Abstract
Aberrant zinc (Zn) homeostasis is associated with abnormal control of mammalian growth, although the molecular mechanisms of Zn's roles in regulating systemic growth remain to be clarified. Here we report that the cell membrane-localized Zn transporter SLC39A14 controls G-protein coupled receptor (GPCR)-mediated signaling. Mice lacking Slc39a14 (Slc39a14-KO mice) exhibit growth retardation and impaired gluconeogenesis, which are attributable to disrupted GPCR signaling in the growth plate, pituitary gland, and liver. The decreased signaling is a consequence of the reduced basal level of cyclic adenosine monophosphate (cAMP) caused by increased phosphodiesterase (PDE) activity in Slc39a14-KO cells. We conclude that SLC39A14 facilitates GPCR-mediated cAMP-CREB signaling by suppressing the basal PDE activity, and that this is one mechanism for Zn's involvement in systemic growth processes. Our data highlight SLC39A14 as an important novel player in GPCR-mediated signaling. In addition, the Slc39a14-KO mice may be useful for studying the GPCR-associated regulation of mammalian systemic growth.
Introduction
Zn is an essential trace element that is involved in diverse cellular events by affecting the structural and catalytic functions of enzymes and transcription factors [1], [2]. Zn homeostasis is tightly controlled by two types of Zn transporters, SLC39/ZIP importers and SLC30/ZnT exporters [3], [4], and by metallothioneins (MTs) [5], all of which participate in various physiological events. For instance, SLC39A4/ZIP4 is expressed in the intestine and has a role in Zn uptake through enterocytes [6], [7]. Patients with Acrodermatitis Enteropathica (AE), who suffer from severe skin disease and frequent infections, have unusually low serum concentrations of Zn due to pathogenic loss-of-function mutations in SLC39A4 [6], [7]. Another Zn transporter, SLC39A13/ZIP13, is expressed on the Golgi and controls the intracellular Zn distribution in cells of mesenchymal origin. Slc39a13-KO mice show dwarfism and abnormal bone and cutaneous development, and a loss-of-function mutation in this gene was found in patients with a novel type of Ehlers-Danlos Syndrome (EDS), demonstrating that SLC39A13 plays a critical role in growth control and connective tissue formation in mouse and human [8]. In fact, considerable evidence indicates that Zn transporters are involved in regulating a variety of intracellular signaling pathways in animals, from flies to vertebrates [8], [9], [10], [11], [12], [13]. In addition, Zn is reported to act as a neurotransmitter [14] or rather, as an allosteric regulator for a Zn-sensing receptor [15], and as an intracellular signaling molecule [11], [16], [17].
Somatic growth, which affects body size, is regulated by endogenous and systemic factors, such as nutrients, hormones, and growth factors [18], [19]. The production of growth hormone (GH) in the pituitary gland and of insulin-like growth factor (IGF-I) in the liver are the main endocrine influences on somatic growth [20]. GH and IGF-I regulate longitudinal bone growth by controlling endochondral ossification, a defined sequence of events underlying chondrocyte differentiation in the growth plate [18],[21],[22].
Aberrant Zn homeostasis is associated with vertebrate growth retardation [1], [8], [20] and metabolic disorders [4], [23]. In particular, Zn deficiency causes dwarfism with reductions in the circulating GH and IGF-I concentrations [20], and decreased growth-plate width, which is correlated with reduced cellular Zn content [24]. Intriguingly, the growth retardation cannot be reversed by maintaining circulating levels of GH or IGF-I through exogenous administration in Zn-deficient animals [20]. These findings collectively suggest that Zn's uptake into cells and the subsequent intracellular Zn accumulation affect the hormone signaling cascade(s) required for GH production and chondrocyte differentiation. Since the endocrine system consists of a complex group of glands involved in growth and metabolism, its perturbation can broadly affect human health, and it is important to elucidate the mechanisms underlying the early stages of endocrine disorders. However, the molecules responsible for Zn homeostasis have been elusive, and how Zn affects the intracellular signaling that regulates growth-related endocrine processes has been little studied.
SLC39A14, a SLC39/ZIP family member, transports the Zn ion into cells in an in vitro culture system [25], [26], but its physiological roles are still speculative. Here, we show that SLC39A14 plays important roles in mammalian growth and energy metabolism by regulating GPCR-cAMP-CREB signaling. Our findings unexpectedly revealed the biological contribution of a Zn transporter to GPCR-mediated signaling, which may help to explain why Zn deficiency results in growth inhibition and metabolic and endocrine-related disorders.
Results
Slc39a14-KO mice show dwarfism and shortened long bones
Since Zn-deficient animals with growth retardation show reduced amounts of cellular Zn [20], it has been assumed that Zn uptake and its subsequent intracellular accumulation in pituitary cells and chondrocytes, which are respectively important for GH production [27] and bone elongation [21], might be a common, critical initial step required for growth regulation. Therefore, first, to identify SLC39 members that might contribute to the influx of Zn into pituitary cells and chondrocytes, we examined the mRNA expression levels of SLC39 Zn transporters in these cells. Among the SLC39 family members, SLC39A14 was expressed in both types of cells (Figure S1). In addition, Slc39a7 was abundant, and Slc39a1, 6, and 13 showed relatively high expression levels in both cell types. SLC39A7 and SLC39A13 are present mainly in intracellular organelles [8], [28], [29], and SLC39A1 and SLC39A6 are localized to both the plasma membrane and intracellular organelles [30], [31], [32], [33]. Slc39a1-deficient mice are reported to display no obvious phenotypes under normal growth conditions [34]. Slc39a8 and Slc39a10 were highly expressed in chondrocytes but poorly in pituitary cells. Since SLC39A14 is so far reported to be a SLC39 member that resides only on the plasma membrane [25], [26], [35], we chose to examine SLC39A14 further as a candidate regulator of systemic growth via Zn influx.
To investigate the physiological role of SLC39A14 in growth, we generated mice with a deletion in the Slc39a14 gene. We constructed a targeting vector designed to eliminate the genomic region encompassing exons 5–8, which contain the histidine-rich domain and conserved HEXPHEXGD motif that is common to SLC39 family members [36], and to delete both alternative splice variants of SLC39A14, designated SLC39A14A and SLC39A14B, encoded by exons 4a and 4b, respectively [35] ( Figure 1A ). After electroporation of this vector into embryonic stem (ES) cells, the correctly targeted ES cell clones were identified by southern blotting analysis (Data not shown). Homologous recombinant ES cell clones were used to generate Slc39a14-KO heterozygotes, which were intercrossed to yield Slc39a14-KO homozygotes. Southern blotting analysis of the genomic DNA of wild-type (WT), heterozygous (HE), and homozygous (HO) mice confirmed the deletion of Slc39a14 in the Slc39a14-KO mice ( Figure 1B ). The gene knockout was further confirmed by the lack of its mRNA ( Figure 1B ). SLC39A14 protein is posttranslationally modified [25], [26]. Western blotting analysis with anti-mouse SLC39A14 and anti-V5 antibodies demonstrated that a group of high-molecular-mass bands (compatible with glycosylated oligomers; >89 kDa) of endogenous SLC39A14 were abundant in the cell lysates of both wild-type liver and Slc39a14a-v5-overexpressing 293T cells, whereas these bands were completely absent from lysates of Slc39a14-KO liver ( Figure 1C ). These data suggested that SLC39A14 was successfully deleted in the Slc39a14-KO cells.
The Slc39a14-KO mice exhibited growth retardation compared to control mice, and dwarfism was visible even in neonates ( Figure 2A ). The mice also exhibited torticollis (wry neck, Figure 2B , upper) and slightly radiolucent bones ( Figure 2B , lower). Bone histomorphometric analysis showed that these moderate osteoporotic phenotypes were associated with decreased bone volume and trabecular number, and increased trabecular separation ( Figure 2C ). The length of the long bones in the Slc39a14-KO mice was also significantly reduced ( Figure 2D ), indicating that SLC39A14 may play critical roles in skeletal formation.
Abnormal chondrocyte differentiation in the growth plate of Slc39a14-KO mice
To investigate the role of SLC39A14 in bone, we first examined the expression profile of Slc39a14 mRNA by in situ hybridization analysis. We found relatively high Slc39a14 mRNA expression in bone tissues such as the limb, spine, and thorax of the E16.5 embryo ( Figure 3A ), leading us to examine the bone morphology of the Slc39a14-KO mice.
Endochondral ossification is a process required for the proper development of long bones and vertebrate growth [37]. In this process, resting chondrocytes differentiate into proliferative chondrocytes with a columnar morphology, stop dividing, and mature into prehypertrophic and then hypertrophic chondrocytes. We first asked whether the shorter long bones of the Slc39a14-KO mice resulted from a defect in this process. In the control growth plate, Slc39a14 was expressed from the resting zone (RZ) to the prehypertrophic zone (pHZ), with relatively high abundance in the proliferative zone (PZ) and little in the hypertrophic zone (HZ) ( Figure 3B and C , top panels). The type II Collagen (Col2a1) gene is exclusively expressed in the RZ and PZ in the growth plate, and its expression level was increased in the growth plate of the Slc39a14-KO mice compared to control mice ( Figure 3B , lower panels). In addition, the expression of pHZ markers indian hedgehog (Ihh) and parathyroid hormone 1 receptor (Pth1r), were enhanced in the Slc39a14-KO growth plate ( Figure 3C , middle panels and Figure S2), and type X Collagen (Col10a1), an HZ marker, was also upregulated in the growth plate and in cultured chondrocytes from the Slc39a14-KO mice ( Figure 3C bottom panels, and Figure 3D ). In line with these observations, both the pHZ and HZ were elongated, and the RZ and PZ were narrowed, indicating that hypertrophy was accelerated in the Slc39a14-KO growth plate ( Figure 3E ).
SLC39A14 positively regulates PTH1R-cAMP-CREB signaling in chondrocytes
A number of signaling pathways regulate the steps of chondrocyte differentiation in the growth plate [18], [21]. Among them, we were particularly interested in PTH1R signaling, because it regulates chondrocyte differentiation by suppressing hypertrophy in the growth plate [37], and the morphology of the Slc39a14-KO growth plate partly phenocopies that of PTH1R-mutant or -deficient mice [38], [39]. Parathyroid hormone-related peptide (PTHrP) stimulates the phosphorylation of cAMP response element-binding protein (CREB) by the nuclear-translocated catalytic alpha subunit of protein kinase A (PKA-Cα), and the phosphorylated CREB (p-CREB) then induces the transcription of c-fos [40]. As shown in Figure 4A , the PTHrP-mediated c-fos transcription was significantly reduced in the Slc39a14-KO chondrocytes. The induction of CREB phosphorylation and the nuclear translocation of PKA-Cα in response to PTHrP treatment were also downregulated in the Slc39a14-KO cells ( Figure 4B ), although the PTH1R expression level was not diminished in these cells ( Figure 4B and Figure S2).
PTHrP stimulation leads to elevated cAMP levels through adenylyl cyclase (AC) activation, and cAMP then activates PKA by binding to its regulatory subunit [41]. In the Slc39a14-KO chondrocytes, the basal cAMP level was significantly reduced ( Figure 4C , left), and even after treatment with either PTHrP or the AC activator forskolin (FSK), the level was lower than in control chondrocytes, although the fold increase in cAMP levels after stimulation was comparable between the control and Slc39a14-KO chondrocytes ( Figure 4C , right). These findings indicated that SLC39A14 was not required for the ligand-mediated AC activation, but rather, for maintaining the basal cAMP level in chondrocytes. Since PDE is known to control the cAMP level through its enzymatic activity [42], we next asked whether PDE activity was elevated in the Slc39a14-KO chondrocytes. As shown in Figure 4D , the Slc39a14-KO chondrocytes showed enhanced PDE activity and a reduced cAMP level compared with control cells, both of which were brought to normal levels by treatment with a PDE inhibitor, 3-isobutyl-1-methylxanthine (IBMX), suggesting that SLC39A14 negatively regulates PDE activity to upregulate the PTH1R-signaling pathway.
SLC39A14 was localized to the plasma membrane ( Figure 5A ), and is thought to increase the intracellular Zn level by Zn influx [25], [26], raising the possibility that SLC39A14-mediated Zn influx plays a role in chondrocyte differentiation. To address this hypothesis, we measured the Zn level in control and Slc39a14-KO growth plates. Electron Probe X-ray Micro Analysis (EPMA) revealed that the intracellular Zn level was significantly decreased in the PZ of the Slc39a14-KO growth plate ( Figure 5B ), consistent with the idea that SLC39A14 functions to transport Zn from the outside to the inside of a cell. The forced introduction of Zn into cells using Zn plus pyrithione elevated the cAMP levels in Slc39a14-KO chondrocytes ( Figure 5C , left) with a significant reduction of the PDE activity ( Figure 5C , right) in a Zn-concentration- and time-dependent manner. Furthermore, the ectopic expression of SLC39A14 in Slc39a14-KO cells rescued the intracellular Zn ( Figure 5D , left), and cAMP levels ( Figure 5D , right).
The mRNA expression levels of other SLC39 members, which reside on the cell surface or in intracellular spaces, such as Slc39a1, 6, 7, 8, 10, and 13, were not significantly altered in the Slc39a14-KO chondrocytes (Figure S3). Taken together, these results were consistent with the idea that SLC39A14 on the plasma membrane helps to maintain the steady-state level of PTH1R-mediated signaling by importing Zn to inhibit PDE activity, and strongly suggest that SLC39A14 plays a unique role in GPCR signaling in these cells, with little backup by the upregulation of other SLC39 family members to compensate for its loss of function.
SLC39A14 positively regulates GH production via GHRHR signaling in the pituitary gland
Given that SLC39A14 negatively regulates PDE activity and that PDEs regulate several GPCR signaling pathways [42], we looked for likely GPCR pathways that might be affected by SLC39A14 expression. Since the Slc39a14-KO mice showed dwarfism, which is also seen in GH-deficient mouse models and humans [19], we investigated the role of SLC39A14 in signaling through growth hormone releasing hormone (GHRH) receptor (GHRHR), a GPCR expressed on pituitary somatotroph cells that induces the production and secretion of GH upon stimulation [27], [43]. We found that the levels of both pituitary cAMP and Zn were significantly lower in the Slc39a14-KO mice compared with control mice ( Figure 6A ). Furthermore, an intravenous bolus injection of GHRH elicited a smaller increase in the plasma GH level in the Slc39a14-KO mice than in control mice ( Figure 6B ). In addition, the induction of Gh during fasting, to which GHRH-mediated secretion contributes [44], was defective in the Slc39a14-KO mice ( Figure 6C ).
Notably, the Slc39a14-KO mice also showed a reduction in serum IGF-I ( Figure 6D ) and hepatic Igf-I expression levels ( Figure 6E ), which was not due to diminished growth hormone receptor (Ghr) expression, but could be explained by the impaired GH production ( Figure 6E ), because GH secretion stimulates IGF-I synthesis [45]. As seen in the chondrocytes, the mRNA expression levels of other SLC39 members were not significantly altered in the Slc39a14-KO pituitary cells (Figure S3). Collectively, these results indicated that SLC39A14 is selectively involved in the signaling through GHRHR, a GPCR in the pituitary gland.
SLC39A14 positively regulates gluconeogenesis via GCGR signaling in the liver
Since SLC39A14 is expressed in the liver ( Figure. 1B ) [25], [35], it may control gluconeogenesis, which occurs predominantly in the liver via signaling through the glucagon receptor (GCGR), a GPCR. Induction of the phosphoenolpyruvate carboxykinase (Pepck) gene in the liver is a critical event in the gluconeogenesis mediated by GCGR signaling [46]. As shown in Figure 7A , fasting-induced Pepck expression was significantly reduced in the Slc39a14-KO mice, although the Gcgr expression level did not change. In line with the lower Pepck induction, 36 hours of fasting significantly and continuously reduced the plasma glucose level in the Slc39a14-KO mice, whereas the plasma glucose level in the control mice plateaued after 18 hours ( Figure 7B ). These data indicated that fasting gluconeogenesis was significantly impaired in the Slc39a14-KO mice.
The Slc39a14-KO liver had a lower cAMP level, a higher PDE activity ( Figure 7C ), and a lower Zn level ( Figure 7D , left) than the control liver. The reduced Zn level was confirmed by the reduction of the mRNA expression of Mt-I, a Zn indicator whose expression is induced by Zn via the metal response element (MRE) [47] ( Figure 7E ), whereas the level of iron (Fe) in the liver was not affected in the Slc39a14-KO mice ( Figure 7D ). Taken together, these data indicated that SLC39A14 positively controls gluconeogenesis through GCGR, and thus facilitates the hepatic cAMP-CREB signaling pathway.
Discussion
Our current study demonstrated that a Zn transporter, SLC39A14, controls GPCR-mediated signaling by maintaining the basal cAMP level and suppressing PDE activity. Our results showed that SLC39A14 is a novel endogenous regulator for systemic growth and energy homeostasis, and its role may provide a mechanism for the Zn-mediated regulation of endocrine signaling ( Figure 8 ).
PTHrP-PTH1R signaling plays an important role in the endochondral ossification process, in which it blocks the premature hypertrophic differentiation of proliferative chondrocytes [37]. We concluded that SLC39A14 positively regulates PTHrP-PTH1R signaling based on the following findings. (1) The morphology of the Slc39a14-KO growth plate featured accelerated hypertrophy, characterized by the elongated pHZ and HZ, similar to observations in genetically manipulated-Pth1r mice [38], [39]. (2) The Slc39a14-KO growth plate showed increased expression levels of the hypertrophic markers Ihh and Col10a1. PTH1R signaling is reported to inhibit their expression levels [41], [48], consistent with the observation of elongated pHZ and HZ in the Slc39a14-KO mice. (3) Slc39a14-KO chondrocytes possessed a lower potential for PTH1R signal transduction.
The accelerated hypertrophy in Pth1r mutant mice might be caused not only by the accelerated differentiation of proliferative cells into hypertrophic cells, but also by the accelerated differentiation of resting cells into proliferative cells [39]. Given that Ihh acts to promote the differentiation of resting to proliferative cells and Ihh-KO mice display markedly reduced proliferation, with hypertrophy at inappropriate positions [49], it is reasonable to propose that the enhanced Ihh expression might stimulate the proliferation of resting chondrocytes accompanied by an increase in Col2a1 expression ( Figure 3B ), leading to narrowing of the RZ and PZ ( Figure 3E ), in close coordination with accelerated hypertrophy in the Slc39a14-KO growth plate. However, the morphological abnormality of the Slc39a14-KO growth plate was less severe than that of the Pth1r mutant. It is possible that other Zn transporters and/or Zn-permeable channels [50] have similar functions (e.g. Zn transport activity) as the SLC39A14 protein, although their mRNA expression levels were not altered by the loss of SLC39A14 (Figure S3). This issue remains to be clarified. Nonetheless, the intracellular Zn level was significantly reduced in the PZ but not the HZ in the Slc39a14-KO mice ( Figure 5B ), reflecting the expression pattern of Slc39a14 in the growth plate ( Figure 3B and 3C ). Our results collectively indicate that SLC39A14 plays an indispensable role in proper chondrocyte differentiation in the growth plate, by positively regulating PTH1R-mediated signaling.
Besides PTHrP-PTH1R signaling, the role of the GH-IGF-I axis in longitudinal bone growth is well established [18], [22]. It has been suggested that GH acts locally at the growth plate to induce IGF-I production, which then stimulates the proliferation of chondrocytes in a paracrine/autocrine manner, or induces resting chondrocytes to enter a proliferative state, independent of endocrine or paracrine IGF-I [22]. The Slc3914-KO mice showed significant decreases in their plasma concentrations of GH and IGF-I (aberrant GH-IGF-I axis), correlating with a low Zn level in the pituitary gland. In sharp contrast to mice lacking the Ghr gene, which have a normal birth weight and size [51], the Slc39a14-KO mice had a reduced birth weight and size ( Figure 2A and data not shown). In addition, the growth plates of Igf-I-deficient mice display reduced hypertrophy [52], whereas hypertrophy was augmented in the Slc39a14-KO mice. Therefore, it is unlikely that the reduced GH and IGF-I levels impair chondrocyte differentiation in the Slc39a14-KO mice; rather, their role is probably related to the postnatal systemic growth retardation of these mice. However, we do not exclude the possibility that the reduced IGF-I level has an effect on growth during gestation, because Igf-1-deficient mice show intrauterine growth retardation with low birth weights [53]; therefore this issue requires further clarification. Nonetheless, it seems likely that in systemic growth, SLC39A14 plays an important role in controlling GH production by regulating the basal cAMP level in GHRHR-mediated signaling. This highlights SLC39A14′s importance as a positive GPCR regulator, not only in endochondral ossification, but also in GH production, thus concomitantly regulating systemic growth through these processes. Finally, our findings provide a mechanism that explains the reductions in GH and IGF-I in cases of Zn deficiency [20].
Here, we extended previous work on the importance of SLC39A14 in the signaling of a hepatic GPCR, GCGR, which controls gluconeogenesis during fasting. The liver regulates the metabolism of both Zn and Fe [54], [55]. We found that neither the hepatic ( Figure 7D ) nor the serum (data not shown) Fe level was altered in the Slc39a14-KO mice, suggesting that SLC39A14 specifically regulates the Zn metabolism in the liver at steady state. Overall, our results indicate that SLC39A14 may be a new player in the positive regulation of GPCR-mediated signaling in various systems ( Figure 8 ).
It is noteworthy that the single ablation of the Slc39a14 gene was sufficient to provoke abnormal chondrocyte differentiation. There are phenotypic similarities between the Slc39a14-KO mice and mice deficient in SLC39A13, another Zn transporter that is also required for mammalian growth. Slc39a13-KO mice show systemic growth retardation accompanied by impaired endochondral ossification [8]. In addition, Slc39a14 and Slc39a13 have similar distributions in the growth plate; they are both highly expressed in the PZ. However, the growth plate morphologies of the Slc39a14-KO mice are quite different from those of the Slc39a13-KO mice: the PZ shows narrowing in the Slc39a14-KO mice but elongation and disorganization in the Slc39a13-KO mice, and the HZ is elongated in the Slc39a14-KO mice, but is scanty in Slc39a13-KO mice, suggesting that SLC39A14 and SLC39A13 have distinct biological roles in growth control. These Zn transporters also have different cellular localizations. SLC39A14 is a cell-surface-localized transporter that controls the total cellular Zn content, whereas SLC39A13 localizes to the Golgi and regulates the local intracellular Zn distribution. Thus, the intracellular Zn status (e.g. accumulation and distribution of Zn) is controlled by various Zn transporters (e.g. SLC39A14 and SLC39A13), which influence distinct signaling pathways (GPCR by SLC39A14 and BMP/TGF-β by SLC39A13) leading to mammalian growth, in which many essential signaling events participate [18], [21], [22]. Furthermore, the expression level of Slc39a13 was not changed in Slc39a14-KO cells (Figure S3), suggesting that SLC39A14 plays a unique biological role in controlling the GPCR signaling pathway, with little help from a backup system to compensate for its loss. The intracellular localization, expression level, Zn-transport activity, and post-translational modifications [4] may determine the specificity of each Zn transporter. Thus, our findings strongly suggest that SLC39A14 and SLC39A13 control skeletal growth by differentially regulating the Zn status to affect distinct signaling pathway(s), even though the growth phenotypes of their KO mice are similar. Our results support a new concept that different “Zn transporter-Zn status” axes act in unique signaling pathways to promote systemic growth.
In this study, it was not clarified how Zn acts through SLC39A14 to suppress PDE activity. SLC39A14 may regulate PDE activities by modulating the intracellular Zn level [56], [57] in tissues that express SLC39A14 and contain high concentrations of Zn [20], [58], [59]. As illustrated in Figure 8 , the SLC39A14-mediated inhibitory effect may be due to the direct action of the transported Zn or to an indirect one via unidentified molecular chaperone(s) (Protein X) that receives Zn through SLC39A14 and provides it to PDE. Since GPCRs are expressed in numerous tissues, the Slc39a14-KO mice may be useful for studying GPCR-mediated biological events. Further studies on the mechanism by which SLC39A14 provides Zn to target molecules should help illuminate the regulation of GPCR-mediated signaling and Zn–associated biological events.
Materials and Methods
Mice
Mice were maintained on a 12-hour light-dark cycle, with a regular unrestricted diet available ad libitum. Mice at 6-8-weeks old were used for X-ray radiographic bone analysis, using a composite X-ray analyzing system (In vivo 3D Micro X-ray CT System R_mCT, Rigaku), and for bone histomorphometric analysis, using a semiautomatic image analyzing system (OsteoplanII; Carl Zeiss). Four-week-old mice were used for in situ hybridization analysis by the method of GENOSTAFF CO., LTD., and for analysis of the intracellular Zn level using an Electron Probe X-ray Micro Analyzer (JXA9200 II, JOEL). For analysis of the pituitary gland and liver, 3-52-week-old mice were evaluated under ad libitum or fasted conditions.
Generation of Slc39a14-KO mice
The knockout mouse line of the Slc39a14 gene was generated using previously described methods [60]. The RPCI-23 MM BAC (bacterial artificial chromosome) clone (Clone ID; 125B6), containing the mouse Slc39a14 gene, was purchased from Invitrogen. A targeting vector was created to eliminate the genomic region encompassing exons 5–8 by inserting a Neo-cassette between exons 4 and 9 of Slc39a14, and deleting the intervening exons ( Figure. 1A ). This region contains the histidine-rich domain and conserved HEXPHEXGD motif that are common to SLC39 family members [36]. This vector was introduced into B6×129+Ter/SvJcl hybrid M1 ES cells, the cloned homologous recombinants were selected with antibiotics, and the genotypes were verified. We developed chimeric mice with the targeted ES-cell clones, and obtained homozygous mice by interbreeding the offspring. Heterozygous mice were phenotypically normal, and crosses between heterozygotes produced homozygous mutant mice according to Mendelian expectations. Genotyping was done by PCR using Taq polymerase (GE Healthcare). The primers used for genotyping were:
Forward: 5′- TGCTGCTGCTATTTGGGTCT -3′ for the wild-type allele
Forward: 5′- CTCGTGCTTTACGGTATCGC -3′ for the targeted allele and Reverse: 5′-GAATGCTGCATTGAAAAGGTC –3′, which was the same for the wild-type and targeted alleles.
Ethics Statement
All animal experimental procedures were conducted according to guidelines approved by the RIKEN Institutional Animal Care and Use Committee (#22-013).
Plasmid construction, transfection, and viral infection
The coding regions of the mouse Slc39a14a and Slc39a14b genes [35] were isolated from a liver cDNA library of the C57BL/6 mouse. To construct a C-terminally V5-tagged Slc39a14a (Slc39a14a–v5), the Slc39a14a fragments were amplified by PCR, followed by sequencing and cloning into the expression vector pcDNA6.2/V5-DEST (Invitrogen). To construct an N-terminally hemagglutinin (HA)-tagged Slc39a14a or Slc39a14b cDNA-lentiviral vector, the HA-tag sequence was inserted into the N-terminus of Slc39a14a or Slc39a14b by PCR, followed by ligating with CSII-CMV-IRES-hrGFP. Cells were transfected with expression vectors using Lipofectamine 2000 (Invitrogen). For lentiviral infections, 293T cells were transfected with Slc39a14a or Slc39a14b cDNA-containing CSII-CMV-IRES-hrGFP, pMDLg/p.RRE, pRSV-Rev, and pMD.G (VSV-G). After a 12-hour incubation, the culture medium was replaced with fresh medium, and then collected 24- and 48-hours later. The culture supernatants containing packaged lentivirus were pooled and concentrated using a Lenti-X concentrator (Clontech). The virus pellet was resuspended, and the virus titer was measured using the Lenti-X qRT-PCR Titration Kit (Clontech). Two or three days after starting the primary chondrocyte cell culture, the cells were infected with the Slc39a14a or Slc39a14b cDNA-carrying lentivirus in 8 µg/ml polybrene (Sigma) containing 10% FCS-α-MEM. After 2 days of infection, the cells were used for further analysis.
Reagents and Antibodies
Human PTHrP (1-34) and (Nle27)-GHRH (1-29) amide were from Bachem. FSK and the broad-range PDE inhibitor (IBMX) were from Sigma. Pyrithione and Zn sulfate heptahydrate were from Molecular Probes and Wako Pure Chemical Industries, Ltd., respectively. Peptide N-glycosidase F (PNGase F) was from New England Biolabs. The anti-mouse SLC39A14 antibody was raised by immunizing rabbits with a KLH-conjugated peptide (CNSELDGKAPGTDEKV). Anti-CREB and anti-p-CREB (S133; 634-2) antibodies were from Millipore. The anti-PKA-Cα antibody was from Cell Signaling Technology. The anti-tubulin and anti-HDAC1 antibodies were from Sigma. The anti-PTH1R (K-20) and anti-V5 antibodies were from Abcam and Invitrogen, respectively.
PNGase F treatment
Cell lysates were denatured in denaturing buffer (0.5% SDS and 40 mM DTT) at 37°C for 30 min. Nonidet P-40 and sodium phosphate (pH 7.5, 25°C) were added at final concentrations of 1% and 50 mM, respectively. Subsequently, PNGase F was added and the mixture was incubated at 37°C for 1 h. The samples were then denatured with SDS-PAGE loading buffer (37°C for 15 min) prior to immunoblotting.
Measurement of cAMP level and PDE activity
The cAMP level and PDE activity in primary chondrocytes, pituitary cells, and liver were measured with the cAMP-Glo assay kit and PDE-Glo Phosphodiesterase assay kit (Promega), according to the manufacturer's instructions.
RT-PCR and Quantitative RT-PCR (RT-qPCR) analyses
The total RNA was extracted from primary chondrocytes, pituitary cells, and liver using Sepasol-RNA I (Nacalai Tesque), and reverse-transcribed with an oligo-(dT) primer and reverse transcriptase (ReverTra Ace, Toyobo). RT-qPCR analysis was performed using the SYBR Green PCR Master Mix (Applied Biosystems). Samples were normalized to the Gapdh or β-actin expression. Primer sequences are available upon request.
Enzyme-linked Immunosorbent assay (ELISA)
The serum IGF-I and plasma GH level were measured using the Mouse/Rat IGF-I Quantikine ELISA Kit (R&D Systems) and Rat/Mouse Growth Hormone ELISA kit (Millipore), according to the manufacturers' instructions.
Measurement of Zn level
To measure the intracellular Zn level in pituitary cells, the pituitary gland was isolated and incubated with Trypsin/EDTA (Nacalai Tesque) at 37°C for 10 min. After being washed with PBS, the cells were loaded with 10 µM cell-permeant FluoZinTM-3 AM (Invitrogen) in plain RPMI medium (Sigma) at 37°C for 30 min. The cells were further incubated in fresh plain RPMI medium for 30 min prior to measuring the Zn level by flow cytometric analysis.
For the experiment using lentivirus-transduced chondrocytes, the cell lysates were boiled at 98°C for 10 min to inactivate the reporter protein, hrGFP, expressed from the IRES translation initiation sequence in the lentiviral vector. The cell lysates were diluted in cell-impermeant 10 µM FluoZinTM-3, tetrapotassium salt (Invitrogen) in 10 mM Tris-HCl (pH 7.4), and incubated for 30 sec prior to measuring the maximal emission at 516 nm (excitation at 494 nm) using a Varioskan (Thermo Electron Corporation). The hepatic Zn and Fe levels were measured by Inductively Coupled Plasma Mass Spectrometry (ICP-MS). An Electron Probe X-ray Micro Analyzer (JXA9200 II, JOEL) was used to measure the intracellular Zn level in the growth plate. Control- and Slc39a14-KO-derived growth plates were fixed with 1.25% glutaraldehyde and 1% paraformaldehyde in 0.1 M phosphate buffer, pH 7.4, then post-fixed in 2% osmium tetroxide, dehydrated in an ascending series of alcohol, and embedded in epoxy resin. The proliferative and hypertrophic chondrocytes in the embedded growth plate were scanned by an electron beam. The characteristic X-ray for Zn generated by the electron-beam exposure was detected.
Histological and in situ hybridization analyses
Paraffin sections (4∼6 µm) processed from the tibia of 4-week-old mice or E17.5 embryos were prepared for hematoxylin and eosin (H&E) staining and for in situ hybridization analysis. Digoxigenin-labeled antisense RNA probes for Slc39a14, Col2a1, Col10a1, Ihh and Pth1r were used for in situ hybridization analysis by the method of GENOSTAFF CO., LTD. The sections used in the in situ hybridization analysis were counterstained with Kernechtrot stain solution. The probe sequences and hybridization conditions are available upon request.
Isolation and culture of mouse primary chondrocytes, subcellular fractionation, immunoblotting, confocal microscopy, X-ray analysis, and bone histomorphometric analysis
Primary chondrocytes were isolated from the ribs as described previously [8]. The subcellular fractionation, immunoblotting, confocal microscopy, X-ray analysis, and bone histomorphometric analysis were performed using previously described methods [8].
Statistical analysis
Differences among multiple groups were compared by 1-way ANOVA followed by a post-hoc comparison using Fisher's PLSD test. The two-tailed Student's t-test was used to analyze the difference between two groups.
Supporting Information
Acknowledgments
We thank Dr. Daniel Nebert (University of Cincinnati Medical Center) for critical reading and various suggestions, Dr. Jun Shinga (RIKEN, RCAI) for helpful experimental advice on the generation of the knockout mouse, and Drs. Akira Shibuya and Kazuko Shibuya (University of Tsukuba, Center for TARA) for the CSII-CMV-MCS-IRES-hrGFP, pMDLg/p.RRE, pRSV-REV, and pMD.G. We are grateful to Mr. Masaru Emura and Mr. Masami Kawamura for their excellent technical assistance. We also thank Ms. Mizuki Shimura and Ms. Ryoko Masuda for their secretarial assistance.
Footnotes
Competing Interests: The authors have declared that no competing interests exist.
Funding: This work was supported by KAKENHI (#20249030) and the JST-CREST program (http://www.jst.go.jp/kisoken/crest/en/area03/2-05.html). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
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