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Nutrient Physiology, Metabolism, and Nutrient-Nutrient Interactions

Chronic Vitamin A Status and Acute Repletion with Retinyl Palmitate Are Determinants of the Distribution and Catabolism of all-trans-Retinoic Acid in Rats¹

Department of Nutritional Sciences, The Pennsylvania State University, University Park, PA 16802

^* To whom correspondence should be addressed. E-mail: acr6{at}psu.edu.

	ABSTRACT

TOP ABSTRACT Introduction Materials and Methods Results Discussion LITERATURE CITED

 
The relation between vitamin A (VA) nutritional status and the metabolism of all-trans-retinoic acid (RA) is not well understood. In this study, we determined the tissue distribution and metabolism of a test dose of [³H]-RA in rats with graded, diet-dependent, differences in VA status. The design included 3 groups, designated VA-deficient, VA-marginal, and VA-adequate, with liver total retinol concentrations of 9.7, 35.7 and 359 nmol/g, respectively, (P < 0.05), and an additional group of VA-deficient rats treated with a single oral dose of retinyl palmitate (RP) 20 h before the injection of [³H]-RA. Plasma, liver, lung, and small intestines, collected 30 min after [³H]-RA, were analyzed for total ³H, unmetabolized [³H]-RA, polar organic-phase metabolites of [³H]-RA, and aqueous phase [³H]-labeled metabolites. In all groups, [³H]-RA was rapidly removed from plasma and concentrated in the liver. VA deficiency did not prevent the oxidative metabolism of RA. Nevertheless, the quantity of [³H]-RA metabolites in plasma and the ratio of total [³H]-polar metabolites to unmetabolized [³H]-RA in liver varied directly with VA status (VA-adequate > VA-marginal > VA-deficient, P < 0.05). Moreover, supplementation of VA-deficient rats with RP reduced the metabolism of [³H]-RA, similar to that in VA-adequate or VA-marginal rats. Liver retinol concentration, considered a proxy for VA status, was correlated (P < 0.05) with [³H]-RA metabolites in liver (R² = 0.54), plasma (R² = 0.44), lung (R² = 0.40), intestine (R² = 0.62), and all combined (R² = 0.655). Overall, the results demonstrate close linkage between dietary VA intake, hepatic storage of VA, and the degradation of RA and suggest that measuring plasma retinoid metabolites after a dose of RA may provide insight into the metabolism of this bioactive retinoid by visceral organs.

	Introduction

TOP ABSTRACT Introduction Materials and Methods Results Discussion LITERATURE CITED

When VA is consumed in excess of requirements it is stored as retinyl esters, primarily in the liver, from which it can be mobilized, distributed to extrahepatic tissues (4), and used as a substrate for the production of oxidative metabolites (Fig. 1) (5). Investigations of retinol kinetics have established that retinol turnover and utilization is directly affected by VA intake and, consequently, by VA status (6,7). Retinol utilization was decreased to 10% of control in rats with low VA stores than in their VA-sufficient counterparts (7). Kinetic analysis also revealed that the uptake, utilization, and storage of retinol by specific tissues in rats were directly influenced by VA status (8–10). These results suggest that VA status is a determinant of the distribution and utilization of retinol during VA supplementation. Furthermore, these studies suggest that VA status may affect the kinetics of other retinoids, such as RA, in a similar manner; however, the relation between VA status and the distribution and metabolism of RA has yet to be fully delineated.

View larger version (6K): [in this window] [in a new window]   Figure 1  Model of retinoid metabolism. RE, retinyl ester; ROH, retinol; RAL, retinal; RA, retinoic acid; 4-OH-RA, 4-hydroxy-retinoic acid; 4-oxo-RA, 4-oxo-retinoic acid.

	Materials and Methods

TOP ABSTRACT Introduction Materials and Methods Results Discussion LITERATURE CITED

 
    Animals and diets. All procedures for animal care and use were approved by the IACUC of The Pennsylvania State University. Female Sprague-Dawley rats with litters of 12 female pups (purchased from Charles River Laboratories) were fed a VA-deficient diet from the time of arrival to reduce the accumulation of VA from milk by nursing pups (23). The rats were housed in a room maintained at 22°C with a 12-h dark:light cycle, and food and water were consumed ad libitum. When the rat pups were 21 d old, they were weaned in pairs and fed a nutritionally complete AIN-93G diet (24), modified to contain either no VA (VA-deficient; n = 15), 0.412 mg (VA-marginal; n = 6), or 7.43 mg (VA adequate; n = 9) of RP per kilogram of diet (Research Diets). Twenty hours prior to the experiment, 6 VA-deficient rats were given an oral dose of 1.67 µmol of RP prepared in 25–30 µL of canola oil (VA-deficient+RP; n = 6). Finally, 3 VA-adequate rats were pair fed to 3 VA-deficient rats for 14 d to ensure that any VA-deficiency-related anorexia did not affect the results.

    Experimental design. When the rats were between 60 and 66 d of age, they were individually anesthetized by isoflurane-oxygen inhalation and 0.15 mL/100 g body weight (BW) of albumin-bound [³H]-RA, prepared as described below, was injected into the exposed left common iliac vein (25). The incision was closed with a sterile surgical staple and the rats were allowed to recover from the anesthesia. Rats were killed 30 min postinjection by carbon dioxide asphyxiation. Blood was drawn from the vena cava into heparinized syringes and the liver, lung, spleen, and small intestine were quickly removed, weighed, and aliquots frozen in liquid nitrogen for storage at –80°C before subsequent analysis. Because RA is rapidly metabolized, it is important to collect tissues quickly (26,27); thus, each rat was treated on a defined schedule so that all tissues could be collected and frozen within 5 min or less after killing. The 30 min time chosen for this experiment was based upon previous reports (28), and pilot work (data not shown) that showed that >95% of the [³H]-RA dose was cleared from plasma within 10 min and that metabolism of [³H]-RA to polar metabolites could be readily detected by 30 min.

    Dose preparation. All procedures involving retinoids were carried out in either dim or yellow light. The doses of [³H]-RA for i.v. injection were prepared fresh immediately prior to injection, similar to doses previously described (25). In brief, for each 1-mL aliquot, 10 µCi of [³H]-RA ([11,12(n)-³H]retinoic acid, specific activity 37.0 Ci/mmol, from PerkinElmer]) was combined with 0.23 µmol of oleic acid, added as a lipid carrier because no nonradioactive RA was added, followed by 5 µL of Tween 20 (Sigma-Aldrich), 0.9 mL of 0.1% rat serum albumin (Calbiochem), diluted in sterile PBS, and 0.10 mL of whole rat plasma. The final concentration of RA in the dose was 0.023 µmol/L, and the dose delivered to each rat was standardized at 0.15 mL (33 pmol RA)/100 g BW. This resulted in a minimally perturbing dose of RA, estimated to transiently elevate plasma RA by 3.7 µg RA (0.012 µmol)/L plasma. Following the preparation and administration of each dose, aliquots were analyzed by HPLC (29), which showed >97% [³H]-RA (data not shown).

    Determination of tissue radioactivity. Aliquots of 0.5 mL of individual plasma, or 0.5 g of liver, lung, and small intestine samples were extracted using a modification of the method of Folch et al. (30,31), as described previously (25). The procedure resulted in a washed organic phase and an aqueous phase (25). Aliquots of the injected dose, along with the organic and aqueous phases from each tissue, were analyzed by liquid scintillation spectrometry (25).

    Separation of RA from polar organic metabolites (4-oxo- and 4-hydroxy-retinoic acid). Reverse-phase solid phase extraction was employed to separate the parent compound, [³H]-RA, from its oxidation products, mainly [³H]-4-oxo- and 4-hydroxy-RA (32,33) in the organic phase of the liver extracts, as described previously (25). Briefly, 300 µL (50 mg tissue) of Folch-washed organic phase along with all-trans-RA and 4-oxo-RA standards were dried to completeness under argon and reconstituted in 1.25 mL of HPLC-grade acetonitrile:water (65:35, vol:vol) containing 10 mmol/L of acetic acid. Following column conditioning, the samples were loaded onto the column and the polar metabolites were eluted first in 3 x 4 mL of acetonitrile:water (65:35, vol:vol), while all-trans-RA was eluted with 3 x 4 mL of acetonitrile:water (80:20, vol:vol) (25). The elution rate was maintained at 1 mL/min with negative pressure, using an elution vacuum apparatus (Supelco). After collection, the samples were dried to completeness and analyzed by liquid scintillation spectrometry as described previously (25).

    Retinol assay. Plasma and liver total retinol were measured in aliquots of plasma or the organic extract of liver. Plasma and liver samples were pooled prior to retinol analysis, such that each retinol concentration data point presented represents either 2 (VA-marginal and RP groups) or 3 (VA-deficient and VA-adequate groups) rats. Pooled samples were saponified and total retinol was quantified by HPLC with UV detection. Trimethylmethoxyphenyl-retinol was used as internal standard (34).

    Real time PCR. Total RNA was extracted from the same pooled liver samples that were used for retinol assays, using TRIzol Reagent (Invitrogen), and quantified by UV spectrophotometry. CYP26A1 mRNA levels were quantitatively assessed by RT-PCR in Penn State's Nucleic Acid Facility using an ABI 7700 (Perkin-Elmer) cycler system. The endogenous 18S RNA transcript was used as the internal control. Briefly, the PCR mixture was assembled using the TaqMan PCR core reagent kit along 10 µmol/L CYP26 forward primer (5'-AGTGATGGGCGCGGATAAT-3') and 10 µmol/L CYP26 reverse primer (5'-TGCACTGACACCAACCGGT-3') The PCR cycling program was run for 1 cycle of 50°C for 2 min, 95°C for 10 min, followed by 40 cycles of 95°C for 15 s, 60°C for 1 min, and then 1 cycle of 25°C for 2 min. RNA samples were assayed in duplicate. For comparison between runs and with previous experiments, a sample of a pool of control rat liver RNA, C-1, and a sample of a pool of RA-induced rat liver RNA, C-2, were run with each set of samples. The results are expressed relative to C-1, equal to 1 before log transformation and 0 after log₁₀ transformation. The data obtained from the RT-PCR were log₁₀ transformed prior to statistical analysis.

    Statistics. All results are expressed as means ± SEM. One-way ANOVA (SuperANOVA, Abacus Concepts) was used to test for the effect of dietary VA level on [³H]-RA metabolism. When warranted, data were then tested by Fisher's Protected LSD test to determine which groups differed significantly (P < 0.05). Simple regression was performed on pooled group data with P < 0.05 considered significant. When necessary, data were log₁₀ transformed prior to analysis.

	Results

TOP ABSTRACT Introduction Materials and Methods Results Discussion LITERATURE CITED

 
    VA status affects plasma and liver retinol concentrations and hepatic CYP26A1 mRNA expression. All rats appeared in good health. No signs of anorexia developed and, at the time of testing, the VA-deficient group did not differ in body weight from the VA-adequate group, nor did the pair-fed VA-adequate rats differ from non-pair-fed VA-adequate rats (Table 1). However, the relative weight of the liver was significantly lower in the VA-deficient and VA-deficient+RP rats than in VA-adequate and VA-marginal rats. In contrast, the relative weight of the lung was slightly but significantly higher in the VA-deficient rats than in the VA-adequate and VA-marginal rats (Table 1). There was no difference due to VA status in the relative weight of the small intestine.

Hepatic CYP26A1 mRNA expression was measured, as previous work has shown that its level differs in a sensitive manner with VA status (35). CYP26A1 was significantly lower (P < 0.001) in the VA-deficient group compared with the other groups by ANOVA (Table 1). Although the VA-marginal, VA-deficient+RP, and VA-adequate groups did not differ significantly, this may have been an artifact of ANOVA, as the mean CYP26 mRNA expression in the VA-adequate group was 6.5 and 5 times those in the VA-marginal and VA-deficient+RP groups, respectively, and all groups differed significantly when analyzed by unpaired t test (P < 0.05).

    VA deficiency increases total ³H radioactivity from [³H]-RA in plasma but decreases the proportion of [³H]-aqueous phase metabolites. In all groups, >96% of the injected dose was eliminated from plasma within 30 min (Fig. 2). However, total [³H]-retinoids in plasma were higher in VA-deficient rats. VA status affected both [³H]-aqueous and [³H]-organic phase metabolites of RA (P < 0.005). [³H]-Aqueous phase metabolites increased as a function of VA-status (VA-adequate > VA-marginal > VA-deficient; Fig. 2). Conversely, the amount of organic phase [³H]-labeled compounds recovered in the plasma of VA-deficient rats was greater than in the other groups (P < 0.01, Fig. 2). The amount of aqueous and organic phase ³H in the plasma of VA-deficient+RP rats was similar to the amount in VA-marginal and VA-adequate rats, but [³H]-aqueous phase metabolites in the plasma of VA-deficient+RP rats were 150% of VA-deficient rats (P < 0.05). Thus, VA status and acute retinol repletion were determinants of both the total amount of ³H and the amount of aqueous phase ³H recovered in plasma 30 min after injection of [³H]-RA.

View larger version (18K): [in this window] [in a new window]   Figure 2  Total radioactivity and [3H]-aqueous phase metabolites in plasma of female Sprague-Dawley rats fed diets with different amounts of VA. Plasma was collected 30 min after injection of [3H]-RA (33 pmol RA mass) and 3H in organic-phase and aqueous-phase extracts was determined. Values are means ± SEM, n = 9 for VA-deficient (VAD) and VA-adequate (VAS) and n = 6 for VA-marginal (VAM) and VA-deficient+RP (VAD+RP) groups. Different letters above bars within panels indicate significant differences, P < 0.05.

View larger version (22K): [in this window] [in a new window]   Figure 3  Total radioactivity (A) and total [3H]-metabolites (B) in liver of female rats fed different amounts of VA 30 min after injection of [3H]-RA. Liver was collected 30 min after injection of [3H]-RA (33 pmol RA mass) and 3H in organic-phase and aqueous-phase extracts was determined (A). Reverse-phase solid phase extraction (SPE) was employed to separate the parent compound [3H]-RA from 3H-labeled in the organic phase of the liver extracts (B). Values are means ± SEM, n = 9 for VA-deficient (VAD) and VA-adequate (VAS) and n = 6 for VA-marginal (VAM) and VA-deficient+RP (VAD+RP) groups. Different letters above bars within panels indicate significant differences, P < 0.05.

    RA metabolism and distribution in extrahepatic tissues is affected by VA status. Less than 0.75% of the injected dose of [³H]-RA was recovered in the lungs of VA-adequate rats (Fig. 4). Total ³H was lower in the lungs of VA-deficient rats than in VA-adequate rats (P < 0.05), but was not different from the VA-marginal rats. VA status affected (P < 0.001) [³H]-aqueous phase metabolites in lung, which increased as a function of VA status (VA-adequate > VA-marginal > VA-deficient; Fig. 4). Aqueous phase ³H was greater in the lung of VA-deficient+RP rats than in VA-deficient, VA-marginal, and VA-adequate rats (P < 0.05), whereas organic phase ³H in the VA-deficient+RP group was similar to that in VA-marginal and VA-adequate rats, but different from VA-deficient rats (P < 0.05, Fig. 4). Thus, unlike the other tissues examined, the lungs of the VA-deficient+RP rats contained 25% more [³H]-aqueous phase metabolites than the VA-adequate rats.

View larger version (20K): [in this window] [in a new window]   Figure 4  Total radioactivity and [3H]-aqueous phase metabolites present in lung of female rats fed different amounts of VA. Values are means ± SEM, n = 9 for VA-deficient (VAD) and VA-adequate (VAS) and n = 6 for VA-marginal (VAM) and VA-deficient+RP (VAD+RP) groups. Different letters above bars within panels indicate significant differences, P < 0.05.

View larger version (18K): [in this window] [in a new window]   Figure 5  Total radioactivity and [3H]-aqueous phase metabolites present in small intestine of female rats fed different amounts of VA. Values are means ± SEM, n = 9 for VA-deficient (VAD) and VA-adequate (VAS) and n = 6 for VA-marginal (VAM) and VA-deficient+RP (VAD+RP) groups. Different letters above bars within panels indicate significant differences, P < 0.05.

View larger version (17K): [in this window] [in a new window]   Figure 6  Regression analysis of [3H]-metabolites of RA in liver (A), lung (B), small intestine (C), and plasma (D) vs. liver total retinol of female rats fed different amounts of VA after the administration of [3H]-RA. Each point represents 2 (VA-marginal and VA-deficient+RP) or 3 (VA-deficient and VA-adequate) rats per treatment group. For lung, 2 separate analyses were performed.

	Discussion

TOP ABSTRACT Introduction Materials and Methods Results Discussion LITERATURE CITED

The liver, lung, and small intestine are intimately involved in retinol and RA homeostasis (41–43). Therefore, we examined each organ for aqueous and organic-phase radioactivity to determine whether VA status affects RA metabolism. The amounts of VA provided in the diets used in our study were selected to create a wide range of hepatic VA stores (44–46), as in previous studies, and resulted in an 35-fold range of total retinol concentrations, from <10 nmol/g in the VA-deficient group to >375 nmol/g in the VA-adequate group (Table 1). The amount of aqueous-phase radioactivity recovered in the liver, lung, and small intestine was lowest in the VA-deficient rats and highest in the VA-adequate rats. Similarly, the ratio of total [³H]-labeled polar metabolites to [³H]-RA in the liver, lung, and small intestine was highest in VA-adequate rats and lowest in VA-deficient rats, indicating that VA-adequate rats catabolized more RA than VA-deficient rats. Moreover, RA metabolism increased in the liver, lung, and small intestine in proportion to hepatic retinol concentrations, indicating that VA stores are a major determinant of RA metabolism in all tissues examined (Fig. 6). Thus, these results suggest that the uptake, recycling, and metabolism of RA by the liver, lung, and small intestine are dependent upon VA stores and that each organ is involved in the regulation of RA homeostasis.

In contrast to the lung and small intestine, the livers of VA-marginal and VA-deficient rats contained 30 and 130% more of the injected dose, respectively, than the VA-adequate rats, suggesting that uptake and/or retention of RA in the liver is greater as VA status declines, which is consistent with greater conservation of RA. Conversely, VA status may be inversely related to the recycling of RA from liver to plasma. On the basis of these results, we speculate that 2 related processes could be working in concert to cause the observed increase in liver radioactivity and decrease in the metabolism of RA in VA-deficient rats and, to a lesser extent, in VA-marginal rats. First, previous work has shown that the ratio of apo- to holo-cellular retinol binding protein (CRBP) affects retinol metabolism (47–50), for as the ratio of apo-CRBP to holo-CRBP increases, retinol storage is inhibited, while retinyl ester hydrolysis is increased. If the converse is true, retinol storage will increase while retinyl ester mobilization will decrease (49,50). Our results for RA metabolism suggest there may be a regulatory mechanism parallel to that for retinol. Specifically, in the case of VA-deficient rats, we hypothesize that the ratio of apo-cellular retinoic acid binding protein (CRABP) to holo-CRABP is high, resulting in a decrease in hepatic RA metabolism and secretion/recycling into plasma, while increasing the residence time of RA in liver. If, in contrast, the ratio of apo-CRABP to holo-CRABP is lower in VA-adequate rats than VA-marginal or VA-deficient rats, both RA metabolism and the excretion of polar and aqueous-phase RA metabolites into bile may be increased (26,40,51). Second, the expression of CYP26A1, an RA-inducible enzyme that catalyzes the oxidation of RA (46,52,53), is directly related to chronic VA intake and VA status, assessed as liver retinol concentration (35). In our studies, CYP26A1 mRNA was highest in the liver of VA-adequate rats and decreased as VA status (liver retinol) declined (Table 1) and CYP26A1 mRNA expression was directly correlated with increased metabolism (Table 2). Additionally, studies in F9 teratocarcinoma cells showed that CRABP expression and RA metabolism are correlated (54). Thus, changes in the ratio of apo- to holo-CRABP, as demonstrated in F9 cells, and differences in the level of expression of CYP26A1 due to VA status, may contribute importantly to the regulation of hepatic RA metabolism in intact rats, which in turn may maintain normal cellular and whole-body levels of RA.

VA supplementation is now used extensively in developing countries to prevent nutritional VA deficiency, which is associated with diminished disease resistance (55), prolonged infection (56), and increased mortality (57,58). Although VA supplementation is known to increase plasma retinol if liver VA stores have been depleted and to increase the storage of VA in the liver and extrahepatic tissues in proportion to the oral dose (59), it is unknown whether the metabolism of RA is affected, either acutely or over a long term, by VA supplementation. To determine whether VA supplementation affects the distribution and metabolism of RA acutely, we compared VA-deficient rats to VA-deficient+RP rats given a single oral dose of RP 20 h before the test dose of [³H]-RA. In the plasma and organs examined we observed 2 distinct trends with regards to RA homeostasis. First, the total amount of radioactivity, both unmetabolized and metabolized, that was recovered in the plasma, liver, lung, and small intestine of the VA-deficient+RP rats was similar to that recovered from VA-adequate rats. This suggests that VA supplementation results very quickly in the resetting of the homeostatic mechanisms that control RA metabolism. Secondly, the amount of [³H]-metabolites of RA recovered from tissues was significantly greater in VA-deficient+RP rats than in VA-deficient rats. Moreover, [³H]-metabolites were nearly identical in VA-deficient+RP rats and VA-marginal rats, except in the lungs, where aqueous phase metabolites were greater in the VA-deficient+RP rats than in VA-marginal rats. We speculate that the decrease in total radioactivity and the increase in RA metabolism in VA-deficient+RP rats was caused by the rapid increase in hepatic VA following supplementation (Table 1), which could have resulted in a substantial increase in the production of RA from retinol. Thus, providing an acute retinol supplement to VA-deficient rats restored plasma retinol concentrations to normal, and increased hepatic stores of VA, but the metabolism of RA was still compromised, suggesting that a complete restoration of VA homeostasis was not achieved within the 20 h following supplementation with RP.

In conclusion, the results of this study demonstrate that VA status affects both the organ distribution and metabolism of RA in rats, and suggest that the uptake, recycling, and utilization of RA are altered in a tissue-specific manner in response to decreasing stores of VA. Furthermore, the administration of RP to VA-deficient rats resulted, in a 20-h interval, in increased hepatic retinol and a pattern of [³H]-RA metabolism similar to that in VA-adequate rats. To our knowledge, this is the first study to show that both the distribution and metabolism of RA are directly affected by VA status and retinol repletion. Our results on the regulated expression of CYP26A1 in liver concur with those of Yamamoto et al. (35) and, together, suggest that molecular mechanisms capable of controlling whole-body RA homeostasis respond sensitively, both to chronic differences and acute changes in VA intake, to maintain normal physiological concentrations of RA. Although our study focused mainly on the metabolism of RA in the liver, it is interesting that difference in plasma [³H]-RA metabolites could be detected as a function both of VA status and retinol repletion. It may be possible that plasma retinoid metabolites would be useful as indicators of tissue retinoid metabolism. Previously, oxidized metabolites of retinol in plasma were correlated with VA status in lactating sows (60). We speculate that the measurement of plasma metabolites of RA following an acute RA dose could be used as a sensitive indicator of VA status in humans.

	ACKNOWLEDGMENTS

 
We are grateful to Dr. Nan-qian Li for retinol analysis and Dr. Deborah Grove for performing the real-time PCR analysis.

	FOOTNOTES

 
¹ Supported in part by NIH CA-90214, the Integrative Biosciences Graduate Program, and the Graduate Program in Nutrition.

² Abbreviations used: BW, body weight; CRABP cellular retinoic acid binding protein CRBP, cellular retinol binding protein; RA, retinoic acid; RP, retinyl palmitate; VA, vitamin A.

Manuscript received 7 September 2006. Initial review completed 3 October 2006. Revision accepted 18 October 2006.

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