing activated Sqh, whereas drak del mutant embryos expressing nonphosphorylatable Sqh, Sqh A21 , or Sqh A20A21 , showed myosin II organization defects similar to drak del mutant embryos (Figure 3). drak del mutant embryos expressing activated Sqh also showed uniform cellularization fronts similar to those of wild-type embryos (data not shown). These results suggest that Drak regulates myosin II organization through the phosphorylation of Sqh.
We analyzed microfilament ring contraction in Anillin-stained embryos. Expression of activated Sqh in drak del mutant embryos restored microfilament ring shape, whereas expression of nonphosphorylatable Sqh did not ( Figure 4A). Microfilament ring circularity indices of drak del ;sqh E21 embryos were higher than those of drak del ;sqh A21 embryos throughout cellularization. Likewise, drak del ;sqh E20E21 circularity indices were higher than drak del ;sqh A20A21 circularity indices (Figure 4, B and C). Circularity indices of drak del ;sqh E21 and drak del ;sqh E20E21 embryos did not show any significant difference from those of wildtype embryos ( Figure 2G and Figure 4, B and C). We did not observe any enhancement of the drak del phenotype by expression of Sqh A21 or Sqh A20A21 when compared to drak del alone ( Figure 2G and Figure 4, B and C). Thus, activation of Sqh restores both the myosin II distribution and organization defects, and the actomyosin contraction defects. Together, these data suggest that Drak regulates both myosin II organization in microfilament rings, and actomyosin contraction by phosphorylating Sqh.
Drak is required for furrow canal structure and membrane integrity Since drak del mutant embryos showed defects in the organization of the cytoskeleton in the microfilament rings, we thought that furrow canal structure might be abnormal in drak mutant embryos. Therefore, we analyzed the furrow canal structure in more detail using transmission electron microscopy. During early cellularization, wild-type embryos had teardrop-shaped furrow canals. However, most furrow canals in drak del mutant embryos were narrow at the bases, and appeared collapsed. A few furrow canals in drak del mutant embryos contained blebs ( Figure 5, A, A', B, and B'). Unexpanded furrow canals in drak del mutant embryos during early cellularization are consistent with defective actomyosin contraction. In the absence of actomyosin contraction in the microfilament network, the furrow canals are not pulled into their normal teardrop shapes. Anti-Anillin antibody-stained drak del mutant embryos expressing Sqh E21 , Sqh E20E21 , Sqh A21 , or Sqh A20A21 . Microfilament rings in drak del ;sqh E21 and drak del ;sqh E20E21 embryos are more rounded and regular in shape than microfilament rings in drak del ;sqh A21 and drak del ;sqh A20A21 embryos. (B, C) Plots of circularity indices of microfilament rings of anti-Anillin antibody-stained drak del mutant embryos expressing Sqh E21 or Sqh A21 (B), and drak del mutant embryos expressing Sqh E20E21 or Sqh A20A21 (C). The circularity index is higher in embryos expressing Sqh E21 compared to embryos expressing Sqh A21 (B), and in embryos expressing Sqh E20E21 compared to embryos expressing Sqh A20A21 (C). Mean 6 SD, Ã P , 0.05, ÃÃ P , 0.01, ÃÃÃÃ P , 0.0001. Data were compared using a two-sided Mann-Whitney test. Scale bars, 20 mm.
During late cellularization, wild-type embryos had flask-shaped furrow canals, with broader bases than during early cellularization. A few furrow canals showed membrane blebbing ( Figure 5, C, C', E, and E'). In drak del mutant embryos, some furrow canals were unexpanded, whereas many were broad and flat-bottomed like wild type ( Figure 5, D, D', F, F', and F''). During late cellularization-I, drak del mutant embryos showed some blebbing, similar to wild-type embryos (data not shown). However, during late cellularization-II, some furrow canals in drak del mutant embryos showed more severe membrane blebbing and larger blebs than wild-type embryos ( Figure 5, F and F'). The failure of many furrow canals to expand in drak del mutant embryos during late cellularization is consistent with the absence of actomyosin ring constriction, which is necessary to pull the furrow canals into flask-like shapes as the basal sides of the cells start to close. Membrane blebbing inside the furrow canals is consistent with a loss of furrow canal membrane integrity, or a loss of cortical cytoskeleton integrity in drak del mutant embryos.
Wild-type embryos had closely apposed lateral plasma membranes apical to the furrow canals ( Figure 5, A, C, E, G, and G'). We observed that, during late cellularization-II, drak del mutant embryos had strings of vesicles instead of lateral plasma membranes in many regions, generating cytoplasmic connections between cells (Figure 5, F, H, and H'). Vesiculated plasma membrane and furrow canal defects could be caused by abnormal membrane compartmentalization. We tested this by assaying the localization of proteins associated with different cell membrane compartments during cellularization: Neurotactin (Nrt), Discs large (Dlg), Armadillo (Arm), Anillin (Ani), and Peanut (Pnut) (Sokac and Wieschaus 2008b;Field et al. 2005;Lecuit and Wieschaus 2000). Localization of these proteins in drak del mutant embryos was similar to that of wild-type embryos during late cellularization ( Figure 2E and Figure  6). These observations suggest that Drak is essential for maintenance of lateral plasma membrane integrity during cellularization, but not for membrane compartmentalization.

Actin is distributed within the actomyosin rings independently of Drak activity
Since myosin II is highly disorganized, and furrow canal structure is defective in drak del mutant embryos, we wondered whether F-actin was also disorganized in drak mutant embryos. To determine whether Drak activity was required for F-actin organization, we examined the distribution of F-actin in microfilament rings. In wild-type embryos and drak del mutant embryos, F-actin was highly enriched at the furrow canals (Figure 7, A and C). Thus, F-actin is localized normally to the cellularization front in the absence of Drak activity. F-actin was distributed uniformly in microfilament rings in both wild-type embryos and drak del mutant embryos during early cellularization ( Figure 7B). During late cellularization, F-actin was not distributed evenly within the microfilament rings in drak del mutant embryos ( Figure 7D). The F-actin distribution defect is not as severe as the myosin II distribution defect (Figure 1, D and F). Interestingly, F-actin distribution defects were not observed during early cellularization when myosin II organization defects were strongest, but were present during late cellularization when myosin II organization defects were somewhat less pronounced in drak mutant embryos. Since F-actin was not found in clumps and gaps like myosin II, we conclude that neither Drak nor myosin II organizes F-actin within the microfilament rings. We speculate that the F-actin distribution defects are a consequence of the furrow canal defects in drak del mutant embryos.
We tested whether the F-actin distribution defect in the microfilament rings was caused by the absence of Drak-mediated Sqh phosphorylation by expressing phosphomimetic Sqh in drak del mutant embryos. Expression of Sqh E21 rescued the drak del F-actin distribution defect, but expression of Sqh A21 did not rescue the drak del F-actin distribution defect during late cellularization ( Figure 7D). Expression of Sqh E20E21 did not completely rescue the drak del F-actin distribution defects during late cellularization ( Figure 7D). This is surprising, in that expression of Sqh E20E21 did rescue both the myosin II organization defects, and the actomyosin contraction defects of drak del mutant embryos (Figure 2, D and F, and Figure 3).

DISCUSSION
Actomyosin organization within the microfilament rings requires drak activity Tight regulation of actomyosin is likely critical for many cellular processes, but how this is accomplished is as yet poorly understood.
A key input to the regulation of myosin II is through phosphorylation of the Serine-19, or the Serine-19 and Threonine-18, residues of MRLC. The variety of MRLC kinases might allow different specific aspects of actomyosin dynamics, such as localization, organization, and contraction to be regulated independently. Such a system would provide greater flexibility and control than either a single kinase, or multiple kinases acting in concert, regulating all of these functions. We find that drak is required for the organization of myosin II into contractile rings, but is not required for localization of myosin to the cellularization front. Since the majority of Sqh phosphorylation during cellularization is dependent on drak activity, Drak either regulates most aspects of myosin II dynamics during cellularization, or Drak-regulated myosin II organization is required for further function of myosin II, such as contraction.
Myosin II is somewhat less disorganized, and Sqh phosphorylation is slightly increased, during late cellularization in drak mutants, suggesting that phosphorylation of myosin II by other kinases occurs during late cellularization. Thus, other kinases might act synergistically with Drak to regulate actomyosin organization during late cellularization. For example, Drak function has been shown to be partially redundant with Rok function during later development (Neubueser and Hipfner 2010;Robertson et al. 2012). An alternative possibility is that other kinases that do not normally function in myosin II organization in the microfilament rings might phosphorylate Sqh to some degree, and lead to some organization of myosin II in the absence of Drak activity.
Myosin II has been implicated in actin bundling and F-actin organization in some contexts (Vicente-Manzanares et al. 2008Anderson et al. 2008;Brodu and Casanova 2006;Ma et al. 2012;Thoresen et al. 2011). Since F-actin appears to be organized normally within drak mutant microfilament rings during early cellularization, we conclude that myosin II does not play a role in initially organizing F-actin within the microfilament rings during cellularization. F-actin is somewhat disorganized during late cellularization in drak del mutant embryos, but not as severely as myosin II, nor does the pattern of F-actin distribution fit the pattern of myosin II distribution in drak del mutant embryos. These observations suggest that F-actin disorganiza-tion is an indirect consequence of Drak regulation of myosin II activity, and that F-actin disorganization might be due to actomyosin contraction defects, or furrow canal structural defects.
Anillin is required for the organization of actomyosin contractile rings during cellularization and cytokinesis (Field and Alberts 1995;Field et al. 2005;Straight et al. 2005;Thomas and Wieschaus 2004). scraps (scra, anillin) mutant embryos have a myosin II organization defect somewhat similar to that of drak mutant embryos: myosin II is found in discrete bars in the actomyosin network Thomas and Wieschaus 2004). Despite this similarity, myosin II defects differ between scra and drak mutant embryos. Myosin II becomes more disorganized during late cellularization in scra mutant embryos (Thomas and Wieschaus 2004). Myosin II becomes slightly better organized during late cellularization in drak mutant embryos. This organizational difference is likely caused by actomyosin contraction during microfilament ring constriction occurring in a highly disorganized cytoskeleton in scra mutant embryos, and occurring in a disorganized cytoskeleton that has slightly improved during constriction in drak mutant embryos. Anillin interacts with myosin II only when MRLC is phosphorylated (Straight et al. 2005). Together with our results, this suggests that Drak phosphorylation of Sqh might be necessary for Anillin-mediated myosin II organization within the contractile ring.
drak is required for actomyosin contraction Phosphorylation of MRLC on Serine-19, or Serine-19 and Threonine-18, leads to the unfolding of inactive myosin II hexamers into an open conformation that allows assembly of bipolar myosin II filaments and their association with F-actin to form actomyosin filaments (Vicente-Manzanares et al. 2009). This is likely how Drak organizes myosin II, as described above. Phosphorylation of MRLC on , also leads to the activation of the Mg 2+ -ATPase activity of myosin II that slides actin filaments past each other, causing actomyosin contraction (Vicente-Manzanares et al. 2009). Three aspects of the drak mutant phenotype support the requirement for Drak in actomyosin contraction: wavy cellularization fronts caused by nonuniform furrow canal depths, abnormal microfilament ring shapes, and failure of microfilament rings to constrict during late cellularization. These are the same defects that suggest an actomyosin contraction defect in src64 mutant embryos. However, src64 mutant embryos do not show myosin II organization defects  Thomas and Wieschaus 2004). Because effective actomyosin contraction likely requires properly organized actomyosin filaments within the contractile ring apparatus, it is unclear whether Drak directly regulates actomyosin contraction or whether Drak enables actomyosin contraction only through proper organization of myosin II within the microfilament rings. One possibility is that phosphorylation of Sqh by Drak both organizes actomyosin filaments into a contractile ring apparatus, and directs actomyosin contraction. An alternative possibility is that Drak is directly responsible for organizing actomyosin filaments into a contractile ring by phosphorylating Sqh, but Drak is not directly involved in its contraction, and different kinases that phosphorylate Sqh regulate actomyosin contraction. Thus, Drak could be an early regulator of myosin II activity during cellularization, such that further phosphorylation of Sqh and myosin II-driven contraction is dependent on Drak-mediated organization of myosin II. At some level, the regulation of actomyosin contraction diverges from the regulation of actomyosin filament organization: Src64 is required for contraction, but has no role in myosin II organization Thomas and Wieschaus 2004).
Rescue of myosin II organization, actomyosin contraction, and F-actin distribution defects in drak mutant embryos by the monophosphorylated Sqh E21 phosphomimetic suggests that Drak-mediated mono-phosphorylation of Sqh at Serine-21 is sufficient for regulation of actomyosin dynamics during cellularization. Although the diphosphorylated Sqh E20E21 phosphomimetic also rescues myosin II organization, and actomyosin contraction defects, it does not rescue F-actin distribution defects in drak mutant embryos. These results are consistent with Drak primarily phosphorylating Sqh at Serine-21, and are consistent with reports that DAPK family members phosphorylate MRLC mainly at Serine-19 (Jin et al. 2001;Kuo et al. 2003).

Drak and membrane and cortex integrity
The normal teardrop shape of the furrow canals in early cellularization is likely caused by actomyosin contraction in the microfilament rings (Thomas and Wieschaus 2004). In drak mutant embryos, unexpanded early cellularization furrow canals, and the failure of many late cellularization furrow canals to expand further, suggest that Drak is required for proper furrow canal structure. Some of the furrow canal structural defects in drak mutant embryos are similar to those of nullo mutant embryos: collapsed furrow canals and blebbing (Sokac and Wieschaus 2008b;Postner and Wieschaus 1994). However, nullo mutant embryos, as well as RhoGEF2 or dia mutant embryos, have other, more severe, furrow canal defects: missing or regressing furrow canals, and compromised lateral membrane-furrow canal compartment boundaries. Furthermore, cytochalasin treatment causes similar defects, suggesting that reduced F-actin levels in the furrow canals are responsible for these defects Wieschaus 2008a, 2008b;Padash Barmchi et al. 2005). Thus Nullo, RhoGEF2 and Dia regulate F-actin and its levels in furrow canals. Our observations suggest that Drak regulates myosin II, and thereby regulates actomyosin organization and contraction, and that these are necessary for structural integrity and expansion of the furrow canals, but not for their continued existence.
The furrow canals of drak mutant embryos during late cellularization show extensive blebbing into the lumens. This is consistent with a defect in furrow canal membrane or cortex integrity. Blebs can be formed by local rupture of the cortical cytoskeleton, or detachment of the plasma membrane from the cortical actomyosin cytoskeleton (Charras and Paluch 2008;Cunningham 1995;Keller and Eggli 1998;Paluch et al. 2005). Actomyosin contraction has been implicated in bleb formation (Charras and Paluch 2008;Fishkind et al. 1991;Hickson et al. 2006;Paluch et al. 2005Paluch et al. , 2006. Therefore, we propose that blebbing in furrow canals is caused by aberrant localized actomyosin contraction during late cellularization in the disorganized actomyosin cytoskeleton of drak mutant embryos. Contraction is presumably driven by phosphorylation of Sqh by kinases other than Drak. Since actomyosin contraction occurs in a disorganized actomyosin cytoskeleton, it does not lead to uniform constriction of the microfilament rings, but instead leads to localized contraction, which produces cytoplasmic blebs. However, other causes of furrow canal defects are possible. Plasma membrane attachment sites might not form or function properly in the disorganized furrow canal cytoskeleton in drak mutant embryos. The disorganized cytoskeleton might inhibit vesicle trafficking (Sokac and Wieschaus 2008a;Smythe and Ayscough 2006;Mooren et al. 2012). Vesicle trafficking itself might be defective: mammalian DAPKs have been shown to be involved in membrane trafficking, and in phosphorylation of syntaxin A1 (Tian et al. 2003;Gozuacik and Kimchi 2004).
Vesiculated lateral plasma membrane in drak mutant embryos during late cellularization suggests that the plasma membrane breaks down. Intriguingly, scra mutant embryos have lines of vesicles where the closely apposed lateral plasma membranes would have been. However, in scra mutant embryos, vesiculation is observed during early cellularization, but to a lesser extent than during late cellularization Figure 7 F-actin distribution. Wild-type, drak del , and drak del embryos expressing Sqh E21 , Sqh E20E21 , Sqh A21 , or Sqh A20A21 stained with phalloidin in cross-sections (A, C), and grazing section projections (B, D). (A) Early cellularization front. F-actin is localized normally to the furrow canals of all genotypes. (B) F-actin distribution in microfilament rings during early cellularization. F-actin is distributed uniformly in the microfilament rings of all genotypes. (C) Late cellularization front. F-actin is localized normally to the furrow canals of all genotypes. (D) F-actin distribution in microfilament rings during late cellularization. Wild-type embryos and drak del ;sqh E21 embryos show uniform distribution of F-actin in the microfilament rings. F-actin is not distributed evenly within the microfilament rings of drak del , drak del ;sqh A21 , drak del ;sqh E20E21 , and drak del ;sqh A20A21 embryos. Scale bar, 10 mm. . drak mutant embryos do not show lateral plasma membrane vesiculation defects until late cellularization. drak mutant defects in both the furrow canal membrane and the lateral plasma membrane might reflect a general defect in membrane integrity. It will be interesting to investigate the potential role of myosin II organization in furrow canal structure and plasma membrane integrity.