Figures
Abstract
The Pik3c3 gene encodes an 887 amino acid lipid kinase, phosphoinositide-3-kinase class 3 (PIK3C3). PIK3C3 is known to regulate various intracellular membrane trafficking events. However, little is known about its functions during early embryogenesis in mammals. To investigate the function of PIK3C3 in vivo, we generated Pik3c3 null mice. We show here that Pik3c3 heterozygous are normal and fertile. In contrast, Pik3c3 homozygous mutants are embryonic lethal and die between E7.5 and E8.5 of embryogenesis. Mutant embryos are poorly developed with no evidence of mesoderm formation, and suffer from severely reduced cell proliferations. Cell proliferation defect is also evident in vitro, where mutant blastocysts in culture fail to give rise to typical colonies formed by inner cell mass. Electron microscopic analysis revealed that epiblast cells in mutant embryos appear normal, whereas the visceral endoderm cells contain larger vesicles inside the lipid droplets. Finally, we provide evidence that mTOR signaling is drastically reduced in Pik3c3 null embryos, which could be a major contributor to the observed proliferation and embryogenesis defects.
Citation: Zhou X, Takatoh J, Wang F (2011) The Mammalian Class 3 PI3K (PIK3C3) Is Required for Early Embryogenesis and Cell Proliferation. PLoS ONE 6(1): e16358. https://doi.org/10.1371/journal.pone.0016358
Editor: Madhuri Kango-Singh, University of Dayton, United States of America
Received: August 19, 2010; Accepted: December 22, 2010; Published: January 20, 2011
Copyright: © 2011 Zhou et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: This work is supported by the McKnight Scholar Award and the Wings for Life Foundation to F.W. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Introduction
In mammals, there are three classes of phosphoinositide-3-kinases (PI3Ks). Most of the previous studies on the in vivo role of PI3Ks focused on class I PI3Ks, which were shown to be required for early embryonic development [1], [2], [3]. However, the role of the class III PI3K, PIK3C3 (also called Vps34), during mammalian development is not known. PIK3C3/Vps34 represents the most ancient form of PI3Ks and is the only PI3K in yeast [4]. Previous studies have shown that PIK3C3 regulates several membrane trafficking events including homotypical fusion between early endosomes [5], [6], [7], bi-directional transportation of early endosomes along the microtubules [8], [9], maturation of endosomes or phagosomes [10], [11], [12], [13], biogenesis of multivesicular bodies [14], [15] and retrograde transportation from endosomes to the Golgi apparatus [16], [17]. PIK3C3 is also critical for the formation of pre-autophagosomes which are important for degradation of large protein aggregates and organelles [18], [19], [20], [21], [22]. Finally, PIK3C3 is shown to be required for nutrient/amino acid mediated activation of mTOR signaling in cultured cells [23], [24], [25], [26].
Deletion phenotypes of Pik3c3/vps34 have been analyzed in several yeast and invertebrate organisms. In Saccharomyces cerevisiae, mutation in the Vps34 gene results in mis-sorting and secretion of Golgi-modified precursor forms of several vacuolar hydrolases [27]. It also results in temperature-sensitive growth defects, osmo-regulation defects, vacuole segregation defects during mitosis [28], as well as a disruption of macroautophagy [20]. In Caenorhabditis elegans, Pik3c3 mutation arrests worm development at the L3-L4 molt [29]. In Drosophila melanogaster, deletion of Pik3c3 gene causes hemizygous larval lethality, failure in autophagosome formation and defective endocytosis in fat body cells. However, TOR signaling is not affected in Pik3c3 mutant flies [30]. In mice, conditional knockout of Pik3c3 in postmitotic sensory neurons results in fast and differential neurodegeneration caused by a severe disruption of the endosomal pathway [31], [32].
Here, we generated a null allele of Pik3c3 in mouse. We found that homozygous mutant embryos are poorly developed, die at the beginning of gastrulation, and show significantly reduced cell proliferation rate both in vivo and in vitro. We also examined the ultrastructure and mTOR signaling in Pik3c3 mutant embryos. Our study provides new insights into the importance of PI3KC3 for normal cell proliferation and embryogenesis.
Results
Generation of Pik3c3 knockout mice
We first examined the expression pattern of the Pik3c3 gene in early embryos. Previous studies have shown that Pik3c3 mRNA is universally expressed in all types of tissues in mammals [33]. Consistent with this, our in situ hybridization shows ubiquitous expression of Pik3c3 in all cells of the developing embryos (Figure 1A1). Our lab previously generated a conditional allele of Pik3c3 in which the ATP binding domain of the kinase is flanked by two LoxP sites (Pik3c3flox/flox mice) and thus can be deleted in the presence of Cre recombinase to result in a functional null allele [31]. We generated heterozygous mice (Pik3c3+/-) by crossing the conditional allele (Pik3c3flox/flox) with Meox-cre transgenic mice in which Cre is expressed in the germ line [34]. The resulting (germline deletion) null allele was subsequently introduced into C57BL/6J mice background through back crossing. Heterozygous Pik3c3+/- mice are fertile, phenotypically comparable to the wild-type controls and can live at least up to 18 month. We observed neither obvious behavioral defects nor spontaneous tumor genesis in heterozygous mice during this period.
A. A1: fluorescence in situ hybridization detected Pik3c3 mRNA expression (red) in embryo at E6.5, counter stained with DAPI (blue). A2: representative PCR genotyping result of one litter at E7.5 from heterozygous intercrosses. The deleted allele produces a 670 bp fragment while the wild type allele produces a 450 bp fragment. A3: genotyping analysis of offspring from heterozygous intercrosses at different embryonic stages. Most mutant embryos are dying after around E7.5. B. Representative wholemount preparation of a heterozygous control (B1) and a homozygous mutant (B2) embryo at E7.5. Genotypes were obtained by PCR. Mutant embryos are smaller than controls. EX: extraembryonic region. EM: embryonic region. Scale bars: A, B: 100 µm.
Early embryonic lethality in Pik3c3 mutation
Pik3c3 homozygous mutants (Pik3c3-/-) were obtained by intercrosses between the heterozygous mice. Of the 64 P0 (postnatal day 0) offsprings from the intercrosses examined, 42 were heterozygous and 22 were wild-type, but no viable Pik3c3-/- pups were ever identified, indicating that homozygosity for the Pik3c3 mutation leads to embryonic lethality. To identify the timing of lethality, embryos at the stages of E7.5, E8.0, E8.5 and E10.5 from heterozygous intercrosses were collected and genotyped by PCR (Figure 1A2). Homozygous embryos with a correct Mendelian ratio were recovered at E7.5 (Figure 1A3). Between E7.5 and E8.5, absorbed debris or empty deciduae were frequently observed and the number of viable homozygous mutants decreased (Figure 1A3). No homozygous mutant embryos were obtained at or after E8.5 (Figure 1A3). The results indicate that PIK3C3 is essential for embryogenesis at the initiation of gastrulation.
Histological analysis of Pik3c3-/- embryos
To examine the phenotypes prior to embryo death, whole embryos were dissected out at E7.5. Heterozygous null embryos and wild-type controls are comparable and equally well developed at this stage (Figure 1B1). However, the homozygous mutant embryos remain the shape of a compact egg and are less than half the size of the wild-type and heterozygous embryos (Figure 1B2). Both embryonic and extra-embryonic regions in mutant embryos are smaller than controls, suggesting abnormal embryogenesis (Figure 1B1 and 1B2). To examine the mutant phenotypes in further detail, we performed H&E staining of serial sagittal sections of E5.5, E6.5 and E7.5 embryos (Figure 2). At E5.5 egg cylinder–stage, the mutant embryos can be readily distinguished by their smaller size (Figure 2A1 and 2A2). At E6.5, control embryos exhibit well-organized visceral endoderm (ve), embryonic ectoderm (ee), a proamniotic cavity (pc) and a forming mesoderm (m) that is more obvious at E7.5. By contrast, mutant E6.5 embryos do not appear to progress much beyond E5.5 (Figure 2A3 2A4 and 2A5; arrows). They contain less identifiable layers of visceral endoderm (ve) and embryonic ectoderm (ee), and are much smaller in size and have much less number of cells compared with controls. Mutant embryos exhibit no detectable primitive streak and some contain a small proamniotic cavity (pc) (Figure 2A3 and 2A4; arrows). At E7.5, mutant embryos grow slightly in size. A layer of cells that appear to be visceral endoderm (ve) can be seen surrounding the embryo, but the rest of the embryos are disorganized and it is difficult to discern any structures (Figure 2A5 and 2A6; arrows). These data indicate that the development of Pik3c3-/- embryos arrests at the beginning of gastrulation.
A. Representative images of Hematoxylin & Eosin (H&E) staining on control and Pik3c3 deleted embryo sections at E5.5, E6.5 and E7.5. Arrows in E6.5 and E7.5 embryo point to ectoplacental cone (epc), extraembryonic ectoderm (eee), embryonic ectoderm (ee), mesoderm (m), proamniotic cavity (pc), visceral endoderm (ve). The mutant embryos are disorganized, smaller in size and have much less number of cells compared with controls. Scale bars: 100 µm.
Pik3c3 mutant embryos lack mesoderm
We next examined the expression of molecular markers for different embryonic layers at E6.5. Visceral endoderm in wild-type embryos expresses transcription factors Hnf4 (hepatocyte nuclear factor-4) [35], [36] and Gata4 [37], [38] (Figure 3A1 and 3A3). Both markers also label a thin layer of cells covering the mutant embryos (Figure 3A2 and 3A4), suggesting that mutant embryos indeed possess visceral endoderm. On the other hand, morphological and histological studies mentioned above implicate a missing mesoderm in mutant embryos. Consistent with this, the transcript factor Brachyury that labels primitive streak at E6.5 in wild-type animals [39] (Figure 3A5) is completely missing in mutant embryos (Figure 3A6). The results further confirm that mutant embryos fail to form mesoderm.
A. Representative images of in situ hybridization of Gata4, Hnf1 and Brachyury in control and Pik3c3 mutant embryo sections at E6.5. Both Gata4 and Hnf1 label visceral endoderms in control and mutant. No Brachyury labeling was observed in mutant embryos. Scale bars: 100 µm.
Pik3c3 mutation causes cell proliferation defects in vivo
The growth defects and reduced cell numbers in Pik3c3 mutant embryos could result from either an excess of programmed cell death or a reduced cell proliferation rate. To distinguish between these two possibilities, we first examined apoptosis. E6.5 control and mutant embryos were serially sectioned and stained with antibody against active Caspase 3 (Figure 4A1 and 4A2). Cells in both control and mutant embryos lack positive Caspase 3 signal (Figure 4A1 and 4A2). The lack of apoptosis is further confirmed by electron microscopic analysis of E6.5 embryos, in which we did not detect any morphological alterations associated with apoptotic cell death, such as condensed and fragmented nuclear chromatin or interrupted nuclear envelope, for either of the genotypes (see below the ultra-structural analyses part). These results suggest that there is no excessive apoptosis occurring in Pik3c3 mutant embryos.
A. Activated caspase 3 immunostaining (green) and BrdU labeling (red) in control and mutant embryos at E6.5. Scale bar: 100 µm. B. Bar graph shows percentage of BrdU positive cells over total number of cells in control and mutant embryos at E6.5. Wild type embryos show an average ratio around 0.7 while mutant embryos show an average ratio around 0.4 (p<0.001).
Next, we examined the effect of the Pik3c3 mutation on cellular proliferation in vivo by BrdU incorporation. BrdU was injected into pregnant females at E6.5 and allowed to label proliferating cells for one hour (Figure 4A3 and 4A4). The ratio of the number of BrdU-positive nuclei to the total number of cells (as indicated by DAPI staining) was calculated to serve as the proliferation index (Figure 4B). Many cells in wild-type embryos were BrdU-positive, producing an average proliferation index of 72.8% (with a standard error of the mean, or SEM, of 2.6%) (Figure 4A3 and 4B). However, the mutant embryos analyzed showed an average index of only 43.1% (with a SEM of 6.7%) (Figure 4A4 and 4B), suggesting a significantly impaired cell proliferation capacity in mutant embryos in vivo. Therefore, reduced proliferation, but not excessive cell death, is likely to account for the small size and retarded growth of Pik3c3 mutant embryos.
Pik3c3 mutation causes cell proliferation defects in vitro
To directly test the growth capacity of mutant Pik3c3 embryos, we performed in vitro blastocysts growth assay. Blastocysts were collected from E3.5 embryos, cultured and imaged in vitro for 8 days followed by genotyping. Initially, all blastocysts have similar appearance, indicating that Pik3c3 mutation does not affect pre-implantation development (Figure 5A1 and 5B1). During the first two days in vitro, both control and mutant blastocysts exhibited substantial trophoblast giant cell outgrowth and inner cell mass growth (Figure 5A2 and 5B2). Subsequently, however, the growth of both trophoblast giant cells and inner cell mass in all mutant blastocysts (n = 6) slowed down significantly compared with controls. In fact, there was very limited increase in cell numbers in the mutant cultures between day 3 and day 8 (Figure 5A3–A6, 5B3–B6). By contrast, the inner cell mass from all control blastocysts (9 heterozygous, 5 wildtype) proliferated substantially and formed big colonies after 8 days of culture. These results suggest that even with nutrients provided in culture, Pik3c3 mutant embryonic cells still proliferate poorly.
A. Representative images of cultured blastocysts from a heterozygous control embryo. Embryos were collected from heterozygous intercrosses at E3.5 and genotyped after cultured in vitro for 8 days. Inner cell mass (ICM) and trophoblast giant cells (TGC) are indicated at Day 8. B. Representative images of cultured blastocysts from a homozygous mutant embryo. Mutant embryos have defects in proliferation.
Ultra-structural analyses of Pik3c3 deficient visceral endoderm and epiblast cells
Since PIK3C3 plays a critical role in the later steps of the endocytic pathway [4], and previous work showed that loss of PIK3C3 function results in an accumulation of enlarged vesicles inside cells [14], [15], [31], we wanted to examine whether loss of Pik3c3 causes similar subcellular defects in embryos. We performed electron microscopy (EM) studies on E6.5 embryos. Figure 6A is a schematic representation of the regions in the embryo where EM images were taken. We first examined visceral endoderm cells, which are responsible for uptaking and transporting nutrient to support the rapid proliferation and growth of the epiblasts during the initiation of gastrulation [40], [41], [42]. In both control and mutant embryos, the visceral endoderm cells surrounding the developing embryos exhibit a well-defined brush border composed of dense apical microvilli (Figure 6A, 6B1-2, 6B4-5; red arrows). No apparent differences were found for these microvilli structures. Inside the visceral endoderm cells, there is a subtle but observable change in the morphological organizations of the internalized lipid droplets. In the control visceral endoderm cells, numerous small clear vesicles can be observed inside the dark lipid droplets (Figure 6B1-2, orange stars mark lipid droplets), with an average diameter of 0.55 um (and a SEM of 0.04 um) (Figure 6C). In mutant embryos, the size of the vesicles inside lipid droplets is significantly increased, with an average diameter of 1.28 um (and a SEM of 0.13 um) (Figure 6B4-5 and 6C), and most of lipid droplets appear only lightly stained with only a few dark-stained spots (Figure 6B4-5; blue arrowheads). These morphological differences suggest the possibility that either the processing or the transportation of internalized lipids and fluids might be subtly altered in mutant embryos. We next examined the epiblast cells which are cells give rise to the embryo (Figure 6A). Epiblasts are in the process of rapid growth and dividing, and they have somewhat irregularly shaped nuclei (Figure 6B3, 6B6; green stars). We found no obvious ultrastructural differences between control and mutant epiblasts (Figure 6B3 and 6B6). This result suggests that there is probably only limited endocytosis going on in the proliferating epiblasts, and thus no overt abnormal endosome structures are observed in these cells.
A. Schematic representation of locations of visceral endoderm cells and epiblasts of E6.5 embryos. Boxed regions show where EM images are taken. Microvilli, lipid droplets and cell nucleus are illustrated. B. Representative EM images of control and mutant embryonic cells at E6.5. B1-2 (control) and B4-5 (mutant) are high magnification EM images of visceral endoderm cells. Microvilli (red arrows) and lipid droplets (orange stars) are indicated. Notice the increases in size of clear vesicles inside the lipid droplets in mutant embryos. Most lipid droplets appear only light stained with only a few dark-stained spots in mutants (blue arrowheads). B3 (control) and B6 (mutant) are high magnification EM images of epiblast cells in embryonic ectoderms. Green stars point to nucleus. No differences in cell morphology or subcellullar organelles were observed in mutant epiblasts. Scale bars: 2 µm. C. Quantification on the diameter of vesicles inside lipid droplets, with scatter plot of both control and mutant embryos. There is a statistically significant increase in vesicle size inside the lipid droplets in mutant embryos (p<0.001).
Reduced mTOR signaling in Pik3c3 mutation embryos
If an endocytic process does not contribute significantly to the proliferating defects of Pik3c3 embryos, what other PIK3C3 regulated processes might cause the failed growth? PIK3C3 has been shown to regulate nutrient sensing and amino acid induced mTOR activation in cultured cells [23], [24], [25], [26]. mTOR mutant embryos show similar early embryonic lethality and defects in cell proliferation as the Pik3c3 mutant mice [43], [44], [45]. On the other hand, growth factor signaling through activation of Akt pathway can also lead to mTOR activation. Thus it is not immediately clear whether mTOR signaling is affected in Pik3c3 mutant embryos. We performed immunostaining of phosphorylated ribosomal protein S6 (phospho-S6), the downstream target of mTOR complex 1 and S6 kinase 1 (S6K1) and also a commonly used indicator for mTOR activation, in E6.5 control and mutant embryos [45]. Strong phospho-S6 staining can be clearly visualized in control embryos (Figure 7A1), indicating a highly active mTOR signaling pathway during early embryogenesis. In contrast, phospho-S6 level is drastically reduced in Pik3c3 mutant embryos (Figure 7A2). This result is consistent with previous findings that during earliest stages of development, the embryo is very much dependent on branched chain amino acids and glucose, rather than growth factors, to activate mTOR signaling for growth [46], [47], [48]. Thus, the loss of mTOR signaling in Pik3c3 mutant embryos could be a major contributor to the observed cell proliferation defects and early embryonic lethality.
A. Immunostaining of phosphor-S6 (red) in control and mutant embryos at E6.5, counter stained with DAPI (blue). Notice the drastically decreased phospho-S6 level in mutant embryos. Scale bar: 100 µm.
Discussion
In the present study, we generated Pik3c3 knockout mice and characterized the in vivo function of PIK3C3 during embryogenesis. The most prominent defect caused by Pik3c3 deletion is a severely reduced embryonic cell proliferation. The death of Pik3c3 mutant embryos prior to gastrulation is likely due to the lack of proliferative burst required for the development of different germ layers. It has been shown that mouse gastrulation occurs at around E6.5 when mesoderm is generated from epiblast [42]. Importantly, there is normally a ∼100-fold increase in cell number between E5.5 and E7.5 [42]. The dramatic increase in cell proliferation is necessary for proper gastrulation since cells need to accumulate to certain numbers to initiate this process [49]. In fact, mutations in genes that affect proliferation rate during this period often result in missing of mesoderm, abnormal embryonic development and early embryonic lethality [39]. For instance, embryos carrying null mutation in genes encoding proteins of the bone morphogenetic protein (BMP) signaling pathway, including Smad4 [50], [51], Bmp4 [52] and Bmpr [53], all fail to develop mesoderm and die at the beginning of gastrulation partly due to defects in cell proliferation. Germline deletion of tumor suppressor genes regulating cellular growth such as Brca1 [39] and Tsg101 [54] also leads to cell proliferation defect, lack of mesoderm and early embryonic lethality before E7.5. Here we show that Pik3c3 mutation leads to significantly retarded cell proliferation both in vivo and in vitro. Interestingly, the blastocysts isolated from E3.5 Pik3c3 mutant embryos appear normal compared with controls and display similar growth and proliferation capability in the first two days in culture. It is possible that persistence of maternal PIK3C3 protein or mRNA may permit cell proliferation and the initial development of blastocysts. Subsequently, as PIK3C3 proteins are gradually depleted, the growth of embryos stops.
Previous studies have established critical roles of PIK3C3 in autophagic and endocytic pathways [4]. Since knockout of genes essential for autophagy, Atg5 or Atg7, results in normal embryonic development and postnatal lethality [55], [56], autophagy alone is unlikely to contribute to the phenotypes observed in Pik3c3 mutant embryos. On the other hand, we found somewhat altered lipid uptake/transportation in visceral endoderm cells in Pik3c3-/- embryos, which could potentially contribute to the significantly reduced proliferation in vivo. Visceral endoderm cells function in nutrient uptake, to support rapid cell proliferations during early development [40]. Amino acids are taken into these cells by transporter proteins, whereas lipids are internalized through endocytosis. In vitro, the endoderm surrounding the inner ectoderm core is also required for the proliferation of inner cell mass [43], [57]. Deletion of several key genes that control visceral endoderm differentiation, including Gata4 [58], [59], Gata6 [60] and Hnf4 [61], all lead to early developmental arrest. Moreover, knockout of the gene encoding the adaptor protein Dab2 which regulates megalin endocytosis in the visceral endoderm cells results in early embryonic lethality and cell proliferation arrest both in vivo and in vitro [62], [63], [64]. EM analysis of Pik3c3 null embryos revealed a mild accumulation of enlarged vesicles inside lipid droplets in mutant visceral endoderm cells. This phenotype is consistent with the role of PIK3C3 in regulating late steps of endocytic pathway [14], [15], [31]. This ultrastructural change is specific to visceral endoderm cells but not to cells inside the embryo proper, in agreement with the fact that endocytosis is particularly active in visceral endoderm cells. However, further experiments are needed to test whether the subtly altered vesicle sizes in lipid droplets indeed affect lipid transportation into the embryo proper.
Finally, our study also provides in vivo evidence that mTOR signaling is significantly reduced in Pik3c3 mutant embryos. Two distinct mTOR signaling complexes exist in mammals [65]. The complex 1 contains mTOR, raptor and other proteins, and is activated by nutrients. The complex 2 contains mTOR, rictor and other components, and is activated by the growth factor mediated Akt/PKB pathway [65]. Interestingly, knockout of genes encoding mTOR or the complex 1 component raptor causes a cell proliferation defect and early embryonic lethality at E6.5, a phenotype closely resembles that in Pik3c3 knockout mice [43], [44], [45]. By contrast, deletion of the gene encoding the complex 2 component rictor only results in death at a much later developmental stage [45]. These results suggest that mTOR is primarily activated by the nutrient pathway in early embryos, consistent with the fact that branched amino acid chains support early embryonic growth [46], [47], [48]. Importantly, recent cell culture studies revealed a critical role of PIK3C3 in nutrient sensing and activation of mTOR complex 1 pathway. It has been shown that amino acids can induce a rise in intracellular Ca2+ that activates a direct binding of calmodulin to PIK3C3 [23]. This binding activates the lipid kinase activity of PIK3C3, which is required for the activation of mTOR complex 1 and the subsequent activation of S6K1 [24], [26]. Our study now provides the in vivo evidence that amino acid activated mTOR signaling is indeed drastically reduced in Pik3c3 mutant embryos. This finding also suggests that the cell proliferation defects and failed embryogenesis in Pik3c3 mutant is at least partially due to the loss of mTOR signaling.
Materials and Methods
Generation of Pik3c3-KO Mice
Mice heterozygous for the conditional allele (Pik3c3flox/+) [31], [32] were bred with mice expressing a Meox-cre transgene with cre expressed in the germ line to generate Pik3c3+/− animals. Note that in some cases, Meox-Cre gave rise to incomplete (mosaic) deletion of the Pik3c3flox allele, so the offsprings are further back crossed with C57/B6 mice to obtain Pik3c3+/- heterozygous mice on the C57/B6 background. Homozygous mutant mice (Pik3c3-/-) were obtained by heterozygous intercrosses. PCR based strategies were used for genotyping and the following PCR primers were used to detect Pik3c3- (deleted) allele: L1, 5′- AACTGGATCTGGGCCTATG-3′; L2 5′-GAAGCCTGGAACGAGAAGAG-3′; L3, 5′-CACTCACCTGCTGTGAAATG-3′. The deleted allele produces a 670 bp fragment while the wild type allele produces a 450 bp fragment. All experiments were conducted according to protocol #A267-09-09, approved by the Duke University Institutional Animal Care and Use Committee.
Blastocyst Cultures and Genotyping
Embryonic stage (days postcoitum) was estimated by timed pregnancy. E3.5 embryos from Pik3c3+/- heterozygous intercrosses were collected by flushing through the uterus of the plugged females. Blastocysts were individually collected with mouth pipettes and cultured in 12-well plates in 5% CO2 incubator at 37°C. Culture medium is the standard embryonic stem cell (ES cell) culture medium without leukemia inhibitory factor (10%FBS, 2 mM L-glutamine, 0.1 mM non essential amino acid, 1 mM sodium pyruvate, 1∶100 penicillin/streptomycin and 50 µM β-mercaptoethanol in 1x GMEM). Photos were taken every 24 hr. After 8 days in vitro, cultured blastocysts were lysised overnight at 55°C in 100 ul of lysis buffer (50 mM KCl, 10 mM Tris (pH 8.3), 2 mM MgCl2, 0.1 mg/ml gelatin, 0.45% NP-40, and 0.45% Tween-20) containing 200 µg/ml proteinase K. Samples were boiled for 10 min afterwards. 1-5 µl of samples were subjected to PCR amplification with 40 cycles to determine the genotypes. A total of 20 blastocysts obtained from two pregnant females were cultured and genotyped, among which 5 were confirmed to be wild-type controls, 9 were heterozygous and 6 were homozygous mutants.
Histological Analyses
Fixation and embedding.
Plugged females at the desired stage were sacrificed. The uteri were removed and the decidual swellings were fixed in 4% paraformaldehyde at 4°C overnight. They were either embedded in OCT, or dehydrated and embedded in paraffin. 16–18 µm sections were cut from OCT embedded samples and 5–7 µm sections were cut from paraffin embedded samples.
In situ hybridization.
In situ probe templates were generated by RT-PCR from embryonic tissues. Specifically, Pik3c3 probe was amplified with 5′-ACCACGATCTCAAACCCAACGCTAC-3′ and 5′-AGGGTAGCTGTTTCCGGGATGATGC-3′; the Brachyury probe which labels mesoderm was amplified with 5′-TGACCAAGAACGGCAGGAG-3′ and 5′-GAACCAGAAGACGAGGACG-3′; the Hnf-4 probe was amplified with 5′-ACACGTCCCCATCTGAAGGTG-3′ and 5′-CTTCCTTCTTCATGCCAGCCC-3′; the Gata-4 probe was amplified with 5′-GGCTGTCATCTCACTATGG-3′ and 5′-TGGGGTGAAGGAGATTATGTG-3′. DIG labeled antisense probes were synthesized by in vitro transcription using T7 RNA-polymerase (Roche) with Digoxigenin (DIG)-UTP (Roche). In situ hybridization was performed according to standard methods. 3 embryos from each group (control or mutant) were used for each molecular marker labeling, and 2 wild-type embryos from each developmental stage (E6.5 or E7.5) were used for in situ hybridization of Pik3c3.
Immunostaining.
The following antibodies were used: rabbit anti-caspase 3 active (R&D Systems, 1∶500), rabbit anti-phospho-S6 ribosomal protein (ser235/236, Cell Signaling, 1∶100), DAPI (Sigma, 1∶5000), Alexa Fluor 488- and 568-conjugated goat anti-rabbit IgG (Invitrogen, 1∶400), Alexa Fluor 568-conjugated goat anti-mouse IgG (Invitrogen, 1∶400). Standard immunofluorescence procedure was used as described before [66]. Briefly, sections were incubated with 1° antibody at 4°C overnight, washed with 1X PBS three times for 10 min each, incubated with 2° antibody at room temperature for 2 hr, and finally washed with 1X PBS three times for 5 min each. 2 to 10 embryos from each group (control or mutant) were used for immunostaining.
H&E staining.
Hematoxylin and eosin staining was performed according to standard protocol. 2–3 embryos from each group (control or mutant) at each different embryonic stage (E5.5, E6.5 or E7.5) were used. Different embryonic structures were identified by location.
BrdU labeling.
Bromo-deoxyuridine (BrdU) labeling reagent (GE Health, 2 ml/100 g) was IP injected into plugged heterozygous female with E6.5 embryos. After one hour, all embryos from the litter were collected, fixed, embedded in paraffin, and sectioned with a microtome. Sections were incubated in 2N HCl at 37°C for 2 hr, treated with 0.05% Trypsin in PBS at room temperature for 2 min, and were finally stained with monoclonal anti-BrdU antibody (Sigma, 1∶500). Embryo boundaries were identified by both BrdU staining and bright field image. The number of BrdU positive cells in embryos on each section was counted and normalized with respect to the total number of cells to yield a proliferation index. N = 7–11 sections from 3 different embryos of the same genotype (control or mutant) were used for quantification and the p-value was calculated using standard Student's t-test.
Electron microscopy
Litters of E6.5 embryos from Pik3c3+/- heterozygous intercrosses were collected and fixed for electron microscopy studies. Tissues were perfused and fixed with 2% paraformadehyde+2.5% glutaraldehyde (Polysciences, Inc) in 0.1M sodium cacodylate buffer pH 7.4 (Electron Microscopy Sciences) for 3 days, washed with PBS, fixed with 1% osmiumtetroxide (Electron Microscopy Sciences)+1.5% potassiumferrocyanide (Electron Microscopy Sciences) in H2O for 2 hr, washed with maleate buffer (Electron Microscopy Sciences), dehydrated in 70%, 90% and 100% ethanol 15 min each, dehydrated again in propyleneoxide (Electron Microscopy Sciences) for 1 hr, infiltrated in 50% Epon (TAAB+DDSA+NMA+DMP-30, Canemco & Marivac)+50% propyleneoxide for 3 hr, all at room temperature. Tissues were eventually embedded in Epon for 2 days at 60°C. Semi-thin and Ultra-thin sections were cut using a Reichert Ultracut S microtome. Semi-thin sections of all embryos were first cut and stained with toluidine blue solution (0.2% toluidine blue O and 1% sodium chloride, pH 2.3) to identify which embryos are mutants and which embryos are controls, and to find the region where the embryo is located. All mutant embryos show similar disorganized and smaller appearance. Subsequently ultra-thin sections were cut and observed with a JEOL 1200 EX transmission electron microscope.
The diameters of all the vesicles inside each lipid droplets in 6–7 randomly selected ecdoderm cells from 2 controls and 2 mutant embryos were measured with Metamorph and the p-value was calculated using standard Student's t-test.
Acknowledgments
We thank M. Gignac for assisting the EM analysis. We thank Dr. Brigid Hogan for many advices on studying and characterizing the development of mouse embryos. We thank the members of the Wang laboratory for technical help as well as useful comments on the manuscript.
Author Contributions
Conceived and designed the experiments: XZ FW. Performed the experiments: XZ JT. Analyzed the data: XZ FW. Wrote the paper: XZ FW.
References
- 1. Bi L, Okabe I, Bernard DJ, Wynshaw-Boris A, Nussbaum RL (1999) Proliferative defect and embryonic lethality in mice homozygous for a deletion in the p110alpha subunit of phosphoinositide 3-kinase. J Biol Chem 274: 10963–10968.
- 2. Bi L, Okabe I, Bernard DJ, Nussbaum RL (2002) Early embryonic lethality in mice deficient in the p110beta catalytic subunit of PI 3-kinase. Mamm Genome 13: 169–172.
- 3. Fruman DA, Mauvais-Jarvis F, Pollard DA, Yballe CM, Brazil D, et al. (2000) Hypoglycaemia, liver necrosis and perinatal death in mice lacking all isoforms of phosphoinositide 3-kinase p85 alpha. Nat Genet 26: 379–382.
- 4. Lindmo K, Stenmark H (2006) Regulation of membrane traffic by phosphoinositide 3-kinases. J Cell Sci 119: 605–614.
- 5. Christoforidis S, Miaczynska M, Ashman K, Wilm M, Zhao L, et al. (1999) Phosphatidylinositol-3-OH kinases are Rab5 effectors. Nat Cell Biol 1: 249–252.
- 6. Liang C, Lee JS, Inn KS, Gack MU, Li Q, et al. (2008) Beclin1-binding UVRAG targets the class C Vps complex to coordinate autophagosome maturation and endocytic trafficking. Nat Cell Biol 10: 776–787.
- 7. Murray JT, Panaretou C, Stenmark H, Miaczynska M, Backer JM (2002) Role of Rab5 in the recruitment of hVps34/p150 to the early endosome. Traffic 3: 416–427.
- 8. Nielsen E, Severin F, Backer JM, Hyman AA, Zerial M (1999) Rab5 regulates motility of early endosomes on microtubules. Nat Cell Biol 1: 376–382.
- 9. Hoepfner S, Severin F, Cabezas A, Habermann B, Runge A, et al. (2005) Modulation of receptor recycling and degradation by the endosomal kinesin KIF16B. Cell 121: 437–450.
- 10. Fratti RA, Backer JM, Gruenberg J, Corvera S, Deretic V (2001) Role of phosphatidylinositol 3-kinase and Rab5 effectors in phagosomal biogenesis and mycobacterial phagosome maturation arrest. J Cell Biol 154: 631–644.
- 11. Vieira OV, Botelho RJ, Rameh L, Brachmann SM, Matsuo T, et al. (2001) Distinct roles of class I and class III phosphatidylinositol 3-kinases in phagosome formation and maturation. J Cell Biol 155: 19–25.
- 12. Stein MP, Feng Y, Cooper KL, Welford AM, Wandinger-Ness A (2003) Human VPS34 and p150 are Rab7 interacting partners. Traffic 4: 754–771.
- 13. Zoncu R, Perera RM, Balkin DM, Pirruccello M, Toomre D, et al. (2009) A phosphoinositide switch controls the maturation and signaling properties of APPL endosomes. Cell 136: 1110–1121.
- 14. Futter CE, Collinson LM, Backer JM, Hopkins CR (2001) Human VPS34 is required for internal vesicle formation within multivesicular endosomes. J Cell Biol 155: 1251–1264.
- 15. Johnson EE, Overmeyer JH, Gunning WT, Maltese WA (2006) Gene silencing reveals a specific function of hVps34 phosphatidylinositol 3-kinase in late versus early endosomes. J Cell Sci 119: 1219–1232.
- 16. Burda P, Padilla SM, Sarkar S, Emr SD (2002) Retromer function in endosome-to-Golgi retrograde transport is regulated by the yeast Vps34 PtdIns 3-kinase. J Cell Sci 115: 3889–3900.
- 17. Skanland SS, Walchli S, Utskarpen A, Wandinger-Ness A, Sandvig K (2007) Phosphoinositide-regulated retrograde transport of ricin: crosstalk between hVps34 and sorting nexins. Traffic 8: 297–309.
- 18. Tassa A, Roux MP, Attaix D, Bechet DM (2003) Class III phosphoinositide 3-kinase–Beclin1 complex mediates the amino acid-dependent regulation of autophagy in C2C12 myotubes. Biochem J 376: 577–586.
- 19. Petiot A, Ogier-Denis E, Blommaart EF, Meijer AJ, Codogno P (2000) Distinct classes of phosphatidylinositol 3′-kinases are involved in signaling pathways that control macroautophagy in HT-29 cells. J Biol Chem 275: 992–998.
- 20. Kihara A, Noda T, Ishihara N, Ohsumi Y (2001) Two distinct Vps34 phosphatidylinositol 3-kinase complexes function in autophagy and carboxypeptidase Y sorting in Saccharomyces cerevisiae. J Cell Biol 152: 519–530.
- 21. Itakura E, Kishi C, Inoue K, Mizushima N (2008) Beclin 1 forms two distinct phosphatidylinositol 3-kinase complexes with mammalian Atg14 and UVRAG. Mol Biol Cell 19: 5360–5372.
- 22. Obara K, Sekito T, Niimi K, Ohsumi Y (2008) The Atg18-Atg2 complex is recruited to autophagic membranes via phosphatidylinositol 3-phosphate and exerts an essential function. J Biol Chem 283: 23972–23980.
- 23. Gulati P, Gaspers LD, Dann SG, Joaquin M, Nobukuni T, et al. (2008) Amino acids activate mTOR complex 1 via Ca2+/CaM signaling to hVps34. Cell Metab 7: 456–465.
- 24. Nobukuni T, Joaquin M, Roccio M, Dann SG, Kim SY, et al. (2005) Amino acids mediate mTOR/raptor signaling through activation of class 3 phosphatidylinositol 3OH-kinase. Proc Natl Acad Sci U S A 102: 14238–14243.
- 25. Nobukuni T, Kozma SC, Thomas G (2007) hvps34, an ancient player, enters a growing game: mTOR Complex1/S6K1 signaling. Curr Opin Cell Biol 19: 135–141.
- 26. Byfield MP, Murray JT, Backer JM (2005) hVps34 is a nutrient-regulated lipid kinase required for activation of p70 S6 kinase. J Biol Chem 280: 33076–33082.
- 27. Schu PV, Takegawa K, Fry MJ, Stack JH, Waterfield MD, et al. (1993) Phosphatidylinositol 3-kinase encoded by yeast VPS34 gene essential for protein sorting. Science 260: 88–91.
- 28. Herman PK, Emr SD (1990) Characterization of VPS34, a gene required for vacuolar protein sorting and vacuole segregation in Saccharomyces cerevisiae. Mol Cell Biol 10: 6742–6754.
- 29. Roggo L, Bernard V, Kovacs AL, Rose AM, Savoy F, et al. (2002) Membrane transport in Caenorhabditis elegans: an essential role for VPS34 at the nuclear membrane. EMBO J 21: 1673–1683.
- 30. Juhasz G, Hill JH, Yan Y, Sass M, Baehrecke EH, et al. (2008) The class III PI(3)K Vps34 promotes autophagy and endocytosis but not TOR signaling in Drosophila. J Cell Biol 181: 655–666.
- 31. Zhou X, Wang L, Hasegawa H, Amin P, Han BX, et al. (2010) Deletion of PIK3C3/Vps34 in sensory neurons causes rapid neurodegeneration by disrupting the endosomal but not the autophagic pathway. Proc Natl Acad Sci U S A 107: 9424–9429.
- 32. Zhou X, Wang F (2010) Effects of neuronal PIK3C3/Vps34 deletion on autophagy and beyond. Autophagy 6: 798–799.
- 33. Volinia S, Dhand R, Vanhaesebroeck B, MacDougall LK, Stein R, et al. (1995) A human phosphatidylinositol 3-kinase complex related to the yeast Vps34p-Vps15p protein sorting system. EMBO J 14: 3339–3348.
- 34. Tallquist MD, Soriano P (2000) Epiblast-restricted Cre expression in MORE mice: a tool to distinguish embryonic vs. extra-embryonic gene function. Genesis 26: 113–115.
- 35. Duncan SA, Manova K, Chen WS, Hoodless P, Weinstein DC, et al. (1994) Expression of transcription factor HNF-4 in the extraembryonic endoderm, gut, and nephrogenic tissue of the developing mouse embryo: HNF-4 is a marker for primary endoderm in the implanting blastocyst. Proc Natl Acad Sci U S A 91: 7598–7602.
- 36. Taraviras S, Monaghan AP, Schutz G, Kelsey G (1994) Characterization of the mouse HNF-4 gene and its expression during mouse embryogenesis. Mech Dev 48: 67–79.
- 37. Arceci RJ, King AA, Simon MC, Orkin SH, Wilson DB (1993) Mouse GATA-4: a retinoic acid-inducible GATA-binding transcription factor expressed in endodermally derived tissues and heart. Mol Cell Biol 13: 2235–2246.
- 38. Heikinheimo M, Scandrett JM, Wilson DB (1994) Localization of transcription factor GATA-4 to regions of the mouse embryo involved in cardiac development. Dev Biol 164: 361–373.
- 39. Hakem R, de la Pompa JL, Sirard C, Mo R, Woo M, et al. (1996) The tumor suppressor gene Brca1 is required for embryonic cellular proliferation in the mouse. Cell 85: 1009–1023.
- 40. Bielinska M, Narita N, Wilson DB (1999) Distinct roles for visceral endoderm during embryonic mouse development. Int J Dev Biol 43: 183–205.
- 41. Cross JC, Werb Z, Fisher SJ (1994) Implantation and the placenta: key pieces of the development puzzle. Science 266: 1508–1518.
- 42. Snow MHL (1977) Gastrulation in the mouse: Growth and regionalization of the epiblast. J Embryol Exp Morphol 42: 293–303.
- 43. Gangloff YG, Mueller M, Dann SG, Svoboda P, Sticker M, et al. (2004) Disruption of the mouse mTOR gene leads to early postimplantation lethality and prohibits embryonic stem cell development. Mol Cell Biol 24: 9508–9516.
- 44. Murakami M, Ichisaka T, Maeda M, Oshiro N, Hara K, et al. (2004) mTOR is essential for growth and proliferation in early mouse embryos and embryonic stem cells. Mol Cell Biol 24: 6710–6718.
- 45. Guertin DA, Stevens DM, Thoreen CC, Burds AA, Kalaany NY, et al. (2006) Ablation in mice of the mTORC components raptor, rictor, or mLST8 reveals that mTORC2 is required for signaling to Akt-FOXO and PKCalpha, but not S6K1. Dev Cell 11: 859–871.
- 46. Martin PM, Sutherland AE (2001) Exogenous amino acids regulate trophectoderm differentiation in the mouse blastocyst through an mTOR-dependent pathway. Dev Biol 240: 182–193.
- 47. Gwatkin RB, Meckley PE (1966) Chromosomes of the mouse blastocyst following its attachment and outgrowth in vitro. Ann Med Exp Biol Fenn 44: 125–127.
- 48. Naeslund G (1979) The effect of glucose-, arginine- and leucine-deprivation on mouse blastocyst outgrowth in vitro. Ups J Med Sci 84: 9–20.
- 49. Power MA, Tam PP (1993) Onset of gastrulation, morphogenesis and somitogenesis in mouse embryos displaying compensatory growth. Anat Embryol (Berl) 187: 493–504.
- 50. Sirard C, de la Pompa JL, Elia A, Itie A, Mirtsos C, et al. (1998) The tumor suppressor gene Smad4/Dpc4 is required for gastrulation and later for anterior development of the mouse embryo. Genes Dev 12: 107–119.
- 51. Yang X, Li C, Xu X, Deng C (1998) The tumor suppressor SMAD4/DPC4 is essential for epiblast proliferation and mesoderm induction in mice. Proc Natl Acad Sci U S A 95: 3667–3672.
- 52. Winnier G, Blessing M, Labosky PA, Hogan BL (1995) Bone morphogenetic protein-4 is required for mesoderm formation and patterning in the mouse. Genes Dev 9: 2105–2116.
- 53. Mishina Y, Suzuki A, Ueno N, Behringer RR (1995) Bmpr encodes a type I bone morphogenetic protein receptor that is essential for gastrulation during mouse embryogenesis. Genes Dev 9: 3027–3037.
- 54. Ruland J, Sirard C, Elia A, MacPherson D, Wakeham A, et al. (2001) p53 accumulation, defective cell proliferation, and early embryonic lethality in mice lacking tsg101. Proc Natl Acad Sci U S A 98: 1859–1864.
- 55. Komatsu M, Waguri S, Ueno T, Iwata J, Murata S, et al. (2005) Impairment of starvation-induced and constitutive autophagy in Atg7-deficient mice. J Cell Biol 169: 425–434.
- 56. Kuma A, Hatano M, Matsui M, Yamamoto A, Nakaya H, et al. (2004) The role of autophagy during the early neonatal starvation period. Nature 432: 1032–1036.
- 57. Coucouvanis E, Martin GR (1995) Signals for death and survival: a two-step mechanism for cavitation in the vertebrate embryo. Cell 83: 279–287.
- 58. Kuo CT, Morrisey EE, Anandappa R, Sigrist K, Lu MM, et al. (1997) GATA4 transcription factor is required for ventral morphogenesis and heart tube formation. Genes Dev 11: 1048–1060.
- 59. Molkentin JD, Lin Q, Duncan SA, Olson EN (1997) Requirement of the transcription factor GATA4 for heart tube formation and ventral morphogenesis. Genes Dev 11: 1061–1072.
- 60. Morrisey EE, Tang Z, Sigrist K, Lu MM, Jiang F, et al. (1998) GATA6 regulates HNF4 and is required for differentiation of visceral endoderm in the mouse embryo. Genes Dev 12: 3579–3590.
- 61. Chen WS, Manova K, Weinstein DC, Duncan SA, Plump AS, et al. (1994) Disruption of the HNF-4 gene, expressed in visceral endoderm, leads to cell death in embryonic ectoderm and impaired gastrulation of mouse embryos. Genes Dev 8: 2466–2477.
- 62. Morris SM, Tallquist MD, Rock CO, Cooper JA (2002) Dual roles for the Dab2 adaptor protein in embryonic development and kidney transport. EMBO J 21: 1555–1564.
- 63. Yang DH, Smith ER, Roland IH, Sheng Z, He J, et al. (2002) Disabled-2 is essential for endodermal cell positioning and structure formation during mouse embryogenesis. Dev Biol 251: 27–44.
- 64. Maurer ME, Cooper JA (2005) Endocytosis of megalin by visceral endoderm cells requires the Dab2 adaptor protein. J Cell Sci 118: 5345–5355.
- 65. Guertin DA, Sabatini DM (2007) Defining the role of mTOR in cancer. Cancer Cell 12: 9–22.
- 66. Zhou X, Babu JR, da Silva S, Shu Q, Graef IA, et al. (2007) Unc-51-like kinase 1/2-mediated endocytic processes regulate filopodia extension and branching of sensory axons. Proc Natl Acad Sci U S A 104: 5842–5847.