Developmental Biology Journal
Volume 2013 (2013), Article ID 131529, 8 pages
Targeted Disruption of Calcium/NFAT Signaling Reveals a Left-Right Determination Disorder in the Pharyngeal Arch Artery
Laboratory for Occupational Safety and Health, National Cerebral and Cardiovascular Center Research Institute, 5-7-1 Fujishirodai, Suita 565-8565, Japan
Received 7 December 2012; Accepted 18 February 2013
Academic Editor: Tetsuya Kojima
Copyright © 2013 Yukihisa Miyachi. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
An immunosuppressant was injected into pregnant mice in order to investigate whether the immune response is involved in differentiation during embryonic development. Injection of 3 mg/kg of FK506, an inhibitor of calcineurin, early in the organogenesis period increased the penetrance of right aortic arch formation by 32% compared with saline injection. Immunosuppressants such as FTY720 and rapamycin did not affect left/right (L/R) determination. FK506 is known to work by restricting NFAT (nuclear factor activated T-cell) dephosphorylation. An L/R determination disorder in cardiac outflows appeared when an NFATc4 siRNA was directly injected into the amniotic fluid. As for the mechanism, Pitx2, which is normally expressed on the left-hand side, was found to be expressed also on the right-hand side. Furthermore, it turned out that administration of FK506 also prevented the dephosphorylation of NSFL1 cofactor p47. When an siRNA targeting p47 was introduced into the amniotic fluid of FK506-treated fetuses, both of the dorsal arteries—which should normally become one—remained. These findings indicate that the mother's immune system contributes not only to self defense, but also to remodeling processes in fetal morphogenesis.
Recently there have been reports that the immune response controls vertebrate morphogenesis. Mukaigasa et al.  indicated a role for the immune response in metamorphosis, based on the finding that syngeneic grafts of tadpole tail skin into adult Xenopus animals are rejected by T cells. I reported that lens regeneration in newt eyes was induced by antigen-presenting cells that had engulfed the remains of the destroyed lens . Amphibians are the most commonly used models in this field, and there is little experimental data for the role of the immune response in morphogenesis of mammals.
The morphogenetic processes underlying pharyngeal arch artery (PAA) remodeling from the symmetrical configuration toward the unilateral left-sided aortic arch have not been fully unraveled . The early embryonic mammalian system consists of five paired arch arteries, numbered I to VI from cranial to caudal. The fifth artery is considered to be rudimentary or absent. At day 11.5 of pregnancy, the PAA system consists of a left and right third (III), fourth (IV), and sixth (VI) arch artery, connecting two continuous dorsal aortas with the ventrally located aortic sac. Around day 12 of pregnancy, the arterial system develops toward the mature left-sided configuration, due to regression of the right-sided sixth arch artery, the right dorsal aorta (α-segment), and both the left and right carotid ducts. It is known that a congenital disorder of the cardiac outflow tract results from abnormal PAA remodeling. I speculated that the immune response in mothers might act in the remodeling process of fetuses, as shown for amphibian development. Therefore, to evaluate the possible causes of abnormalities in the cardiac outflow tract, fetuses taken from mothers injected with immunosuppressants were examined.
Calcium/NFAT (nuclear factor activated T-cell) signaling regulates a range of cellular processes and plays essential roles during embryonic development of the heart, skull, and brain. A rise in Ca2+ levels activates calcineurin, which dephosphorylates NFAT transcription factors, facilitating their translocation to the nucleus and subsequent transcriptional activation of target genes . Five mammalian NFAT transcription factors have been identified. In the present study, FK506, an inhibitor of calcineurin/NFAT signaling, was used to examine the relationship between the immune response and the developing vascular system.
2.1. Mice and Histochemistry
C57BL/6 were reared in polycarbonate cages in an environmentally controlled room (water temperature: °C), with a standard 12-hour light/dark cycle. Injection of mother mice with the immunosuppressants, FK506, FTY760, and rapamycin, was performed three times: on days 6.5, 7.5, and 8.5 of pregnancy. Experiments in which the drugs were introduced into the amniotic fluid were also performed. Laparotomy was performed on days 6.5 or 8.5 of pregnancy, and FK506 or saline was injected directly into the amniotic fluid using a microsyringe of 10 μL volume. After the operation, the mice were returned to their original cages and observed. To evaluate abnormalities in cardiovascular development, fetuses were removed from the uterus on days 13.5 or 18.5 of pregnancy and examined histologically. The mating of mice was performed at midnight, and pregnancy day 0.5 was the morning when a vaginal plug was detected.
In order to investigate the participation of NFAT in aortic arch formation, siRNAs targeting NFATc1 (Santa Cruz Biotechnology, sc-36054) or NFATc4 (Santa Cruz Biotechnology, sc-38116) were administrated into the amniotic fluid on day 6.5 or 8.5 of pregnancy.
Embryos were fixed for 24 hours in a 4% paraformaldehyde solution buffered with 0.15 M sodium phosphate at a pH of 7.3. They were then washed in several changes of the same buffer and embedded in paraffin. Serial sections of 2 μm were prepared and stained with Mayer’s hematoxylin and eosin.
The protocol for immunohistochemistry used to detect CD31 was similar to that described by Cursiefen et al. . Briefly, the whole embryos were frozen on dry ice in Tissue-Tek and sectioned into 8 μm thick slices. The sections were collected onto microscope slides, dried at room temperature, fixed in acetone, rinsed in PBS, blocked in 2% BSA, and stained with Alexa Fluor 488-conjugated CD31 antibody overnight. All staining procedures were performed at room temperature. Staining with secondary antibody alone, or with an isotype control instead of with CD31 primary antibody, was negative. A similar procedure was adopted for CD34 and CD117 (c-kit) immunohistochemistry. All experiments were approved by the animal ethics committee of the National Cerebral and Cardiovascular Center.
2.2. Two-Dimensional Electrophoresis and Western Blotting
Whole embryos were first washed in cold saline and then homogenized in the presence of 5 M urea, 2 M thiourea, 2% CHAPS, 2% SB3-10, and 1% DTT. Supernatants were collected after centrifugation at 20,000 g for 30 min. The total protein concentrations of the samples were determined using a protein assay kit (Pierce). First-dimensional separation of the proteins was performed on an IPGphor IEF system using immobiline DryStrips pH 4–7 (GE Healthcare Bio-sciences) or Pharmalyte broad range, pH 3-10 (GE Healthcare Life Sciences). The extracts were loaded onto rehydrated immobiline strips and electrophoresed with internal protein markers (Promega). Running conditions were 3,500 volts maxium for 8 hours. Vertical SDS-PAGE was used for the second dimension, using 9~18% acrylamide gradient gels.
After 2DE, gels were dyed using a fluorescence staining reagent for the detection of phosphorylated proteins (Pro-Q Diamond phosphoprotein gel stain, Molecular Probes) or all proteins (SYPRO Ruby protein gel stain). Gel images were obtained using a fluorescence scanner, and images were evaluated using ImageMaster Platinum (GE). The signal intensity of all spots was computed using this software. Signal intensity was shown with the value (%volume value) which was divided by the total of the signal intensity of all spots on gel.
The phosphorylation index (i.e., the number of phosphate groups per molecule of protein) was calculated from the two %volume values as follows: phosphorylation index = (D/S ratio) = (%Vol. value of the Pro-Q Diamond dye spot)/(%Vol. value of the SYPRO Ruby dye spot). Spots satisfying the following two conditions were listed as protein identification candidates. (1) The sum of the % values from two 2DE gels dyed with SYPRO Ruby was 0.1 or more. (2) The relative change in phosphorylation index for a spot in the FK506-injected groups was 1.5 or more relative to the saline-injected groups.
The same samples used for 2DE were used for western blotting. First, equal quantities of each sample were mixed with SDS sample buffer (125 nM Tris-HCl, 4% SDS, 10% sucrose, 2% DTT) and heated for 5 minutes at 95°C. Each sample was then run on 4% SDS-PAGE gels using standard procedures. Subsequently, the proteins were transferred onto a PVDF membrane (GE Healthcare Bio-Sciences) using a blotting unit (GE Healthcare Bio-Sciences) with blotting buffer (25 mM Tris-HCl, 200 mM glycine, 10% methanol, 0.02% SDS). Blots were incubated with primary antibodies against Lefty2 (PTG 13991-1-AP) and Pitx2 (NOV NBP1-70363) for 16 h at 4°C and with the corresponding secondary antibody (GE NA934, anti-rabbit IgG, HRP-linked whole Ab from donkey) for 1 h at RT. Finally, the PVDF film was used to expose the X-ray film.
2.3. Mass Spectrometry
First, isolated gel pieces representing spots were decolorized, and then the peptide was extracted using 50% acetonitrile and 1% TFA. The peptide extraction liquid was condensed with a vacuum dryer, loaded into a ZipTip C18 (Millipore) column, and extracted with 50% acetonitrile again. These extracts were used for mass spectrometry (Bruker Daltonics).
3.1. Restriction of Calcineurin/NFATc4 Signaling by FK506
My analysis demonstrated a change in aortic arch formation; results are summarized in Table 1. In saline-injected fetuses, the cardiac outflow tract (aorta) arose from the left ventricle, ascended for a short distance, and then curved to the left and descended through the left side of the chest (Figures 1(a) and 1(c)). Injection of 3.0 mg/kg of FK506 into the mother mouse on days 6.5, 7.5, and 8.5 of pregnancy induced an L/R determination disorder, in which the cardiac outflow tract ascended toward the right side, formed an arch, and then descended through the right side of the chest (Figures 1(b) and 1(d)). Injection of 3.0 mg/kg of FK506 increased the penetrance of the right aortic arch by 32% (ten of 31) relative to saline injection. The ductus arteriosus also ran toward the right side of the chest and connected with the right aortic arch after the right subclavian artery branch. When the dose of FK506 was increased to 6.0 mg/kg, vascular abnormalities could not be evaluated because of abortion of the fetuses before 10.5 days of pregnancy. The L/R determination disorder was observed in fetuses given a dose of 1.5 mg/kg, when FK506 was injected directly into the amniotic fluid at day 8.5 of pregnancy (Table 2). The same effects could be observed after injections at 7.5 days. However, the right aortic arch was not seen in fetuses after injections into the amniotic fluid at 10.5 days. FK506 blocks the dephosphorylation reaction of calcineurin signaling. Therefore, additional experiments were performed. A phosphate buffer (pH 7.4, TAKARA Bio T-900) was introduced into the amniotic fluid at day 8.5 of pregnancy for the purpose of raising the concentration of intracellular phosphoric acid. Also after administration of a phosphate buffer into amniotic fluid, right aortic arches appeared clearly (Table 3) although the effect was not as strong as that with FK506. These results indicated that there is a critical time during remodeling of the aortic arch between 7.5 and 8.5 days of pregnancy and that remodeling of PAA involves a phosphorylation reaction.
Interruption of the aortic arch, ventricular septal defects, and persistent truncus arteriosus were not induced by FK506 injection. Interestingly, other immunosuppressants, such as FTY720 and rapamycin, did not induce an L/R determination disorder (Table 1).
Calcineurin causes the rapid dephosphorylation and nuclear import of the products of the NFATc genes. Therefore, I next looked for abnormalities in fetuses given an siRNA targeting NFATc4 (nuclear factor of activated T cells, calcineurin-dependent 4) in the amniotic fluid at day 8.5 of pregnancy. In these fetuses, there was a significant increase in the right aortic arch being accompanied by right ductus arteriosus when compared with saline-injected fetuses (Table 3). However, the NFATc1 siRNA caused embryonic lethality. These findings indicate that the reversed orientation of the cardiac outflow tract might be related to the expression of cytokine genes following the action of NFATc4.
It is known that haematopoietic stem cells (HSCs), which are responsible for blood production, emerge in the dorsal aorta at day 10.5 of pregnancy . Therefore I investigated whether the emergence of HSCs moves to the right side when the cardiac outflow tracts of the fetuses injected with FK506 move from the left to the right using an immunohistochemical analysis of CD34+ and CD117+ (c-kit). In the saline-injected group, CD34+ and CD117+ (c-kit) cells were found to be attached to the endothelium in the left side of the dorsal artery, where HSCs might localize (Figure 2). However, when FK506 was given directly into the amniotic fluid, CD34+ and CD117+ cells existed clearly in the right side of the dorsal artery and could remain there during development. These findings suggest that not only is the L/R direction of the blood vessel reversed, but so is the L/R localization of specific functions.
3.2. Mechanism of the L/R Determination Disorder
The mechanisms underlying L/R determination have fascinated biologists for decades. Pitx2 is a homeobox gene that has been shown to play a central role in the late aspects of L/R asymmetric morphogenesis . Since expression of Pitx2 takes place before the aortic arch is formed, all embryos treated with FK506 were investigated. After that, the difference in Pitx2 expression between FK506- and saline-treated embryos was evaluated. As shown in Figure 3, the expression of Pitx2 in the FK506-treated group shifted to the right-hand sides of embryos, crossing the median line, whereas Pitx2 expression in saline-treated embryos was restricted to the left side at the 8-somite stage. Importantly, FK506 induced ectopic expression on the right side. Western blotting revealed increased expression of Pitx2 by a factor of approximately 1.5 compared with saline-injected fetuses. In contrast, the expression of Lefty 2 (left-right determination factor 2) decreased slightly relative to the levels in saline-injected fetuses. These findings demonstrated that the expression of Pitx2 might be regulated by calcineurin signaling and that the right aortic arch may be induced by the ectopic expression of Pitx2.
3.3. Phosphorylation Analysis by Two-Dimensional Electrophoresis
To investigate how many intracellular dephosphorylation events were prevented by injection of FK506, two-dimensional electrophoresis (2DE) analysis was performed. Using a staining solution for phosphorylated proteins, spots were selected from the gels obtained after FK506 injection based on the strength of their signals. In Figure 4, spots are arranged according to their D/S ratio and mass spectrometry (MS) was performed on the six spots with the highest D/S ratio. MS of fetuses from mothers given FK506 early in the organogenesis period identified hyperphosphorylation of the NSFL1 cofactor p47 (p97 cofactor p47) protein. Hyperphosphorylation was also seen at a spot of poly(C) binding protein 2. Therefore I investigated whether NSFL1 cofactor p47 is related to L/R determination. FK506-treated fetuses were subjected to siRNA against p47 in the amniotic fluid. Figure 5 shows that not only the right dorsal artery but also the left dorsal artery remained: in other words, siRNA against P47 inhibited the disappearance of the left dorsal artery in FK506-treated fetuses.
4. Discussion and Conclusion
This study has clearly revealed that Pitx2, which is normally expressed at the left-hand side of embryos, is also expressed at the right-hand side and promotes the formation of a right aortic arch when calcineurin is inhibited using FK506. Furthermore, it was observed that administration of FK506 prevented dephosphorylation of NSFL1 cofactor p47.
This study also found that an siRNA targeting NFATc4 exhibits the same effects as FK506, inducing an L/R determination disorder in aortic arch remodeling. NFATc4 plays a role in the inducible expression of cytokine genes in T cells, including the induction of IL-2 and IL-4. The p38 MAP kinase phosphorylates multiple residues in the NFAT homology domain of NFATc4. The answer to the question that was the purpose of this research—whether the immune system is involved in the morphogenesis of an animal—was considered to be likely yes in the case of aortic remodeling. My result showed that the dephosphorylation reaction that is required for T-cell activation is important for embryonic development and that it is not an immune regulator, such as a cytokine, that was thought to be directly involved in early development. The data in Table 3, in which the injection of a phosphate salt into amniotic fluid also easily induced the L/R determination disorder, has supported this result.
When a cell enters mitosis, p47 localized to the nucleus moves to the cytoplasm after nuclear envelope breakdown and forms a complex with p97. However, it has been suggested that if p47 cannot be phosphorylated by cdc2 in cytoplasm, it cannot form a complex with p97. As a result, Golgi bodies are destroyed and changed to small-granule vesicles . In the present study, when p47 siRNA was introduced into the amniotic fluid of FK506-treated fetuses, both dorsal arteries remained. There is a high probability that p47 is involved in the cell death in the dorsal artery, where cells normally disappear during embryonic development.
It has been proposed that the process of LR determination commonly involves a cilia-driven leftward flow in the mammalian node and its equivalents, such as the Kupffer vesicle in zebrafish and the gastrocoel roof plate in Xenopus . Asymmetric Ca2+ signaling has been detected at the left margin of the node . The asymmetric elevation of Ca2+ and its lateral propagation have also been reported . Moreover, it was reported that Ca2+ flux regulates Kupffer’s vesicle development and is required for LR determination. Microinjection of an IP3 receptor function-blocking antibody that can inhibit IP3 calcium channel activity randomized the LR axis in terms of left-sided Pitx2 expression and organ laterality . There are also some reports that L/R asymmetry depends on early differential ion flux created by H+/K+ ATPase transporter activity . An H+/K+ ATPase blocker inhibited the expression of Nodal and Pitx-2, which are normally expressed in the left lateral mesoderm, and induced these genes on the right side. The result was heterotaxia of all organs. However, in this present study, after FK506 treatment, only cardiac outflows showed reversed left-right positioning: reversal of internal organs did not occur. Moreover, after FK506 treatment, hematogenous functions also appeared among the blood vessels that ran on the right-hand side. The phenomenon of how the hematopoietic stem cell, which moves from yolk sac, discerns the blood vessel that remains is interesting.
FTY720 is an immunosuppressant drug, approved for treating multiple sclerosis. It is a sphingosine-1-phosphate receptor modulator, which sequesters lymphocytes in lymph nodes, preventing them from contributing to an autoimmune reaction. Rapamycin is not a calcineurin inhibitor, but the action of rapamycin is to bind the cytosolic protein FKBP12 in a manner similar to that of FK506. Unlike the FK506-FKBP12 complex, which inhibits calcineurin, though, the rapamycin-FKBP12 complex inhibits the mammalian target of rapamycin (mTOR) pathway by directly binding the mTOR complex 1 (mTORC1) . In the present study, immunosuppressants such as FTY720 and rapamycin did not induce an L/R determination disorder. My results suggest that only NFATc signaling is important for L/R axis determination during embryonic development. Of additional importance was the finding that although the fetuses given an NFATc siRNA exhibited an L/R determination disorder, the infusion did not induce an abnormality in myocardial development, including any apparent defects in cardiac morphology.
The important issue that must be considered in the future is whether the immune system of the fetus is involved in the determination of the L/R axis. The thymus is generated from the 3rd pharyngeal pouch, and it is thought that T-lymphocyte progenitors move into the thymus around day 11.5 of pregnancy. In the present study, it was hypothesized that the determination of the L/R axis had a high possibility of having happened by day 8.5 of pregnancy (Table 2). It seemed that the appearance of the right aortic arch would be a phenomenon that occurred in collaboration with the immune system of the mother, including that associated with the placenta.
Conflict of Interests
The author declares that there is no conflict of interests.
The author thanks Yoko Kitai and Haruna Hirose for their technical assistance.
- K. Mukaigasa, A. Hanasaki, M. Maéno et al., “The keratin-related Ouroboros proteins function as immune antigens mediating tail regression in Xenopus metamorphosis,” Proceedings of the National Academy of Sciences of the United States of America, vol. 106, no. 43, pp. 18309–18314, 2009.
- T. Kanao and Y. Miyachi, “Lymphangiogenesis promotes lens destruction and subsequent lens regeneration in the newt eyeball, and both processes can be accelerated by transplantation of dendritic cells,” Developmental Biology, vol. 290, no. 1, pp. 118–124, 2006.
- T. Hiruma and Y. Nakajima, “Development of pharyngeal arch arteries in early mouse embryo,” Journal of Anatomy, vol. 201, no. 1, pp. 15–29, 2002.
- G. R. Crabtree, “Generic signals and specific outcomes: signaling through Ca2+, calcineurin, and NF-AT,” Cell, vol. 96, no. 5, pp. 611–614, 1999.
- C. Cursiefen, L. Chen, L. P. Borges et al., “VEGF-A stimulates lymphangiogenesis and hemangiogenesis in inflammatory neovascularization via macrophage recruitment,” Journal of Clinical Investigation, vol. 113, no. 7, pp. 1040–1050, 2004.
- J. C. Boisset, W. Van Cappellen, C. Andrieu-Soler, N. Galjart, E. Dzierzak, and C. Robin, “In vivo imaging of haematopoietic cells emerging from the mouse aortic endothelium,” Nature, vol. 464, no. 7285, pp. 116–120, 2010.
- J. Capdevila, K. J. Vogan, C. J. Tabin, and J. C. Izpisúa Belmonte, “Mechanisms of left-right determination in vertebrates,” Cell, vol. 101, no. 1, pp. 9–21, 2000.
- X. Yuan, P. Simpson, C. McKeown et al., “Structure, dynamics and interactions of p47, a major adaptor of the AAA ATPase, p97,” The EMBO Journal, vol. 23, no. 7, pp. 1463–1473, 2004.
- H. Shiratori and H. Hamada, “The left-right axis in the mouse: from origin to morphology,” Development, vol. 133, no. 11, pp. 2095–2104, 2006.
- J. McGrath, S. Somlo, S. Makova, X. Tian, and M. Brueckner, “Two populations of node monocilia initiate left-right asymmetry in the mouse,” Cell, vol. 114, no. 1, pp. 61–73, 2003.
- Y. Tanaka, Y. Okada, and N. Hirokawa, “FGF-induced vesicular release of Sonic hedgehog and retinoic acid in leftward nodal flow is critical for left-right determination,” Nature, vol. 435, no. 7039, pp. 172–177, 2005.
- M. Hatayama, K. Mikoshiba, and J. Aruga, “IP3 signaling is required for cilia formation and left-right body axis determination in Xenopus embryos,” Biochemical and Biophysical Research Communications, vol. 410, no. 3, pp. 520–524, 2011.
- M. Levin, T. Thorlin, K. R. Robinson, T. Nogi, and M. Mercola, “Asymmetries in H+/K+-ATPase and cell membrane potentials comprise a very early step in left-right patterning,” Cell, vol. 111, no. 1, pp. 77–89, 2002.
- S. B. Helliwell, P. Wagner, J. Kunz, M. Deuter-Reinhard, R. Henriquez, and M. N. Hall, “TOR1 and TOR2 are structurally and functionally similar but not identical phosphatidylinositol kinase homologues in yeast,” Molecular Biology of the Cell, vol. 5, no. 1, pp. 105–118, 1994.