Chapter 24
Comparative Intestinal Absorption and Subsequent Metabolism of Metal Amino Acid Chelates and Inorganic Metal Salts
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H. DeWayne Ashmead Albion Laboratories, Inc., 101 North Main Street, Clearfield, UT 84015
Intrinsic, extrinsic, and luminal conditions all influence mineral bioavailability resulting in different intestinal absorption rates and subsequent body metabolism for inorganic salts versus amino acid chelates. Those differences are demonstrated by in vitro comparisons of mucosal cell uptakes of minerals as amino acid chelates, SO , O , and CO . In perfusion studies the differences in rates of transfer of isotopes of chelates and metal salts from the mucosal to serosal solutions are examined. Finally, in vivo isotope studies are summarized which compare the tissue uptake of minerals from amino acid chelates and inorganic salts. These investigations, utilizing Fe, Zn, Mn, Ca, Mg, and Cu, demonstrate that intestinal absorption and subsequent metabolism of the above minerals is greater when they are ingested as amino acid chelates compared to inorganic salts of the same metals. 4
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In its most basic terms, nutrition is the intake of protein, carbohydrates, fats, vitamins, minerals, and water for growth and maintenance of body tissues, for energy, and to regulate all of the body processes. Health and well being are dependent upon the correct balance and intake of these nutrients. Minerals function in all of the nutrient roles. This necessitates having an optimum amount of the essential minerals to carry out their multitude of assigned functions. Optimum is the key to efficacy. Too much or too little of a mineral has an equally deteriorative effect. Deficiencies are generally of greater practical concern than excesses. The fact that a specific mineral is chemically present in food does not guarantee intestinal absorption. Numerous factors will enhance the bioavailability of a particular metal, while others will detract from its usage in the body as summarized in Table 1(1). 0097-6156/91/0445-0306$06.00/0 © 1991 American Chemical Society
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
24.
Metal Amino Acid Chelates and Inorganic Metal Salts
ASHMEAD
Table I. Factors Affecting Mineral Bioavailability
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Intrinsic factors: 1. 2. 3. 4. 5. 6. 7.
Animal species (including man) and its genetic makeup Age and sex Monogastric or ruminant (intestinal microflora) Physiological function: growth, maintenance, reproduction Environmental stress and general health Food habits and nutrition status Endogenous ligands to complex metals (chelates)
Extrinsic factors: 1. Mineral status of the soil on which the plants are grown 2. Transfer of minerals from soil to food supply 3. Bioavailability of mineral elements from food a. Chemical form of the mineral (inorganic salt or chelate) b. Solubility of the mineral complex c. Absorption on silicates, calcium phosphates, dietary fiber d. Electronic configuration of the element and competitive antagonism e. Coordination number f. Route of administration, oral or injection g. Presence of complexing agents such as chelates h. Theoretical (in vitro) and effective (in vivo) metal binding capacity of the chelate for the element under consideration i. Relative amounts of other mineral elements In the lumen: 1. Interactions with naturally occurring ligands a. Proteins, peptides, amino acids b. Carbohydrates c. Lipids d. Anionic molecules e. Other metals 2. Interactions at and across the intestinal membrane a. Competition with metal-transporting ligands b. Endogenously mediating ligands c. Release to the target cell
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
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A complete review of Table I is outside the scope of this chapter. This present discussion will examine the effect of the chemical form of the mineral on mineral bioavailability. Inorganic metal salts have different absorption levels than chelates^. Even among chelates, absorption rates will vary according to the ligand, stability constant of the chelate, molecular weight, etc. (5), so the field of chelates must be narrowed further to deal only with molecules resulting from the binding of a polyvalent cation to the alpha-amino and carboxyl moieties of an amino acid to form a five-membered ring. The structure of the ring consists of the metal atom, the active carboxyl oxygen atom, the carbonyl carbon atom, the alpha-carbon atom, and the alpha-nitrogen atom. The bonding is accomplished by both coordinate covalent and ionic bonding. At least two and sometimes three amino acids can be bound to a single metal ion, depending upon its oxidative state, to form bicyclic and/or tricyclic-ringed molecules as seen in Figure 1. Even though the oxidative states of certain cations would allow for a fourth amino acid to be chelated to the cation, the bonding angles and the atomic distances required for chelation would tend to preclude its occurrence. Several in vitro studies have shown intestinal uptake of amino acid chelates to be more rapid and in greater amounts than equivalent quantities of metal salts. Jejunal segments from adult male Sprague-Dawley albino rats beginning 10 cm below the pylorus and continuing for another 20 cm were removed, cut into 2 cm segments, and severed longitudinally along the mesenteric line. After randomization, washing, and incubation in Krebs-Ringer buffer solution, they were then exposed for 2 min to 50 μ% of Cu, Fe, Mg, or Zn as C 0 , 0 , or S0 or as amino acid chelates, all of which had been dissolved in simulated gastric solutions. Following exposure period, the segments were washed and assayed by atomic absorption spectrophotometry. The summarized results are shown in Table HQ). Clearly, under controlled conditions, the uptake of the amino acid chelates was significantly greater than any of the metal salts tested. 3
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Table II. Mean Jejunal Uptake of Different Mineral Forms (ppm)
Copper Magnesium Iron Zinc a
Chelate
so
35 94 298 191
8 36 78 84
4
co
Control
6 51 53 87
Trace 7 23 14
3
11 23 61 66
oxide
Differences in absorption rates can be demonstrated visually as well. Fasted experimental animals were fed Fe as C 0 or the amino acid chelate. Sections of their mucosal tissue were excised and examined by scanning electron microscopy. Figure 2a shows unabsorbed FeC0 on the microvilli whereas Figure 2b shows iron amino acid chelate being absorbed. The difference is 3
3
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
Figure 1. A two dimensional drawing of a tricyclic chelate of iron with glycine and methionine as amino acid ligands.
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Figure 2a. The absorption of Fe from F e C 0 on the microvilli. 3
Figure 2b. The absorption of Fe from Fe amino acid chelate on the microvilli.
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
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24.
ASHMEAD
Metal Amino Acid Chelates and Inorganic Metal Salts
dramatic. Fe absorption from the amino acid chelate is not only greater, but more rapid. For absorption of a mineral from a salt to occur, it must be presented to the mucosa as a cation. Numerous studies have demonstrated that, after ingestion, metal salts are generally ionized in the stomach, providing they are soluble. If no interfering chemical reactions occur, the cations enter the intestine where they are bonded to amino acids from the chyme or to the carrier proteins embedded in the luminal membranes of the mucosal cells and transported to the cytoplasm by passive diffusion or active transport. This absorption can occur anywhere in the small intestine, but generally takes place in the duodenum where the metal ions retain their solubility due to a lower pH(2). Conversely, the amino acid chelate is not ionized before absorption. It is not affected by different precipitating anions because the metal ion in the molecule is chemically inert due to the coordinate covalent and ionic bonding by the amino acid ligands. It is not affected by the acid p H of the stomach and survives as an intact molecule particularly after the chelate has been stabilized through a particular buffering process(f). Fats and fibers do not interfere with its absorption due to the high formation constant (or the low dissociation constant). A n d finally, the transport of the amino acid chelate across the mucosal cell does not require vitamin intervention as is the case with some metal ions. Instead, its absorption follows the pathway of a low molecular weight peptide. When an amino acid chelate is formed, it assumes many of the characteristics of a dipeptide or tripeptide. Due to their stabilities, the chemical structures of amino acid chelates are not altered throughout the digestive process. Therefore, as an amino acid chelate, the metal can easily travel through the intestine in the guise of a dipeptide-like or tripeptide-like molecule. The low molecular weight of this molecule (200 to 400 daltons) allows intact absorption into the mucosal cell without further luminal hydrolysis. Stability of amino acid chelates is of great concern to its absorption. When only one amino acid is used to chelate the metal ion, it may not form a chelate bond that is sufficiently strong to resist dissociation in the gut. Two chelating amino acids provide four bonds (three amino acids - 6 bonds) into a single metal atom. The combination of the bonds projecting out at tetrahedral angles (as in the case of the bicyclic species) and the steric hindrance of the chelating amino acid rings impede competing electrophilic molecules or atoms from disrupting the chelate bond. When only one amino acid chelates to a metal atom, the result is an open side where competitive electrophilic species may attack. Thus, two- and three-ringed amino acid chelates are more stable. The weaker single amino acid chelates, or amino acid complexes, can dissociate chemically in the stomach and intestines, thus freeing the metal ion to the chyme and allowing it to become susceptible to any of the various kinds of competing reactions which are adverse to absorption. A n amino acid chelate will also resist the action of the peptidases that break internal peptide bonds, due to the presence of the metal atom in the molecule as well as a result of a higher stability constant. As noted above, luminal changes in p H do not alter the amino acid chelate. Consequently, the amino acid chelate molecule can be absorbed intact through the intestinal mucosa, pulling the metal along with it. A s illustrated in Figure
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
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3, when the intact amino acid chelate is absorbed into the mucosal cells, it is believed that a coordinating link is formed through one of its amino acids with the gamma-glutamyl moiety of glutathione, a tripeptide found in the mucosal cell membrane. After the formation of the chelate-glutathione molecule, an enzymatic breakdown of this molecule would occur, resulting in the active transport of the amino acid chelate from the luminal side of the mucosa to the cytoplasm within the cell (2,). After traversing the mucosal cell membrane, the amino acid chelate is released at the terminal web due to a pH change which breaks the linkage of the transport molecule with the chelate. The amino acid chelate can then migrate across the mucosal cell to the basement membrane and from there directly into the plasma, as an intact molecule. No intracellular carrier is required. While a certain amount of cytoplasmic peptide hydrolysis can take place, intracellular hydrolysis of the amino acid chelates occurs less frequently than the hydrolysis of dipeptides without a metal, due to the steric hindrance of the ring structure inherent in the chelate molecule, as noted above, in connection with restrained luminal hydrolysis. The actual separation of the metal from its amino acid ligand molecules generally takes place at the sites of usage. Most metals function in the body as parts of amino acid chelates and complexes and as components in enzyme systems. When hydrolysis occurs, the coordinating bonds break, possibly due to enzymatic action together with site-specific pH changes that can lower the stability constants of the amino acid chelates, favoring the release of the cation to a cytoplasmic ligand with a higher stability constant. Previously cited work has demonstrated that mucosal uptake of the amino acid chelate is more rapid than that of metal salts. Perfusion studies have demonstrated that the transfer of the amino acid chelate to the serosa is also more rapid. In these experiments, rat small intestines were excised, washed, and everted in an oxygenated (95% 0 and 5% C0 ) buffer solution. Fifteencentimeter (15 cm) segments were cut, tied at the ends, and run in tandem in separate vessels at 37° C which contained 1 χ 10" ^Zn as ZnCl or as Zn amino acid chelate in the mucosal solution. Each hour, for a period of eight hours, intestines were removed, rinsed and digested prior to scintillation counting to determine absorbed radioactivity in the tissues. Each hour, for a period of five hours, samples of the serosal solution were removed and analyzed for ^ Z n transferred from the mucosa to the serosa. Figures 4a and b show the moles of Zn per gram of tissue in the duodenum and in the jejunum, while Figure 5 shows the quantity of ^Zn transferred to the serosal solution^. The transfer of Zn from the mucosa to the serosa in the form of an amino acid chelate is not only more rapid than Zn as ZnCl , but the quantity of Zn absorbed and transferred is significantly higher. When chelated to amino acids, approximately four times as much Zn was transported to the serosa leaving less in the intestinal tissues. When the mucosal cell is dependent upon a cytoplasmic generated carrier (metallothionein) to transport the Zn to the serosa, as in the case of ZnCl , the movement of the Zn appears hindered, or even blocked due to lack of carrier molecules. This results in higher concentrations of Zn from ZnCl in the mucosal cells but less in the serosal solution. 2
2
4
2
2
2
2
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
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24. A S H M E A D
LUMEN
Metal Amino Acid Chelates and Inorganic Metal Salts 313
AMINO ACID CHELATE.
ADP*PI
(glutathione) /
17-QLUTAMYL
TRAN8PEPTIDA8ËI 7Γ
ATP
- - - r r r ** f ***\^ HTH
T
glyolng
I \y*H-gly
MEMBRANE
T-glu-C>HE LATE ELATE irePTiBagg ΣΖΓ ^-GLUTAMYL CYCLOTRAN8FERA8E1 oyfoln* f^QLU-CVRH
6-oxv rollng
ADP
[VATP
fiVNTHETA8El
glutamw /
•OXÛfrftOLINÀÔË
CYTOPLA8M AMINO ACID CHELATE
ATP
^SDP^PI
Figure 3. The membrane transport of an amino acid chelate illustrating steps involved.
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
*'
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BIOLOGICAL TRACE ELEMENT RESEARCH
-e-ZnCI fô
2
-s-ZIno Amino Acid Chelate fô
Figure 4a. The transfer of Zn from ^ZnC^ and Zn amino acid chelate to the duodenum from mucosal solution.
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
ASHMEAD
Metal Amino Acid Chelates and Inorganic Metal Salts315
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24.
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
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BIOLOGICAL TRACE ELEMENT RESEARCH
Greater mucosal absorption and transfer of amino acid chelates results in greater body tissue levels of the minerals from those chelates. Several studies presented below illustrate this. In the first example, Sprague-Dawley albino male adult rats were fasted for 24 hours before being divided into two groups of eight animals each. While under light ether anesthesia each animal was given an intraperitoneal dose of 5.0 //g of ^Zn as an amino acid chelate or as ZnCl . Four hours after dosing, all of the animals were sacrificed and their tissues assayed for ^Zn with a gammaray spectrometer. Table III presents the amount of ^Zn found in the assayed tissues of the animals^. While the levels differed from tissue to tissue, the mean increase of Zn in the tissues was almost 19% when the amino acid chelate was ingested.
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2
Table III. Mean ^Zinc Levels in the Tissues (cc/m/gm) Tissue
Zn amino acid chelate
ZnCl
Muscle Heart Liver Kidney Brain
186 1,457 10,250 8,629 541
153 1,433 7,529 7,797 444
2
% Increase 22 2 36 11 22
M
In a second study, which was designed similarly to the above Zn study, M n amino acid chelate was compared to ^MnCl^ After being fasted for 24 hours, two groups of adult male Sprague-Dawley albino rats were orally administered 32 μ% of M n as either the chelate or chloride salt. Fourteen days following dosing, the animals were sacrificed and their tissues assayed for ^Mn. The delay in sacrificing was to allow for homeostasis. Wfaen the body is loaded with a stable Mn there is a rapid excretion of old tissue Mn via the bile and a redistribution of new Mn within the tissues^. The 14 days between dosing and tissue assay allowed the distribution of M n to occur. The results are shown in Table TV(2). When Mn was chelated to the amino acids, its metabolism within body tissues was much greater (X=82.3%) than as an inorganic salt. Fecal recovery of ^MnC^ was 33% more than from M n amino acid chelate. The remainder of the M n from MnCl was excreted via the urine after absorption, indicating lower metabolism of Mn from MnCl . M
M
M
M
2
2
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
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ASHMEAD
Metal Amino Acid Chelates and Inorganic Metal Salts
317
Table IV. Mean ^Manganese Levels in Tissue (cc/m/gm) Mn amino acid chelate
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Tissue
2
% Increase 197 104 21 109 4 58 27 138
36 52 80 190 54 89 22 112
107 106 97 397 56 141 28 266
Heart Liver Kidney Spleen Lung Sm Intestine Muscle Bone
MnCl
45
A third comparative study was designed using Ca. Adult male SpragueDawley albino rats were divided into two groups. After fasting for 24 hours each animal received 1 mg of C a orally as either Ca amino acid chelate or as CaCl . One week following the dosing, all of the animals were sacrificed and their tissues assayed for Ca. The delay in sacrificing the animals was to allow for hormonal production of a vitamin D dependent carrier to transfer the Ca from CaCl through the mucosal cell cytoplasm. The Ca amino acid chelate does not require this carrier molecule in order to be transferred to the plasma. Table V presents the results^. 45
2
2
Table V. Mean ^Calcium Levels in the Tissues (cc/m/gm) Ca amino acid chelate
Thsue Bone Muscle Heart Liver R. Cerebrum Kidney Serum Erythrocytes Whole Blood a
5,772 1,206 932 742 804 730 31 13 44
CaCl
% Increase*
3,682 614 642 664 698 686 8 19 27
57 96 45 12 15 6 288 (-32) 63
2
With the exception of the erythrocyte compartment.
45
The chelate group excreted 76% less C a in their feces than the C l group, indicating greater absorption from the chelate. Furthermore, the mean absorption and transfer of the C a from the amino acid chelate was 61.1% greater. 2
45
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
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BIOLOGICAL TRACE ELEMENT RESEARCH 59
In a fourth series of studies, 4.4 μο of Fe were administered in a single oral dose as either the amino acid chelate or as FeCl to fasted pregnant SpragueDawley female albino rats 4 days before expected parturition. Approximately 72 hours after dosing, the 15 animals in each group were sacrificed, and their tissues and fetuses assayed for Fe. The delay between dosing and assaying was to allow placental transfer of Fe. Table VI presents the results^). 3
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Table VI. Mean Fe Levels i n the Tissues of Pregnant Rats and Fetuses (cc/m/gm) Tissue
Fe amino acid chelate
Uterus Liver Kidney Spleen Heart Lung Fetus (X/Fetus)
4,925 9,675 950 325 1,425 2,925 46
FeCl
2
3,333 8,167 567 134 333 1,367 16
% Increase 48 18 68 143 328 114 188
The data in Table VI demonstrate that when Fe is chelated to amino acids, its uptake, and certainly, its utilization (X= 129.6%), are significantly greater than when equivalent amounts of Fe in the chloride form are ingested. An added finding in this study is the placental transport of the Fe as the amino acid chelate. Traditionally, in the latter stages of gestation, transplacental Fe transport has been difficult. Other studies have indicated that increased placental transport of Fe amino acid chelate is primarily due to the molecular weight of the chelate in the plasma (approximately 300 daltons) versus that of iron transferrin in the blood (approximately 90,000 daltons) (7). This research further demonstrated that the amino acid chelate is absorbed into the blood intact in the same molecular form as when it was ingested. The smaller molecule can then be more easily transferred through the so-called "placental barrier" than Fe attached to the much larger transferrin molecule. In conclusion, it has been shown that there are numerous factors which will affect mineral bioavailability. One of these factors is the chelation of the mineral with amino acids. The above data demonstrate that chelation with amino acids result in greater absorption and metabolism of the mineral than in the form of soluble salts.
Literature Cited 1.
Kratzer, F.; Vohra, P. In Chelates in Nutrition; CRC Press: Boca Raton, Fl., 1986; pp 35.
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.
24. 2. 3. 4.
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5.
6. 7.
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Metal Amino Acid Chelates and Inorganic Metal Salts319
Ashmead, H. D., Burton, S. Α.; Peterson, R. V. In Intestinal Absorption of Metal Ions and Chelates; Charles C Thomas: Springfield, Il., 1986. Miller, R. In Chelating agents in poultry nutrition; Proc. Delmarva Nutr. Short Course, 1968. Jensen, N. Biological Assimilation of Metals, U.S. Patent No. 4,167,546, Washington D. C., Sept. 11, 1979. Fang, S.; Burton, S. Α.; Peterson, R. V., et al. In Chelated Mineral Nutrition in Plants, Animals, and Man; Ashmead, D., Ed.; Charles C Thomas: Springfield, Il., 1982; pp 137-151. Underwood, E . In Trace Elements in Human and Animal Nutrition; Academic Press: New York, N.Y., 1977; pp 174-176. Ashmead, D., Graff, D. In Placental transport of chelated iron, Proc. IPVS, Mexico, 1982; pp 207.
R E C E I V E D August 1, 1990
In Biological Trace Element Research; Subramanian, K., et al.; ACS Symposium Series; American Chemical Society: Washington, DC, 1991.