Trp-Asp (WD) Repeat Domain 1 Is Essential for Mouse Peri-implantation Development and Regulates Cofilin Phosphorylation*

Trp-Asp (WD) repeat domain 1 (WDR1) is a highly conserved actin-binding protein across all eukaryotes and is involved in numerous actin-based processes by accelerating Cofilin severing actin filament. However, the function and the mechanism of WDR1 in mammalian early development are still largely unclear. We now report that WDR1 is essential for mouse peri-implantation development and regulates Cofilin phosphorylation in mouse cells. The disruption of maternal WDR1 does not obviously affect ovulation and female fertility. However, depletion of zygotic WDR1 results in embryonic lethality at the peri-implantation stage. In WDR1 knock-out cells, we found that WDR1 regulates Cofilin phosphorylation. Interestingly, WDR1 is overdosed to regulate Cofilin phosphorylation in mouse cells. Furthermore, we showed that WDR1 interacts with Lim domain kinase 1 (LIMK1), a well known phosphorylation kinase of Cofilin. Altogether, our results provide new insights into the role and mechanism of WDR1 in physiological conditions.


Trp-Asp (WD) repeat domain 1 (WDR1) is a highly conserved actin-binding protein across all eukaryotes and is involved in numerous actin-based processes by accelerating
Cofilin severing actin filament. However, the function and the mechanism of WDR1 in mammalian early development are still largely unclear. We now report that WDR1 is essential for mouse periimplantation development and regulates Cofilin phosphorylation in mouse cells. The disruption of maternal WDR1 does not obviously affect ovulation and female fertility. However, depletion of zygotic WDR1 results in embryonic lethality at the periimplantation stage. In WDR1 knock-out cells, we found that WDR1 regulates Cofilin phosphorylation. Interestingly, WDR1 is overdosed to regulate Cofilin phosphorylation in mouse cells. Furthermore, we showed that WDR1 interacts with Lim domain kinase 1 (LIMK1), a well known phosphorylation kinase of Cofilin. Altogether, our results provide new insights into the role and mechanism of WDR1 in physiological conditions.
The actin cytoskeleton is a highly dynamic structure that regulates cell motility, adhesion, division, and growth and has a fundamental function in embryonic development (1)(2)(3). In physiological conditions, actin filaments are continually assembled and disassembled in response to varied cellular activities (4,5). The dynamics of F-actin is well orchestrated by a large number of actin-binding proteins (5,6). Actin-depolymerizing factor Cofilin plays critical roles in the modulation of actin cytoskeleton dynamics (7). In vitro, Cofilin severs actin filament at low concentrations, whereas it fully decorates actin filaments and suppresses the severing activity at high concentrations (8,9). In addition, Cofilin severing F-actin is not explained well for how the filaments of actin cytoskeleton can be rapidly disassembled in physiological conditions (4). Thus, the function of Cofilin in actin dynamics depends not only on its relative concentration to actin, but also on other regulatory proteins in vivo. Dysfunction of these regulating proteins results in aberrant actin cytoskeleton in various cellular and developmental processes (10 -12).
Cofilin directly binds with actin to function as a regulator of the actin dynamics (13). However, the phosphorylation of Cofilin at Ser-3 blocks its binding site to actin (14,15). Thus, the activity of Cofilin is controlled by phosphorylation and dephosphorylation processes, which are regulated by cascade reactions of several protein kinases and phosphatases. Lim domain kinases (LIMKs) 4 and testis-specific protein kinases (TESKs) are responsible for the phosphorylation of Cofilin, whereas slingshot (SSH) family protein phosphatases and pyridoxal phosphatase (PDXP) catalyze the dephosphorylation reaction (16 -20). These kinases and phosphatases are also regulated by their phosphorylation or localization in cytoplasm to maintain the level of Cofilin phosphorylation in response to extracellular stimuli (21)(22)(23).
The activity of Cofilin on actin disassembly is greatly accelerated by other actin-binding proteins (24,25). WDR1 (WD40 domain repeat 1, also known as actin interaction protein 1), is conserved and was originally identified as an actin-binding protein by a yeast two-hybrid screen (26). WDR1 is involved in actin dynamics by promoting the actin disassembly activity of Cofilin. Mutations in WDR1 result in abnormal cytoskeletal behavior in many organisms (27)(28)(29). A Gene-trap vector inserted Wdr1 intron 2 disrupts its expression completely and results in embryonic lethality before E10.5 (embryonic day * This work was supported by National Natural Science Foundation of China 10.5) in mice, whereas a hypomorphic insertion mutation in this gene leads to autoinflammatory disease because of the impairment of cytoskeletal response in neutrophils and thrombopoiesis (27). WDR1-mediated actin disassembly is also required for spermatogenesis and myocardial growth in mice (30,31). In humans, the aberrant expressions of WDR1 have been shown to be connected to several diseases, including gout, pancreatitis, and primary glioblastoma (32)(33)(34). Although WDR1 is critical for numerous physiological conditions, how it acts in early embryonic development remains largely unclear.
In our study, we demonstrated that zygotic, but not maternal, expression of WDR1 is important for mouse early embryonic development. We showed that WDR1 is essential for mouse peri-implantation development. Most interestingly, we found that WDR1 regulates the level of Cofilin phosphorylation through LIMK, a novel mechanism of WDR1 involved in Cofilin activity.

Results
Zygotic, Not Maternal, WDR1 Is Required for Mouse Development-To investigate the function of Wdr1 in oocyte maturation and pre-implantation embryogenesis, we first examined the expression of Wdr1 in mouse oocytes and preimplantation embryos by quantitative RT-PCR and Western blotting analysis. Our results showed that Wdr1 mRNA was highly expressed in mouse germinal vesicle (GV) oocytes, decreased in metaphase II (MII) oocytes, 1-cell, 2-cell, and morula stage embryos, and then sharply increased in blastocyst stage embryos (Fig. 1A). By comparison, Western blotting analysis showed that WDR1 protein was comparatively highly expressed in GV oocytes, decreased in MII oocytes, increased in 1-cell and 2-cell embryos, and decreased in morula and blastocyst stage embryos again (Fig. 1B).
We generated Wdr1 oocyte-specific knock-out mice by mating Wdr1 f/f mice with Zp3-cre transgenic mice to study the role of WDR1 in female fertility. The mRNA and protein of Wdr1 were dramatically decreased in the GV oocytes from Wdr1 f/f ; Zp3-cre (oocyte-specific knock-out, oKO) females as noted by quantitative RT-PCR and Western blotting analysis ( Fig. 1, C and D). However, Wdr1 f/f ; Zp3-cre females delivered comparable offspring compared with the controls (Wdr1 f/f and Wdr1 f/ϩ ; Zp3-cre females) after mating with Wdr1 f/f males (Fig. 1E). These data demonstrated that maternal WDR1 is not required for Wdr1 f/f ; Zp3-cre female fertility.
We also mated Wdr1 f/f ; Zp3-cre females with Wdr1 f/Ϫ males. The litter size was decreased to about 50% (Fig. 1E), indicating Wdr1 KO embryos was lost during embryonic development, consistent with a previous report in which severe loss function of WDR1 resulted in embryonic lethality before E10.5 (27). Thus, these results suggested that zygotic, but not maternal, expression of Wdr1 is required for mouse development.
WDR1 Is Essential for Mouse Peri-implantation Development-To examine the causes and time point of Wdr1 KO embryo lethality, Wdr1 f/f ; Zp3-cre and Wdr1 f/f female mice mated with Wdr1 f/Ϫ male mice and the deciduas were analyzed at E5.5. Our results showed that the number of deciduas per litter was 7-10 in both groups and were not obviously different from each other ( Fig. 2A). However, after sectioning and H&E staining of these deciduas, 53% of the deciduas from Wdr1 f/f ; Zp3-cre females had normal embryos ( Fig. 2B (a)), and 47% had no embryos ( Fig. 2B (b)), whereas the percentage of empty deciduas from Wdr1 f/f females (control) was only 3% (Fig. 2B, right panel). These data indicated that the blastocysts lacking WDR1 were able to implant and induce the decidualization, but were absorbed at E5.5, suggesting that WDR1 is essential for mouse peri-implantation development.
To further investigate Wdr1 KO embryonic development, blastocysts were obtained from the uteruses of the Wdr1 f/f ; Zp3-cre females after mating with Wdr1 f/Ϫ males at E3.5 and cultured in vitro. KO and control blastocysts could not be distinguished at E3.5 (Fig. 2C). All blastocysts grew, hatched, and adhered to the dish during the first 2 days of culturing. However, 55% (11 of 20) of embryos grew obviously smaller at the third day. No EdU incorporation was detected in the smaller embryos (Fig. 2D). We then examined the genotypes of these embryos by PCR with specific primers and found that the genotype of 81% (9 of 11) of the smaller embryos were Wdr1 Ϫ/Ϫ (Fig. 2E). These data suggest loss of WDR1 has no obvious effect on blastocyst development, but cause the arrested development after adherence in vitro.
Wdr1 Knock-out Decreases Cofilin Phosphorylation in Mouse ES Cells-To investigate WDR1 functions in early embryos, we established ES cell lines from Wdr1 f/Ϫ (control, CTL) and Wdr1 Ϫ/Ϫ (knock-out, KO) blastocysts from Wdr1 f/f ; Zp3-cre females after mating with Wdr1 f/Ϫ males. The Wdr1 mRNA and protein deletion were examined by real-time RT-PCR and Western blotting analysis in these ES cell lines (Fig. 3, A and B). Wdr1 KO ES cells could be normally maintained in a 2i/leukemia inhibitory factor (LIF) medium and form typical clones (Fig. 3D). The expression of pluripotent markers such as NANOG, OCT4, and SOX2, and the cells proliferation were comparable in CTL and KO ES (Fig. 3, B and C).
To investigate their differentiation potentials, CTL and KO ES cells were labeled with EGFP and injected into normal blastocysts. These blastocysts were cultured for 3 days in an in vitro system of growing whole embryos. Our results showed that both CTL and KO ES cells incorporated into the cultured embryos detected by EGFP (Fig. 3D). The defect of Wdr1 disruption on differentiation was further examined by embryoid bodies (EB) formation system, a model of ESC differentiation into germ layer lineages. Compared with their expressions at day 0 (d0), germ layer makers (Sox17, endoderm; T, mesoderm; Pax6, ectoderm) were comparably up-regulated in both CTL and KO EB at day 3 (d3) (Fig. 3E). These results indicate that WDR1 depletion may not affect the ES cells potential of differentiation.
Previous reports showed that WDR1 partial dysfunction (decreased to 20%) affected actin structure and depolarized Cofilin localization in migrating cells (27). Then, we examined F-actin and Cofilin in Wdr1 KO ES cells by immunofluorescence. F-actin (red) was concentrated in the membrane in both knock-out ES cells and controls (Fig. 3F). The detailed actin structure could not be observed clearly in these cells. Surprisingly, different from WDR1 dysfunction in migrating cells (27), Cofilin was more concentrated to the membrane and co-located with actin filaments in Wdr1 Ϫ/Ϫ ES cells, whereas it was more diffused in control (Fig. 3F). We also investigated phosphorylated Cofilin (P-Cofilin) by Western blotting analysis. Our results showed that the P-Cofilin level was much lower in Wdr1 Ϫ/Ϫ ES cells than that in control (Fig. 3G). Then, we separated G-actin and F-actin from KO and control ES cells (35). Distinct from a previous report in Wdr1 knockdown cells (36), F-actin level was not obviously increased in Wdr1 KO ES cells as compared with the control (Fig. 3H). Altogether, Wdr1 KO has no obvious impact on ES pluripotency and growth, but results in dramatically decreased P-Cofilin in these cells.

WDR1 Regulates the Phosphorylation of Cofilin and Controls F-actin in Mouse Embryonic Fibroblast (MEF) Cells-Interest-
ingly, WDR1 expression is much higher in MEF cells than that in ES cells (Fig. 4A). To further investigate the effects of WDR1 on actin cytoskeleton, knock-out MEF cell lines were established by a tamoxifen induction system. Wdr1 f/Ϫ ; Cre-ER TM fetuses were used to establish inducible knock-out (iKO) MEF FIGURE 2. Wdr1 KO embryos in peri-implantation development. A, after mating with Wdr1 f/Ϫ males, oocyte specific knock-out females were injected with Chicago blue. Then, the uteruses were picked up at E5.5 and imaged by differential interference contrast. Scale bar, 5 mm. B, deciduas with embryos from A were frozen and sectioned (8 m). The sections were stained by H&E and imaged. Two types such as (a) and (b) were observed. The percentage of the two types was counted from three pregnant females. Statistical results are represented as mean Ϯ S.D. Scale bar, 50 m. C, oocyte-specific Wdr1 KO females were mated with Wdr1 f/Ϫ males. At E3.5, blastocysts were flushed from the uterus and imaged by differential interference contrast. Scale bar, 40 m. D, blastocysts obtained from C were cultured in vitro for 3 days and treated with EdU for 2 h before being fixed. The outgrowth was stained for EdU (red) according to the protocol provided by the manufacturer. Nuclear DNA was stained by Hoechst 33342 (blue). Scale bar, 200 m. E, Wdr1 f/Ϫ (control, CTL) and Wdr1 Ϫ/Ϫ (knock-out, KO) embryos were genotyped with specific primers.
lines, using Wdr1 ϩ/Ϫ ; Cre-ER TM MEF cells as the control (CTL). After 72 h treatment with tamoxifen, Wdr1 mRNA and protein were decreased to 0.3 Ϯ 0.018% and 4.5 Ϯ 0.2%, respectively, compared with control (CTL) (Fig. 4, B and C). Actin plaques were observed in Wdr1 iKO MEF cells, whereas the clear linear F-actin structure was shown in the control (Fig. 4D). However, we did not detect a significant increase in the overall F-actin level in Wdr1 iKO MEF cells (Fig. 4E). P-Cofilin was observed to be dramatically decreased in Wdr1 iKO MEF cells (Fig.  4F). We also examined the cell cycle by flow cytometry. Our results showed that control MEF cells had complete G 1 , S, and G 2 cell stages, whereas Wdr1 iKO MEF cells lost S stage and expanded G2 stage (Fig. 4G). These data suggested that the WDR1 loss affected MEF cell proliferation. Altogether, our results indicate that WDR1 regulates the formation of special actin plaques, the proliferation, and Cofilin phosphorylation in MEF cells.

WDR1 Regulates Phosphorylation of Cofilin in a Dose-independent Manner-The dramatically decreased P-Cofilin in
Wdr1 KO cells was inconsistent with a previous report for Wdr1 knockdown cells (36), suggesting WDR1 might be overdosed in cells to regulate Cofilin phosphorylation. To test this hypothesis, we used the tamoxifen induction system to gradually reduce WDR1 content and examined the level of P-Cofilin during this process. WDR1, P-Cofilin, and Cofilin were detected in Wdr1 f/Ϫ ; Cre-ER TM and control MEF cells after 0, 24, 48, and 72 h tamoxifen treatments. In Wdr1 f/Ϫ ; Cre-ER TM MEF cells, WDR1 protein gradually reduced at the time course manner and almost failed to be detected at 72 h (Fig. 5A). Although the protein levels of WDR1 were obviously decreased at 24 and 48 h, P-Cofilin was comparable with the control at these time points. The decreased P-Cofilin was only clearly observed at 72 h after tamoxifen treatment (Fig. 5A). Consis- tently, the actin plaques were obviously observed at 72 h, but could not be found at 24 h and only a small number of actin plaques were observed at 48 h (Fig. 5B). These results suggest that WDR1 regulating Cofilin phosphorylation is overdosed in cells.
To further examine the regulation of WDR1 on Cofilin phosphorylation, WDR1 was overexpressed in both ES and MEF cells. Cofilin phosphorylation was not obviously different in both WDR1 overexpressed and control cells (Fig. 5, C and D). When WDR1 was re-expressed in knock-out ES cells, P-Cofilin was obviously increased and comparable with the control (Fig. 5E).
WDR1 Regulates Cofilin Phosphorylation via LIMK1-To investigate how WDR1 regulates Cofilin phosphorylation, WDR1 with a FLAG tag was overexpressed in MEF cells and an immunoprecipitation (IP) experiment was performed with FLAG antibody. Our results showed that WDR1 precipitated LIMK1, but not SSH1, PDXP, or TESK1 (Fig. 6A). We further docked the binding domains of LIMK1 in 293T cells (Fig. 6B). Our results showed that LIMK1-FL and LIMK1-415, but not LIMK1-766, pulled down WDR1 (Fig. 6B). We also examined the levels of P-LIMK1 and total LIMK1 in control and Wdr1 KO MEF cells. Our results showed that both P-LIMK1 and total LIMK1 levels were almost similar in control and KO MEF cells (Fig. 6C).
Previous reports showed that LIMK1 activity was inhibited by binding with BMP-RII (bone morphogenetic proteins receptor II) or microtubules (21,37,38). Because the LIMK1 antibody did not work well for immunostaining, LIMK1 with the Myc tag was overexpressed in control and Wdr1 KO MEF cells to examine whether WDR1 regulates LIMK1 by changing its localization. Our results showed that LIMK1 was diffused in both control and KO MEF cells, but was more concentrated to microtubules in Wdr1 KO MEF cells. We then treated the MEF cells to lightly damage the microtubule structure with a small dosage of nocodazol (1.25 g/ml), a microtubules depolymerization reagent, and examined P-Cofilin by Western blotting analysis in these cells. Our results showed that P-Cofilin was up-regulated in Wdr1 KO MEF cells, but was virtually unchanged in the controls (Fig. 6E). Our IP experiment showed that WDR1 interacts with the PDZ domain of LIMK1, which is a microtubule binding domain (17). Thus, we concluded that WDR1 might regulate LIMK1 function by inhibiting its binding to microtubules.

Lacking of WDR1 Decreases Cofilin Phosphorylation and Disturbs Actin Structure in Both Mouse Blastocyst Outgrowth and
Oocytes-To examine effects of WDR1 loss on F-actin and Cofilin phosphorylation during embryonic development, the blastocysts cultured in vitro for 3 days were stained by phalloidin. Actin filaments were orderly and homogeneous in the control (CTL), whereas random actin plaques were observed in Wdr1 Ϫ/Ϫ (knock-out, KO) blastocyst outgrowth (Fig. 7A). The P-Cofilin level in KO outgrowth was much lower than that in control (Fig. 7B). F-actin and P-Cofilin were also examined in mouse GV oocytes by staining and Western blotting analysis. Our results showed that actin was concentrated to some small plaques in the cytoplasm of Wdr1 Ϫ/Ϫ (oKO) GV oocytes (Fig.  7C, arrowheads), and uniformly distributed in Wdr1 f/f (CTL) (Fig. 7C). P-Cofilin was also dramatically decreased in Wdr1 Ϫ/Ϫ GV oocytes compared with the control (Fig. 7D).

Discussion
WDR1 and its involvement in actin cytoskeleton play important roles in multiple processes during mouse development (27,30,31). However, the role of WDR1 in mouse early embryogen- esis is still largely unknown. In the present study, we showed that depletion of Wdr1 in oocytes by Zp3-cre has no impact on ovulation and pre-implantation embryogenesis, and the oocyte-specific KO females deliver offspring comparable with the controls when they are mated with wild type males. Furthermore, Wdr1 KO ES cells can be established and have no obvious defects in pluripotency and proliferation. Mouse embryos depleted with zygotic Wdr1 are lost at a very early stage of development at E5.5, although these embryos can implant and induce decidualization. Consistently, Wdr1 KO blastocysts can hatch and adhere, but have impaired outgrowth and cannot be labeled with EdU, accompanying the severe defects of actin cytoskeleton. Wdr1 KO MEF cells have growth defects such as losing S phase and abnormal actin plaques, similar to the phenotypes observed in Wdr1-specific KO cardiomyocytes and sertoli cells (30,31). For successful development, mouse trophoblast cells dramatically differentiate and proliferate, accompanying tremendous changes in cytoskeleton after implantation (39,40). Although the exact reason that WDR1 loss of function results in the embryonic arrest at E5.5 is unclear, the role of WDR1 in actin cytoskeleton might be critical in the differentiation and growth of trophoblast cells. Thus, the function of WDR1 regulating actin disassembly might be a cell-type specific manner for cell proliferation and survival.
Taken together, our results demonstrate that WDR1 plays essential roles in mouse peri-implantation development.
Cofilin is important for spatial and temporal regulation of F-actin dynamics in cells and its activity is tightly controlled by several mechanisms (7,41,42). However, which mechanism is the most important process for Cofilin severing activity is still unclear. Cofilin binding and severing F-actin activity is dependent upon its phosphorylation, which is tightly regulated by the protein kinases and phosphatases in vivo, such as LIMK and SSH (15,42). In response to the stimuli, the kinases phosphorylate, whereas the phosphatases dephosphorylate Cofilin to control its interaction with actin for optimal severing activity to regulate the dynamics of actin cytoskeleton (14,44). In addition, some small molecules or actin-binding protein ligands can competitively displace Cofilin to decrease the binding density of this protein on F-actin into a range that favors severing activity (43,44). These results suggest that the regulation of Cofilin binding to F-actin is controlled by multiple mechanisms and might be the primary process for Cofilin severing activity in vivo.
Most studies have shown that WDR1 significantly accelerated Cofilin dissembling of actin cytoskeleton. However, how WDR1 regulates Cofilin severing activity remains obscure. In the current study, we established Wdr1 KO ES, MEF cells, oocytes, and early embryos to investigate the regulation of WDR1 on Cofilin. Unexpectedly, we found that loss of WDR1 down-regulates P-Cofilin in all examined cells. Consistent with this, a very recent report showed that P-Cofilin is decreased in the cells of some patients with Wdr1 mutation (45). Interestingly, WDR1 seems to be present in an excessive amount in the cells, which well explains the discrepancies of Cofilin phosphorylation levels observed in knockdown and KO cells (36). We also found that WDR1 interacts with the LIMK1 PDZ region, which was reported to bind to microtubule (17). In addition, LIMK1 is concentrated to the microtubules in Wdr1 KO MEF cells and the disassembly of microtubules can partly rescue the phosphorylated Cofilin in these cells. Previous reports show that the PDZ domain is a cytoskeleton binding domain and the PDZ domain can localize LIMK1 to the microtubules (21,37,38). Thus, these results suggest that WDR1 might inhibit the binding of LIMK1 to microtubules and release LIMK1 to the cytoplasm to catalyze Cofilin phosphorylation, therefore regulating the binding of F-actin to Cofilin.
Previous results show that WDR1 can bind to Cofilin-actin and induces F-actin structural changes to accelerate Cofilin severing F-actin activity (9). In addition, another report shows that WDR1 might simply compete with Cofilin and dissociate redundant Cofilin from F-actin to accelerate severing activity (44). Furthermore, this regulation of Cofilin severing activity is dependent on the pH (46). In our study, we found WDR1 regulated Cofilin phosphorylation through LIMK1 to control the binding of Cofilin with actin filaments. Thus, WDR1 regulates Cofilin severing F-actin activity at multiple layers, suggesting the interrelationship of WDR1 and Cofilin is very complex in vivo.
It is worth mentioning that WDR1 depletion decreases the level of Cofilin phosphorylation and disrupts the actin structure in mouse oocytes, but does not affect oocyte maturation and fertilization. Similar observations are also reported in some other cytoskeleton relative proteins in mouse oocytes (47). These results indicate mouse oocytes and very early embryos might have tolerance to some level of actin deficiency. Taking together, our results demonstrate that WDR1 is essential for FIGURE 6. WDR1 regulates Cofilin phosphorylation through LIMK1. A, the control and WDR1 overexpressed MEF cells were immunoprecipitated with anti-FLAG antibody. LIMK1, SSH1, PDXP, and TESK1 were detected by immunoblot in the precipitation products with the specific antibodies. B, P-LIMK1 and total-LIMK1 were examined by immunoblot in control and WDR1 knock-out MEF cells. C, WDR1 with a Myc tag was co-expressed with LIMK1-FL (full-length), LIMK1-415 (expressed from 415 bases), and LIMK1-766 (expressed from 766 bases) with HA tag, respectively. Lysates were immunoprecipitated with anti-HA antibody. The immunoprecipitated products were analyzed by Western blotting with antibodies to LIMK1 and Myc tag. D, LIMK1 with a Myc tag was overexpressed in both CTL and Wdr1 iKO MEF cells. LIMK1 and microtubules were stained by antibodies to Myc tag (green) and ␣-tubulin (red). Scale bar, 20 m. E, control and knock-out MEF cells were treated with 1.25 g/ml of nocodazol for 5 min. Then, P-Cofilin, total-Cofilin, and WDR1 in the cell lysates were detected by immunoblot. GAPDH was used as a loading control. mouse peri-implantation development and regulates Cofilin phosphorylation through LIMK1 to optimize its F-actin severing activity in vivo.

Experimental Procedures
Mice Maintenance-In compliance with the guidelines of the Animal Care and Use Committee of the Institute of Zoology at the Chinese Academy of Sciences, the Wdr1 f/f ; Zp3-cre and Wdr1 f/f ; Cre-ER TM mouse lines were maintained on a mixed background (129/C57BL/6). A pair of Flox sequences was inserted in both ends of the fourth exon of Wdr1 to establish Wdr1 f/f mice as previously described (31). Zp3-cre mice (48) were mated with Wdr1 f/f mice to obtain the oocyte-specific Wdr1 knock-out females. To establish Wdr1 inducible knockout MEF cell lines, Wdr1 f/Ϫ mice were mated with Cre-ER TM transgenic mice (49) to obtain Wdr1 ϩ/Ϫ ; Cre-ER TM offspring. E13.5 fetuses from the mating of Wdr1 ϩ/Ϫ ; Cre-ER TM females with Wdr1 fϪ males were used to derive the MEF cells. All mice were maintained in SPF animal houses with a 12-h light/12-h dark cycle. Mouse tail tip or cells were lysed by an alkaline lysate buffer at 95°C for 1 h. Then genotyping PCR was conducted with specific primers (Table 1).
Collection and Culture of Mouse Eggs and Embryos-GV oocytes were collected using M199 medium from ovaries. After female mice were stimulated by injecting PMSG and hCG (Ningbo Second Hormone Factory), metaphase II (MII) oocytes were collected in M2 medium from oviducts after hCG 13 h; 1-cell, 2-cell embryos, and morulas were flushed from oviducts at E0.5, E1.5, and E2.5 days; and blastocysts were collected from uteruses at E3.5. Blastocysts were cultured in 1066 medium supplemented with 10% FBS, 1 M sodium pyruvate, 2 M L-glutamine, and 50 g/ml of penicillin/streptomycin at 37°C in 5% CO 2 (50,51). The culture dishes for blastocysts were pre-treated with 0.2% gelatin. For the E5.5 embryos section, the deciduas were frozen at Ϫ80°C.
Cell Culturing-Wdr1 inducible knock-out MEF cell lines were derived from Wdr1 F/Ϫ ; Cre-ER TM fetuses at E13.5 and Wdr1 ϩ/Ϫ ; Cre-ER TM fetuses as the control. Tamoxifen was added to the medium to induce the Wdr1 knock-out. The 293T cell line was cultured in DMEM with 10% FBS.
Wdr1 knock-out ES cell lines were established from Wdr1 Ϫ/Ϫ blastocysts as in a previous report (52), Wdr1 f/Ϫ ES cells were used as control. Briefly, blastocysts were cultured in 0.2% gelatin-pretreated dishes in N2B27 medium supplemented with PD0325901 (1 M, catalogue number P-9688, LC Laboratories), CHIR99021 (3 M, catalogue number C-6556, LC Laboratories), and LIF (1000 units/ml, catalogue number ESG1107, Millipore) (2i/LIF medium) for 5 days. Then, the inner cell mass clones were digested by trypsin substitution and planted onto MEF cell feeders in 2i/LIF medium or DMEM containing 15% fetal bovine serum, 2 mM sodium pyruvate, 2 mM L-glutamine, 0.1 mM nonessential amino acids, 50 g/ml of penicillin/streptomycin, 0.1 mM ␤-mercaptoethanol, and 10 ng/ml of LIF (ES serum medium). For cell number counting, ES cells cultured on gelatin were digested to single cells and counted in a blood counting chamber. All cell lines were cultured at 37°C in 5% CO 2.
ES Cell Differentiation-ES cells were labeled with EGFP, digested to single cells, resuspended in DMEM with 15% FBS, and kept on ice. Blastocysts were collected from the uterus of E3.5 superovulated ICR females. 10 -15 ES cells were picked up and injected into one blastocyst cavity by an injection pipette. The injected blastocysts were cultured in gelatin-pretreated dishes for 3 days. ES cells in the chimeras were detected by fluorescence confocal microscopy. For EB formation, ES cells were digested to single cells and cultured by seeding 600 cells in one 30-l hanging droplet of ES serum medium without LIF.
Real-time RT-PCR-Total RNA was extracted from cells with the RNAzol RT RNA Isolation Reagent (Molecular Research Center) and isolated from oocytes and pre-implantation embryos with the Dynabeads mRNA Direct Micro Kit (Ambion). The RNA was then reversely transcripted with the PrimeScript TM RT-PCR kit (Takara). The primer sequences were listed in Table 1. Real-time PCR was carried out in the All-In-One RT Master Mix G490 system (Applied Biological Materials). GAPDH was used as a reference gene for normalization of the mRNA levels. Data were processed using the 2 Ϫ⌬⌬Ct method.
Plasmid Construction and Lentivirus Transfection-293FT cells were transfected with the envelope plasmid pMD2G, packaging plasmid psPAX2, and core expression plasmid pHIV-EGFP (Addgene) by PEI. After culturing for 48 and 72 h, the lentivirus supernatant was collected and concentrated through ultracentrifugation at 17,000 rpm for 2 h. For transfection, MEF or ES cells were incubated with lentivirus for 12 h and then cultured with regular medium. For protein expression in 293FT cells, genes were linked to HA-pCMV or Myc-pCMV vector. Wdr1 was added at the FLAG sequence in the forward primer, and linked to pHIV-EGFP through XbaI and SmaI sites. Full-length Limk1, Limk1-415 (deleted two Lim domains), and Limk1-766 (deleted two Lim domains and PDZ domain) were added by the respective forward primer and a common reverse primer, and then linked to pCMV-HA vector through forward sites SalI, BglII, and EcoRI and reverse site NotI. Wdr1 was linked to pCMV-Myc vector through XhoI and NotI sites. The primer sequences for vector construction are listed in Table 1.
Immunoblots and Immunoprecipitation-Samples for IP were lysed by IP/Western lysis buffer (Byotime) with protease inhibitor mixture (Roche Applied Science) and 5 mM NaF. For IP, 5% of the lysates served as input and the rest were incubated with mouse anti-FLAG antibody (1:500, Abmart) or mouse anti-HA antibody (1:500, Abmart) and protein G-agarose (Santa Cruz) at 4°C for 5 h. These samples were diluted with a SDS loading buffer, heated at 95°C for protein denaturalization, and then analyzed by Western blotting. Oocytes, embryos, and cells samples for Western blotting were also lysed and denaturalized by the same buffers.
Samples for immunoblots were separated by 10% SDS-PAGE and transferred to PVDF membranes (Invitrogen). The PVDF membranes were blocked with 5% skim milk and incubated with the primary antibody at 4°C overnight. After being washed three times with PBS supplemented with 0.1% Tween 20, the PVDF membranes were incubated with HRP-conju-  , and mouse anti-HA (1:500 for IP, catalogue number M20003, Abmart). The second antibodies included: goat anti-rabbit, goat anti-mouse, and rabbit antigoat, which were conjugated with HRP (1:4,500, Abmart).
G-actin and F-actin Separation-G-actin and F-actin were separated by a two-step extract and ultracentrifugation protocol. The samples from the separated G-actin and F-actin fractions were proportionally loaded and analyzed by Western blotting using an antibody to pan-actin. G-actin was extracted by a cold lysis buffer 1 (10 mM K 2 HPO 4 , 100 mM NaF, 50 mM KCl, 2 mM MgCl 2 , 1 mM EGTA, 0.2 mM DTT, 0.5% Triton X-100, 1 mM sucrose, pH 7.0) and centrifuged at 15,000 ϫ g for 30 min. Soluble actin (G-actin) was measured in the supernatant. F-actin in the pellet was resuspended in lysis buffer plus an equal volume of buffer 2 (1.5 mM guanidine hydrochloride, 1 mM sodium acetate, 1 mM CaCl 2 , 1 mM ATP, and 20 mM Tris-HCl, pH 7.5) and incubated on ice for 1 h to convert F-actin into soluble G-actin, with gentle mixing every 15 min. The samples were centrifuged at 15,000 ϫ g for 30 min, and F-actin was measured in this supernatant (35).
EdU and PI Staining-Embryos were incubated with 500 M EdU for 2 h and then fixed with 4% paraformaldehyde. Detection of incorporated EdU was performed using the Cell-Light EdU Apollo 567 In Vitro Imaging Kit (RiboBio) according to the manufacturer's protocol.
For cell cycle detecting, MEF cells were digested to single cells and fixed by 70% ethanol at Ϫ20°C overnight. Cells were permeabilized in PBS containing 0.5% Triton X-100 at room temperature for 30 min and then stained by propidium iodide (PI) in PBS at 4°C for 30 min. PI signals were detected by flow cytometry and the results were analyzed by Flowjo software (Tree Star).
Immunohistochemistry-Cells or blastocysts were fixed by 4% paraformaldehyde in PBS at room temperature for 10 min and permeabilized in PBS containing 0.5% Triton X-100. Cells and embryos were blocked by 5% normal donkey serum at room temperature for 1 h and then incubated in primary antibodies at 4°C overnight. After being washed with PBS three times to remove unconjugated primary antibodies, second antibodies, Hoechst 33342 (Invitrogen) and Alexa Fluor 546-labeled phalloidin (Invitrogen), were added and incubated at room temperature for 1 h. For Myc-Limk1 staining, MEF cells were fixed by 0.1% glutaraldehyde, 0.1 M sodium cacodylate, pH 7.3. For GV oocyte F-actin staining, oocytes were fixed with 130 mM KCl, 25 mM HEPES, pH 7.0, 3 mM MgCl 2 , 4% paraformaldehyde, 0.15% glutaraldehyde, and 0.06% Triton X-100 at room temperature for 2 h and permeabilization was extended to 30 min.
Statistical Analyses-Quantitative analyses were carried out with GraphPad Prism software with at least 3 independent biological samples and expressed as the mean Ϯ S.D. p values of comparisons between 2 groups were calculated using Student's t test. p Ͻ0.05 was considered as significant.
Author Contributions-Y. X. designed and performed major experiments, analyzed the data, and wrote the manuscript. H. M. conducted Limk1 overexpression experiments. W. P. established the Wdr1 f/f mouse line. D. Q. harvested GV oocytes and stained F-actin structure. X. W., Z. X., Y-L. X., and W. L. established MEF cell lines, injected ES cells into blastocysts, and performed H&E staining of embryo sections. L. L., Y. Z., and C. J. initiated and organized this project, analyzed the data, and wrote the manuscript. All authors commented on the manuscript.