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World J Gastroenterol. Jun 21, 2015; 21(23): 7142-7154
Published online Jun 21, 2015. doi: 10.3748/wjg.v21.i23.7142
Molecular aspects of intestinal calcium absorption
Gabriela Diaz de Barboza, Solange Guizzardi, Nori Tolosa de Talamoni, Cátedra de Bioquímica y Biología Molecular, Facultad de Ciencias Médicas, Universidad Nacional de Córdoba, Córdoba 5000, Argentina
Author contributions: Diaz de Barboza G, Guizzardi S and Tolosa de Talamoni N participated in information collection, analysis, information organization, writing, figure design, and final editing.
Conflict-of-interest: Dr. N. Tolosa de Talamoni is a Member of Career from CONICET (COnsejo Nacional de Investigaciones CIentíficas y Técnicas. Solange Guizzardi is a fellow from CONICET.
Open-Access: This article is an open-access article which was selected by an in-house editor and fully peer-reviewed by external reviewers. It is distributed in accordance with the Creative Commons Attribution Non Commercial (CC BY-NC 4.0) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited and the use is non-commercial. See: http://creativecommons.org/licenses/by-nc/4.0/
Correspondence to: Nori Tolosa de Talamoni, Professor, Cátedra de Bioquímica y Biología Molecular, Facultad de Ciencias Médicas, Universidad Nacional de Córdoba, Av. Haya de la Torre s/n, Córdoba 5000, Argentina. ntolosa@biomed.fcm.unc.edu.ar
Telephone: +54-351-4333024
Received: January 28, 2015
Peer-review started: January 28, 2015
First decision: March 10, 2015
Revised: March 21, 2015
Accepted: April 17, 2015
Article in press: April 17, 2015
Published online: June 21, 2015
Processing time: 143 Days and 12.5 Hours

Abstract

Intestinal Ca2+ absorption is a crucial physiological process for maintaining bone mineralization and Ca2+ homeostasis. It occurs through the transcellular and paracellular pathways. The first route comprises 3 steps: the entrance of Ca2+ across the brush border membranes (BBM) of enterocytes through epithelial Ca2+ channels TRPV6, TRPV5, and Cav1.3; Ca2+ movement from the BBM to the basolateral membranes by binding proteins with high Ca2+ affinity (such as CB9k); and Ca2+ extrusion into the blood. Plasma membrane Ca2+ ATPase (PMCA1b) and sodium calcium exchanger (NCX1) are mainly involved in the exit of Ca2+ from enterocytes. A novel molecule, the 4.1R protein, seems to be a partner of PMCA1b, since both molecules co-localize and interact. The paracellular pathway consists of Ca2+ transport through transmembrane proteins of tight junction structures, such as claudins 2, 12, and 15. There is evidence of crosstalk between the transcellular and paracellular pathways in intestinal Ca2+ transport. When intestinal oxidative stress is triggered, there is a decrease in the expression of several molecules of both pathways that inhibit intestinal Ca2+ absorption. Normalization of redox status in the intestine with drugs such as quercetin, ursodeoxycholic acid, or melatonin return intestinal Ca2+ transport to control values. Calcitriol [1,25(OH)2D3] is the major controlling hormone of intestinal Ca2+ transport. It increases the gene and protein expression of most of the molecules involved in both pathways. PTH, thyroid hormones, estrogens, prolactin, growth hormone, and glucocorticoids apparently also regulate Ca2+ transport by direct action, indirect mechanism mediated by the increase of renal 1,25(OH)2D3 production, or both. Different physiological conditions, such as growth, pregnancy, lactation, and aging, adjust intestinal Ca2+ absorption according to Ca2+ demands. Better knowledge of the molecular details of intestinal Ca2+ absorption could lead to the development of nutritional and medical strategies for optimizing the efficiency of intestinal Ca2+ absorption and preventing osteoporosis and other pathologies related to Ca2+ metabolism.

Key Words: Intestinal Ca2+ absorption; Transcellular pathway; Paracellular route; 1,25(OH)2D3; PTH; Prolactin; Estrogen; Lactation; Pregnancy; Aging

Core tip: Intestinal Ca2+ absorption occurs through transcellular and paracellular pathways. Apparently, novel proteins, such as Cav1.3 and 4.1R, are involved in the Ca2+ transcellular pathway. Proteins involved in tight junction structures, such as claudins 2, 12, and 15, participate in the paracellular pathway. There is evidence of crosstalk between the transcellular and paracellular pathways. Better knowledge of the molecular details of intestinal Ca2+ absorption could lead to the development of nutritional and medical strategies for optimizing the efficiency of intestinal Ca2+ absorption and preventing osteoporosis and other pathologies related to Ca2+ metabolism.



INTRODUCTION

The Ca2+ ion plays an important role during human life. The accumulation of Ca2+ in the first decades of life allows for the achievement of optimal peak bone mass and, later in life, the maintenance of bone mass. It is a key constituent of many essential physiological processes, from intracellular signals to the mineralization of bone[1]. It is well known that Ca2+ is involved in nerve impulse transmission, muscle contraction, blood coagulation, secretory activity, cell death, cell differentiation, immune response, and enzyme activation[2]. The dysregulation of Ca2+ homeostasis is associated with bone disorders, metabolic diseases[3], and an increase in the risk of epithelial cancers[4].

The intestine, kidney, bone, and parathyroid glands work together to maintain serum Ca2+ within a narrow range. Intestinal Ca2+ absorption is a crucial process for the maintenance of Ca2+ balance and bone health. It occurs through two main mechanisms: transcellular, metabolically driven transport, and a passive non-saturable route called the paracellular pathway[5]. Both pathways are regulated by hormones, nutrients, and other factors. There has been much research work dedicated to ascertaining the regulation mechanisms of these factors due to their high relevance in the prevention of osteoporosis and other pathologies related to Ca2+ metabolism.

The transcellular pathway implicates Ca2+ movement from the mucosal-to-serosal side of the intestinal barrier that occurs against a concentration gradient. It is an active saturable process that predominates in the duodenum and jejunum, and is regulated by nutritional and physiological factors, mainly vitamin D. The paracellular mechanism is a non-saturable and passive transport that occurs across the majority of the intestine and is a linear function of luminal Ca2+ concentration[6]. Recently, it has been demonstrated that Ca2+ transport through the paracellular shunt is also significantly regulated[1].

The total Ca2+ absorbed depends on the amount of Ca2+ consumed, the sojourn time in the various segments of the small and large intestine, and the amount of soluble Ca2+ available for absorption, which is mainly determined by the pH in each segment. The acidic environment of the stomach dissolves calcium salts into Ca2+ ions. However, the pH of stomach is less relevant than that of the other segments, as Ca2+ is absorbed in the small and large intestine. The average pH is 7.3 in the small intestine and 6.6 in the colon. When pH increases, Ca solubility decreases. Nevertheless, the duodenum seems to be the site with the maximum solubility of Ca, as the average pH is 6.0, which is the lowest in the entire gut[7].

TRANSCELLULAR PATHWAY

The transcellular pathway of intestinal Ca2+ absorption comprises 3 steps: the entrance of Ca2+ across the brush border membranes (BBM) of enterocytes through epithelial Ca2+ channels; Ca2+ movement from the BBM to the basolateral membranes (BLM) by binding to proteins with high Ca2+ affinity [(calbindins (CB)]; and Ca2+ extrusion into the blood via plasma membrane Ca2+-ATPase (PMCA1b/Ca2+ pump) and the Na+/Ca2+ exchanger (NCX1)[5].

Epithelial Ca2+ channels

Two epithelial Ca2+ channels seem to be involved with Ca2+ entry to enterocytes: the epithelial Ca2+ channel transient receptor potential vanilloid 6 (TRPV6; previously named ECaC2 and CaT1) and TRPV5 (previously named ECaC1 and CaT2). Both molecules are co-expressed in the human kidney and intestine, but TRPV6 is highly expressed in the intestine and TRPV5 is the major isoform in the kidney. High levels of TRPV6 have been detected in the duodenum and colon of humans, rats, and mice[8-10]. Although TRPV6 is one of the key players in human intestinal Ca2+ absorption, its precise role needs to be investigated. In TRPV6-/- mice, a considerable amount of Ca2+ transport still occurs, which suggests that some other channels or molecules contribute significantly to intestinal Ca2+ absorption[11]. TRPV6 and TRPV5 are also present in other organs, such as the pancreas, prostate, mammary glands, sweat, and salivary glands[11]. Both channels can be combined to form heterotetrameric channel complexes with different properties[12]. They originate from two genes juxtaposed on human chromosome 7q35, have 75% homology, but differ in the N and C terminal tails. They are regulated by calcitriol, estrogen, and dietary Ca2+. However, the inactivation of both by intracellular Ca2+ shows different kinetics, and the response to ruthenium red is also different. Ruthenium red is a potent blocker of epithelial Ca2+ channel activity. However, TRPV6 has a 100-fold lower affinity for ruthenium red (IC50 9 ± 1 μm) than TRPV5 (IC50 121 ± 13 nm)[12]. In vitro studies demonstrate that a negatively charged amino acid (D) within the putative pore region of mouse TRPV6 (position 541 in mice; position 542 in humans) is critical for Ca2+ permeation of the channel. Woudenberg-Vrenken et al[13] analyzed the role of TRPV6 in transepithelial Ca2+ transport in vivo by using a TRPV6D541A/D541A knock-in mouse model. TRPV6D541A/D541A mice showed significantly impaired intestinal Ca2+ uptake compared with wild-type mice, and duodenal TRPV5 expression was increased, but insufficient to correct the diminished Ca2+ absorption. Since intestinal Ca2+ absorption was not totally abolished in the TRPV6D541A/D541A mice, the authors suggest that other transport mechanisms, either paracellular or an as yet unidentified transcellular transport mechanism, were functioning.

Cav1.3 is an L-type channel, located in the apical membrane, capable of active, transcellular Ca2+ absorption in the intestine. It has been hypothesized that TRPV6 and Cav1.3 have complementary roles in Ca2+ entry. TRPV6 plays a dominant role under the polarizing conditions between meals. Overnight or during starvation, the BBM repolarize and the intestine gradually atrophies, so the Ca2+ lost into the lumen by desquamation must be recovered. TRPV6 is activated by apical membrane repolarization and upregulated by vitamin D to avoid massive loss of Ca2+ from the body. In contrast, Cav1.3 plays a dominant role under depolarizing conditions, such as during digestion, mainly when diet and Ca2+ are plentiful. Glucose, amino acids, and peptides may activate Cav1.3 and inhibit TRPV6. The general distribution of TRPV6 and Cav1.3 is in line with the aforementioned hypothesis. TRPV6 levels are higher in the duodenum, which has a polarizing environment and decreases through the jejunum to the ileum. In contrast, Cav1.3 levels are low in the duodenum, but high from the proximal jejunum to the mid-ileum. The interplay of TRPV6 and Cav1.3 maintains the tight control of free Ca2+ concentration in the extracellular space at any time of day. TRPV6 and Cav1.3 would have independent and complementary actions through activation by repolarization or depolarization between digestive periods or during digestion, respectively[14].

TRPV6 transcripts were detected in the duodenum, but not in the ileum of human intestinal biopsies. The duodenal expression of TRPV6 in men was vitamin D dependent, whereas in elderly women TRPV6 and vitamin D receptor (VDR) expressions were low and not vitamin D dependent. This might explain, at least in part, the lower intestinal Ca2+ absorption in elderly post-menopausal women[15]. In mice, the basal levels of TRPV6 protein in the duodenum, ileum, and colon have been found in the rank order of duodenum > colon (72% of duodenum) > ileum (25% of duodenum)[16].

Calbindins

Traditionally, calbindins (CB) were proteins considered to be responsible for carrying Ca2+ from the apical side of the enterocyte to the BLM of the cell. CB9k (human gene symbol: S100G) is present in the intestine of mammals and CB28k (Mr ≈ 29 kDa; human gene symbol: CALB1) in the intestine of avian species[17]. CB9k is the smallest protein with four alpha-helical regions, which form an EF-hand pair consisting of a canonical and non-canonical/pseudo EF-hand domain, joined by a linker region. Two Ca2+ ions bind the EF-hand domains with positive cooperativity[18]. CB28k has six EF-hand domains, but only the four medium/high affinity sites are considered Ca2+-specific[19].

CBs not only carry Ca2+ from the apical side to the BLM of enterocytes, but also buffer Ca2+ maintaining intracellular Ca2+ concentrations below 10-7 mol/L, which prevents premature cell death by apoptosis. Excess Ca2+ resulting from a downregulation of CBs may trigger apoptosis in the epithelial cells[20]. It is known that a high concentration of free Ca2+ provokes apoptosis in many different cell types. CB28k is able to inhibit apoptosis in osteoblastic cells[21] and in germ cells from Robertsonian mice[22,23]. In the kidney, CB28k acts as a dynamic buffer which regulates Ca2+ concentration in the vicinity to the TRPV5 pore by direct association with the channel[24]. The possibility that these mechanisms occur in the intestine and other tissues with important fluctuations of intracellular Ca2+ should be explored.

The regulation of human intestinal CB9k is not completely elucidated. CB9k is actively expressed in enterocytes, which are the predominant cells of the duodenal mucosa, and its expression decreases along the gastrointestinal tract until finally reaching undetectable levels in the distal ileum and large intestine[25]. It is quite intriguing that intestinal CB9k expression increases with age in the bulb and 2nd portion of the duodenum, whereas the plasma Ca2+ levels decrease[26]. In rodents, CB9k is regulated at the transcriptional and post-transcriptional levels by 1,25-dihydroxyvitamin D3 [1,25(OH)2D3 (calcitriol)], with the hormonal form derived from vitamin D[27-29]. It has been observed in mice that TRPV6 and CB9k are similarly regulated. Both proteins are induced at weaning or under low Ca diet and after 1,25(OH)2D3 administration. It is important to note that the induction of these proteins occur before the peak of intestinal Ca2+ absorption[30]. Christakos et al[31] have suggested that CB9k and TRPV6 are associated, with the function of CB9k being to facilitate TRPV6-mediated Ca2+ influx by preventing Ca2+ channel inactivation, but this requires further evidence to be proven.

Hwang et al[32] have demonstrated that an ablation of CB9k alters the expression of paracellular tight junction (TJ) genes. The compensatory expression of paracellular TJ genes in the duodenum was associated with transcellular CB9k, but not CB28k. This crosstalk between the transcellular and paracellular pathways might partially explain the variety of gut responses to the absorption of Ca2+ under different pathophysiological conditions.

Ca2+ pump and Na+/Ca2+ exchanger

Ca2+ extrusion from enterocytes is performed by two proteins: PMCA1 and NCX1. PMCA1 was first detected in erythrocyte membranes and found to have a high affinity for Ca2+[33]. There are four PMCA isoforms (PMCA1 to 4) that are in turn divided into several subtypes by alternative splicing. In mammals, four different genes encode PMCA, which in humans are located on four different chromosomes. For the four genes, two splice sites have been characterized, which are positioned either close to or within the regulatory regions of the pump, giving rise to many spliced isoforms[34]. PMCA1 is known as the housekeeping isoform because its mRNA is found in all tissues, but this concept is now questionable due to several factors involved in its regulation[35]. The predominant form in the intestine is the isoform PMCA1b, the expression and activity of which is higher in enterocytes from the villus tip in comparison with those from the villus crypt[36]. This finding agrees with the idea that mature enterocytes have the greatest capacity for transcellular Ca2+ movement. In chick intestine, vitamin D deficiency decreases the expression and activity of PMCA1b, which can be partially reversed by a single large dose of cholecalciferol[37].

PMCAs can be activated by Ca2+/calmodulin, acidic phospholipids, and serine/threonine phosphorylation, and can interact with numerous molecules[38]. The novel protein 4.1R seems to be a partner of PMCA1b, which could have a crucial role in the transcellular Ca2+ pathway. The protein 4.1R was first identified in the erythrocyte membrane skeleton, and is expressed in the epithelia of the intestine and other epithelia. So far, its physiological function is not well known. Liu et al[39] found that 4.1R co-localizes with PMCA1b. They also found that 4.1R KO mice exhibit impairment in intestinal Ca2+ absorption and decreased expression of PMCA1b in enterocytes. The association between PMCA1b and 4.1R involves the membrane-binding domain of 4.1R, as well as the second intracellular loop and C-terminus of PMCA1b. The finding that the protein 4.1R binds to PMCA1b suggests that protein 4.1R may regulate the function of PMCA1b and, consequently, intestinal Ca2+ absorption.

PMCA1b is the main protein involved in the exit of Ca2+ from enterocytes[40]. In contrast, NCX1 is only responsible for about 20% of Ca2+ extrusion from the intestine to plasma[41]. Because of that, this exchanger has received little attention, with some reviews ignoring it as another molecule involved in the exit of Ca2+ from the intestine. In contrast, NCX1 is critical for Ca² regulation in cardiac muscle, vascular smooth muscle, and nerve fibers, and most of the literature about NCX1 refers to these organs[42-44]. NCX electrogenically exchanges Na+ and Ca2+ across the plasma membrane, depending on membrane potential and ion gradients[45]. This exchanger has a stoichiometry of 3 Na+:1 Ca2+, and can operate in either a forward mode (Ca2+ extrusion) or in a reversed mode (Ca2+ entry), which depends on the Na+ and Ca2+ gradients and the potential across the plasma membrane[46,47]. The expression and activity of NCX1 are quite similar between mature and immature enterocytes from chick duodenum, but are slightly higher in the villus tip cells[36].

PARACELLULAR PATHWAY

The movement of molecules and ions through this pathway is regulated by the TJ, which are specialized membrane domains mostly positioned in the apical region of enterocytes. TJ are intercellular structures where plasma membranes of adjacent cells have very close contact. These junctions are composed of transmembrane proteins, cytoskeleton components, and cytoplasmic plaques[48]. The transmembrane proteins of TJ structures are synthesized in adjacent cells and include occludin (Ocln) and claudins (Cldns). These proteins close intercellular junctions and restrict the free movement of materials through the paracellular space. Cldn 2, 12, and 15 are responsible for transporting Ca2+ in the intestine[49,50]. Cldn 1 and Cldn 5 have clear sealing functions that might also affect Ca2+ transport, as they influence general paracellular permeability[51,52]. The involvement of Ocln in intestinal Ca2+ absorption remains to be determined. Ocln is a tetraspan transmembrane protein, but its precise function is not well established[32]. Cytoplasmic plaques, such as zona occludens (ZO) proteins, contain a binding domain for transmembrane proteins[53]. ZO-1, a cytoplasmic protein with the ability to bind with both occludin and claudins[54], is associated with the structure and formation of the TJ, and possibly with paracellular ion transport[55]. Although it is not clear whether ZO-1 has a physiological role in intestinal Ca2+ transport, the increase in ZO-1 expression in the intestine of rats with 21-d chronic metabolic acidosis suggests that this protein might be implicated in intestinal Ca2+ absorption[56].

Ca2+ transport through the TJ is a passive process which depends on the concentration and electric gradient across the epithelium. The process is non-saturable transport that predominates in the jejunum and ileum when Ca2+ intake is adequate or high[57]. This route becomes important when Ca2+ intake is high, because the sojourn time in the intestine is short and there is a downregulation of proteins involved in the transcellular pathway[58] (Figure 1).

Figure 1
Figure 1 Schematic representation of intestinal Ca2+ absorption. ADP: Adenosine monophosphate; ATP: Adenosine triphosphate; Cldns: Claudins; NCX1: Intestinal Na+/Ca2+ exchanger; PMCA1b: Plasma membrane Ca2+- ATPase 1b; TJ: Tight junctions; TRPV6: Transient receptor potential vanilloid 6; TRPV5: Transient receptor potential vanilloid 5; VDR: Vitamin D receptor; 1,25(OH)2D3: Calcitriol.

As previously mentioned, it seems that there is crosstalk between the transcellular and paracellular pathways involved in intestinal Ca2+ absorption. The expression of most TJ genes in the duodenum was significantly increased in CB9k KO mice compared to wild-type animals under a normal diet. A deficiency in dietary Ca2+ or vitamin D decreased TJ gene expression in CB9k KO mice. The data indicate that the expression of paracellular TJ genes is regulated by transcellular CB proteins, which suggests that active and passive Ca2+ transport pathways may function cooperatively[32]. More research work is necessary to clarify the network of transcellular and paracellular pathways for intestinal Ca2+ absorption.

Intestinal redox status is critical for both transcellular and paracellular pathways of intestinal Ca2+ absorption. Xiao et al[59] have demonstrated that a duodenal oxidation state induced by a high fat diet could significantly downregulate the expression of CB9k, PMCA1b, and NCX, as well as inhibiting intestinal calcium absorption. We have recently demonstrated that type I diabetes mellitus transiently inhibits intestinal Ca2+ absorption. Inhibition is accompanied by oxidative stress, which alters the gene and protein expression of molecules involved in the transcellular and paracellular pathways. When insulin is administered, the duodenal redox state returns to the control values, while intestinal Ca2+ absorption normalizes[60]. Similarly, oxidant drugs such as menadione, DL-buthionine-S,R-sulfoximine, and sodium deoxycholate decrease intestinal glutathione content, thereby affecting mainly the gene and protein expression of molecules involved in the transcellular pathway of intestinal Ca2+ absorption. Normalization of redox status with drugs such as quercetin, ursodeoxycholic acid, and melatonin returns intestinal Ca2+ transport to control values[61-65].

Molecular mechanisms of 1,25(OH)2D3-mediated intestinal Ca2+ absorption

1,25 (OH)2D3 is the major controlling hormone of intestinal Ca2+ absorption. It causes changes in the structure and function of enterocytes[66,37], which enhance Ca2+ transport across the intestine. The action of calcitriol is mediated by genomic and non-genomic mechanisms after binding VDR. This receptor, located mainly in the nucleus, is a transcription factor that mediates the cellular effects of vitamin D by binding the vitamin D response elements of target genes[67]. The critical role of VDR and its ligand in intestinal Ca2+ absorption was confirmed in VDR KO mice in the third week of life. At birth, VDR KO mice are indistinguishable from their normal littermates. Alterations in growth and mineral ion homeostasis begin later[68], which is consistent with the observation that intestinal Ca2+ absorption is vitamin D independent in rodents in the first weeks of life[69]. Ten-week-old VDR KO mice showed a dramatic decrease in duodenal Ca2+ absorption, which was associated with impaired expression of TRPV6, TRPV5, and CB9k[70]. Beyond VDR function in intestinal Ca2+ absorption, a recent proteomic approach has revealed that VDR is also an important factor for controlling cell proliferation, migration, and stress response in the small intestine[71].

Most studies related to the effect of calcitriol on intestinal Ca2+ absorption have been focused on the transcellular Ca2+ pathway. All molecules presumably involved in this route are increased by calcitriol in experimental animals, and even in humans[72-75].

Cyp24a1 is a major VDR-responsive gene that metabolizes 1,25(OH)2D3 into 1,24,25-trihydroxyvitamin D3 and 25(OH)D3 into 24,25-dihydroxyvitamin D3[76], while Cyp27b1 is the gene involved in the synthesis of 1,25(OH)2D3, which is mainly located in the kidney[77], but is also expressed in other tissues, such as the intestine[78] and parathyroid gland[79]. Both genes are regulated by 1,25(OH)2D3 levels. Their temporal profiles and those from other VDR responsive genes were analyzed in the intestine and other tissues of mice after single and multiple dosing of 1,25(OH)2D3. Due to the lipophilic nature of the compound, a rapid distribution of 1,25(OH)2D3 into tissues was observed, regardless of variation in VDR abundance in different tissues. The maximal induction of VDR target genes such as TRPV6 and Cyp24a1 mRNA expression in the intestine were similar after single vs multiple dosing, with a peak between 3 and 9 h post-injection, whereas the peak of 1,25(OH)2D3 concentration in the ileum occurred at 0.5-1 h. This lag time was the result of the time required for translocation of the VDR into the nucleus in order to heterodimerize with the RXR to initiate the transcription. An increase in ileal VDR levels was also observed, as well as an attenuation of serum PTH and a decrease in renal Cyp27b1 expression after a time delay in VDR activation. The data revealed that exogenous 1,25(OH)2D3 enters the intestine, rapidly equilibrates, and then VDR target genes respond quickly. Consequently, plasma Ca2+ levels increase as a result of enhanced intestinal Ca2+ absorption[16].

1,25(OH)2D3-enhanced Ca2+ transport in mice was reported to be inhibited by fibroblast growth factor-23 (FGF-23), as well as Ca2+ transport in colon cancer Caco-2 cells. FGF-23 produced an abolishment of enhanced transcellular active Ca2+ fluxes and a modest downregulation of the paracellular Ca2+ route[80].

VDR null mice adapt to pregnancy by the upregulation of duodenal TRPV6 and intestinal Ca2+ absorption. These mice lactate normally and fully restore bone mineral content after weaning. Therefore, VDR seems not to be required for skeletal adaptation during pregnancy, lactation, and after weaning[81]. In the elderly, there is a decrease in intestinal Ca2+ absorption, and thus higher Ca2+ intake is needed. Increasing Ca2+ intake via dairy products and Ca2+-fortified food is a much better option than supplements. It has been estimated a 30% reduction in fractures for elderly individuals is possible by using the simple and inexpensive strategy of a daily vitamin D intake of 800 IU, together with a total Ca2+ intake of 1000 mg/d[82].

The paracellular pathway of intestinal Ca2+ absorption has been demonstrated to also be increased by 1,25(OH)2D3, predominantly in the jejunum and ileum[83]. It has been found that 1,25(OH)2D3 significantly enhanced Cldn- 2 and Cldn-12 mRNA levels in colon cancer Caco-2 cells. The mRNA and protein levels for these proteins were lower at 12 wk in the jejunum of VDR KO mice in comparison with wild-type mice, and siRNA against these Cldns diminished Ca2+ permeability in Caco-2 cells[84]. Cadherin-17 and aquaporin-8 have been reported to be downregulated by 1,25(OH)2D3 in the intestine[85,86]. Cadherin-17 is involved in cell-to-cell contact, and its decrease might in turn increase intestinal permeability. A decrease in channel aquaporin-8 might influence TJ selectivity towards cations. The data indicate that Ca2+ movement through TJ is regulated and supports the regulation of the paracellular Ca2+ transport route by 1,25(OH)2D3[31].

Evidence for the regulation of Ca2+ absorption by other hormones

PTH acts indirectly on intestinal Ca2+ absorption by the stimulation of renal CYP27B1 and, therefore, increases 1,25(OH)2D3-dependent Ca2+ absorption. A direct effect of PTH on intestinal Ca2+ absorption has not been demonstrated, but some direct effects of PTH on Ca2+ uptake by enterocytes from rat duodenum were reported. PTH/PTHrP receptors have been localized in intestinal epithelial cells along the villus[87]. It has been suggested that an in vivo model would need to be generated with targeted deletion of intestinal PTH receptor 1 in order to test if PTH directly affects intestinal Ca2+ absorption[88].

With regard to thyroid hormones, it has been reported that they produce a cooperative effect with vitamin D for intestinal Ca2+ transport. Apparently, thyroid hormones increase the genomic action of 1,25(OH)2D3 in the intestine[89]. Kumar et al[90] demonstrated that hyperthyroid rats show higher Ca2+ uptake and Ca2+ efflux from enterocytes than hypothyroid rats. They have also observed that NCX1 activity was highly increased by thyroid hormones, presumably via the cAMP-mediated pathway. Orihuela[91] has analyzed the effect of different statuses of thyroid hormones on the inhibitory effect of aluminum (Al) on intestinal Ca2+ absorption by using a rodent model. Mucosa-to-serosa Ca2+ fluxes in Al-exposed rats declined as thyroid hormones levels increased, thereby showing a trend opposite to that seen in non-Al-treated control rats.

Growth hormone (GH) has a major role in linear bone growth and bone Ca2+ deposition during childhood and adolescence. GH has proliferative effects upon the intestinal epithelium[92], and can also stimulate intestinal Ca2+ absorption, which would occur indirectly by increasing serum 1,25(OH)2D3 concentration[93].

However, it has also been shown that GH treatment increases intestinal Ca2+ absorption and duodenal CB9k levels in aged rats without increasing serum 1,25(OH)2D3 levels[94]. In adult men, Ca2+ absorption has been shown to be positively correlated with IGF-1, and age-related declines in IGF-1 have a negative impact on Ca2+ absorption that could not be explained by a decrease in serum 1,25(OH)2D3[95].

Most estrogen studies related to intestinal Ca2+ absorption were performed in ovariectomized (OVX) animals. This ablation significantly decreases endogenous estrogen, but not totally, since adrenal androgens can be aromatized to estrogen[96]. An estradiol replacement in OVX rats has been reported to increase intestinal Ca2+ absorption without stimulation of circulating 1,25(OH)2D3 levels[97]. van Abel et al[98] found increased duodenal gene expression of TRPV5, TRPV6, CB9k, and PMCA1b in OVX rats treated with estradiol. They used Cyp27b1 KO mice to analyze the calcitriol dependency of the stimulatory effects of estradiol on intestinal Ca2+ absorption, and found that estradiol treatment increased mRNA levels of duodenal TRPV6. Cell culture studies suggest that estrogen corrects the decline in the efficiency of intestinal Ca2+ absorption at the onset of menopause[99], but the mechanisms that underlie this effect remain unknown. Estrogen receptor alpha (ERα) KO mice showed a decrease in duodenal TRPV6 mRNA expression, while CB9k, PMCA1b, and VDR levels were not modified. Therefore, it seems that the genomic effects of estrogen on mice are mainly mediated by ERα[100]. In addition to estrogen, prolactin, a hormone that is elevated during pregnancy and lactation, has been shown to stimulate active intestinal Ca2+ transport in vitamin D deficient rats[101]. A direct effect of prolactin on active duodenal Ca2+ transport was shown[102]. Some data indicate that prolactin can regulate intestinal TRPV6 and cooperate with 1,25(OH)2D3 in regulating TRPV6 and CB9k. Prolactin also has a direct effect on the transcription of the Cyp27b1 gene, thus enhancing CYP27B1 protein expression and increasing levels of 1,25(OH)2D3 during lactation when there is an increased Ca2+ requirement for the neonate[103]. It has been suggested that prolactin also has an effect on the paracellular pathway of intestinal Ca2+ absorption through an upregulation of Cldn 15[104]. Some authors indicate that there is enough evidence that prolactin could be considered the cardinal calciotropic hormone in pregnancy and lactation[105].

Although reduced intestinal Ca2+ absorption seems to be part of the pathogenesis of glucocorticoid-induced osteoporosis[106], the mechanisms triggered by GCs in the intestine remain unclear. Short-term GC treatment in young animals does not alter the expression of genes involved in intestinal Ca2+ absorption, such as TRPV6, CB9k and PMCA1b[107], but sustained dexamethasone suppresses mouse duodenal CB9k expression[108]. Kim et al[109] found that gene regulation in the intestine by dexamethasone is complex in mice. It provokes an increase of duodenal TRPV6, CB9k, and PMCA1b 24 h after administration, which was followed by a decrease in a 5-d treatment. Ten days of prednisolone treatment decreases rat intestinal Ca2+ absorption through a diminished expression of the active Ca2+ transporters, which is independent of 1,25(OH)2D3[110] (Figure 2).

Figure 2
Figure 2 Hormonal regulation of intestinal calcium absorption. CB: Calbindin; Cldn: Claudin; GC: Glucocorticoids; GH: Growth hormone; IGF1: Insulin-like growth factor 1; NCX1: Intestinal Na+/Ca2+ exchanger; PI3K: Phosphoinositide 3-kinase C; PKC: Protein kinase C; PMCA1b: Plasma membrane Ca2+- ATPase 1b; PRL: Prolactin; PTH: Parathyroid hormone; ROCK: RhoA-associated coiled-coil-forming kinase; TH: Thyroid hormones; TRPV6: Transient receptor potential vanilloid 6.
Intestinal calcium absorption under different physiological conditions

Intestinal Ca2+ absorption changes according to the physiological conditions of individuals. When needs are high and/or dietary Ca2+ is low, intestinal Ca2+ absorption becomes more efficient. Growth, pregnancy, lactation, dietary Ca2+ deficiency, and high physical activity enhance the Ca2+ demands that promote intestinal Ca2+ absorption. During pregnancy, Ca2+ absorption is higher than before conception or after delivery. The enhancement occurs in early-to-mid pregnancy, and precedes the increased Ca2+ demand from the fetus for skeletal growth. This alteration in Ca2+ absorption during pregnancy may be due to increased serum calcitriol, with little alteration in serum PTH or calcitonin[111].

The maternal adaptation for the enhancement of intestinal Ca2+ absorption in pregnancy and lactation is very important for fetal development and lactogenesis. Intestinal Ca2+ absorption in pregnant adolescents has been shown to be higher in the third trimester of pregnancy than in the early postpartum period[112].

Vitamin D seems to play an important role during pregnancy. Yamagishi et al[113] found in pregnant rats that vitamin D deficiency produces severe hypocalcemia due to reduced intestinal Ca2+ absorption and elevated fetal demand for cation. It has been shown in mice that serum calcitriol was enhanced five-fold during pregnancy, whereas vitamin D binding protein levels were unchanged. A 30-fold higher expression of Cyp27b1 in maternal kidneys vs placenta suggests that the increase in calcitriol comes from the kidneys. Apparently, PTH is not required to upregulate Cyp27b1 expression during pregnancy[114]. A custom-designed cDNA microarray validated by quantitative real time PCR has found in rats that several duodenal transporters, such as TRPV6, are upregulated during pregnancy[115]. In addition, when the plasma estradiol levels are increased in pregnancy, intestinal CB9k gene expression is concomitantly enhanced, which suggests that the CB9k gene is involved in the compensatory induction of other Ca2+ transporter genes in duodenal epithelial cells[116]. Zhu et al[117] have found that both PMCA1 and CB mRNA levels were increased 2- to 3-fold in rats at 21 d of gestation. These levels of PMCA1 and CB mRNA remained elevated at 7 d of lactation.

Recently, in an animal model of preeclampsia, disturbance of Ca2+ metabolism in the placenta, intestine, and kidney has been observed. A decrease in Ca2+ transporting genes (TRPV5, TPRV6, PMCA1, and CB9k) has been detected in all these organs. In the duodenum, there was a slight recovery after calcium supplementation, whereas, in the kidney, these alterations were reverted to the control levels by the supplements[118].

The mechanisms by which intestinal Ca2+ absorption is induced in lactation are not quite clear. One possible adaptive mechanism includes hypertrophy and hyperplasia of the intestinal villi, as shown in lactating mammals such as rodents, pigs, and sheep[119,120]. Wongdee et al[121] have also demonstrated that intestinal hypertrophy in lactating rats is associated with an upregulation of Cldn 15 protein expression. It has been shown in rats that the suckling-induced transient prolactin surge increases intestinal Ca2+ transport during lactation, an effect that occurs through signaling pathways involving phosphoinositide 3-kinase C (PI3K), as well as two serine/threonine kinases, such as protein kinase C (PKC) and RhoA-associated coiled-coil-forming kinase (ROCK)[122].

In newborn rats, intestinal Ca2+ absorption is largely passive non-saturable, and not dependent on calcitriol[123]. This lack of responsiveness to calcitriol at earlier stages is explained by the undetectable levels of VDR within enterocytes at 7 and 14 d after birth[69]. Human data indicate that, in neonates, intestinal absorption is initially a passive process, which is favored by milk lactose. Later, it becomes a calcitriol dependent active process, but the hormone’s role can be bypassed by high dietary Ca2+ content or parenteral Ca2+ administration[124].

Ca2+ supplied in human milk during infancy is primarily derived from maternal bone, which is rapidly replenished during and after weaning[125]. The optimization of Ca2+ intake is crucial in adolescents to maximize calcium retention, acquire a good peak of bone mass, and prevent osteoporosis later in life. At early puberty, there is an association between an increase in both Ca2+ absorption and bone Ca2+ deposition. In girls, bone Ca2+ deposition reaches a maximum shortly before menarche, with the deposition rate being approximately five times that of adulthood. After menarche, bone Ca2+ deposition, as well as intestinal Ca2+ absorption, gradually declines[125]. In boys aged 11-14 years on their usual diets, it has been shown that adolescents absorbed 31% of their dietary Ca2+ intake and retained 20% of their total Ca2+ intake, but their dietary Ca2+ intake failed to meet recommended values[126]. During puberty, polymorphisms of the Fok I site in the VDR gene have been significantly associated with Ca2+ absorption and bone mineral density[127].

Aging has been associated with lower intestinal Ca2+ absorption[128], with an additional decrease at the time of menopause that is reversible with estrogen therapy[129]. This decrease might occur by a declination in serum calcitriol levels and a resistance to the actions of calcitriol in the intestine[130]. It has been reported that low levels of VDR in mouse heterozygotes for the VDR gene KO produce a resistance of intestinal Ca2+ absorption to 1,25(OH)2D3. This resistance seems to be generated by the low translation of CB9k, which is mediated by binding VDR with the ligand[131]. A post hoc analysis of dual isotope studies in post-menopausal women has identified associations of several factors with intestinal Ca2+ absorption. The data indicate that age, 1,25(OH)2D3, and dietary calcium and fat are associated with Ca2+ absorption, whereas serum 25(OH)D levels are not. The authors claim that this study has unique findings, as the dietary intake of kilocalories, carbohydrates, and potassium are also associated with intestinal Ca2+ absorption, suggesting that beyond the traditional focus on Ca2+ and vitamin D, some other factors also influence intestinal Ca2+ absorption in post-menopausal women[129].

Concluding remarks

Since Ca2+ ions are involved in most physiological processes, it becomes important to know the molecular details of intestinal absorption of cation, as the intestine is the only entrance for Ca2+ to the organism. Absorption occurs through two different pathways, transcellular and paracellular, which apparently interact with each other depending on physiological conditions. Calcitriol [1,25(OH)2D3] is the major regulating hormone, which clearly operates through VDR signaling, but the exact mechanism by which Ca2+ moves from the lumen to the serosa remains elusive. The role of other hormones, such as PTH, GC, GH, estrogens, thyroid hormones, and prolactin, is under investigation due to controversial data. Some of them act indirectly through the regulation of renal 1,25(OH)2D3 production, others by direct action, and still others by both methods. Different physiological conditions, such as growth, pregnancy, lactation, and aging, significantly alter intestinal Ca2+ absorption, according to Ca2+ requirements. Further research should be carried out to improve the current knowledge concerning the regulation of intestinal Ca2+ absorption in order to develop nutritional or medical strategies to optimize the efficiency of intestinal Ca2+ absorption and prevent osteoporosis and other pathologies related to Ca2+ metabolism.

Footnotes

P- Reviewer: Caviglia RD, Daniel F, Serafino A, Tovo CT, Wang DS S- Editor: Qi Y L- Editor: Rutherford A E- Editor: Liu XM

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