Introduction
‘The significance of the protein–phytate complex in the digestive tract of animals has not yet been determined; whether this is associated with a low absorption of protein as amino acids is by no means certain.’ Now, nearly 60 years later and 20 years after the commercial introduction of phytate-degrading feed enzymes, this statement by Hill & Tyler(Reference Hill and Tyler1) is still largely correct and the uncertainty remains. Numerous scientific investigations into the phytate–phytase axis in pig and poultry nutrition alone have been completed without clarifying the position. This situation reflects the complexity of the relevant analytical, physiological and biochemical aspects in general and protein–phytate interactions specifically.
In 1991, an Aspergillus niger-phytase feed enzyme with the capacity to hydrolyse dietary phytate was introduced in The Netherlands. It was developed to provide pig and poultry producers with the means to reduce P concentrations in waste outputs from intensive production units in order to ameliorate P pollution of the environment. This is ecologically beneficial because P promotes eutrophication of fresh-water reserves(Reference Daniel, Sharpley and Lemunyon2). The substrate, phytate, is present in all feedstuffs of plant origin predominantly as a Mg and K salt of phytic acid (myo-inositol hexaphosphate; IP6), which may be represented as Mg3-K6-IP6(Reference Lott, Ockenden and Raboy3). Consequently, all practical pig and poultry diets contain variable concentrations of phytate, often in the order of 10 g/kg. Phytic acid contains 282 g phytate-bound P (phytate-P)/kg and has a molecular weight of 660 Da. However, the capacity of pigs and poultry to utilise phytate-P in practical diets via endogenous, mucosal phytase and phosphatase activities is limited. This is mainly due to the insolubility of mineral calcium phytate complexes at small-intestinal pH levels(Reference Wise4) in diets with conventional levels of Ca. Proximally, in the more acidic conditions of the stomach of pigs or the proventriculus and gizzard of poultry, phytate is relatively soluble and exogenous phytases have the capacity to hydrolyse IP6, at least partially at standard inclusion rates, thereby liberating inorganic P moieties. The enzymic degradation of phytate and the release of phytate-bound P, coupled with reductions in dietary P concentrations, combine to reduce P levels in excreta. In the landmark study of Simons et al. (Reference Simons, Versteegh and Jongbloed5), an A. niger-phytase reduced P excretion in pigs by 35% and in broiler chickens by 47% at an inclusion rate of 1000 phytase units (FTU)/kg.
Nevertheless, for nearly a decade the usage of phytase feed enzymes was essentially confined to The Netherlands in response to stringent anti-pollution legislation. However, the acceptance of phytase feed enzymes has expanded remarkably since 2000, as now the majority of pig and poultry rations are supplemented with phytase on a global basis. The prohibition of meat-and-bone meal in pig and poultry diets in Europe and elsewhere contributed to the upsurge in acceptance because it is usually a cheap P source. Also, declining inclusion costs of phytases coupled with increasing prices for feed ingredients generally have been contributing factors. The introduction of phytase feed enzymes of bacterial origin, which are more effective than the original fungal phytases, is a further reason for the increasing acceptance. More recently the escalating costs of inorganic P supplements, such as di-calcium phosphate, have driven the increasing usage of microbial phytases as these feed enzymes are, effectively, a more economical P source.
The world is now faced with a P crisis driven by the declining global reserves of rock phosphate(Reference Abelson6) and it has been predicted that P production will peak before 2040 and that commercially viable rock phosphate deposits will be depleted in less than 100 years(Reference Cordell, Drangert and White7). Thus, by reducing P inputs to pigs and poultry, phytase feed enzymes are making a positive ecological contribution aligned with more sustainable production of pig-meat, chicken-meat and eggs.
In addition to the liberation of phytate-bound P by phytase, Bryden et al. (Reference Bryden, Selle, Ravindran, Planter, Wieregna and Pfister8) suggested that ‘the enzyme (phytase) has provided new insights into the anti-nutritive properties of phytate. In particular, the interaction of phytate with dietary proteins, carbohydrates and fats may have significant economic consequences for animal nutrition.’ Some 10 years ago, we reviewed the accumulated knowledge of the consequences of protein–phytate interactions for protein utilisation in single-stomached animals(Reference Selle, Ravindran and Caldwell9); an update of this review is now timely for several reasons. The ‘extra-phosphoric effects’ of phytase are being increasingly recognised with the development of matrix values for amino acids in addition to P and Ca in the formulation of phytase-supplemented diets. There is now a better understanding of the phytate-induced increase in endogenous amino acid flows. New data on the relationship between phytate and outputs of mucin and Na within the gut have important implications. There is also the possibility that the polyanionic phytate molecule stabilises protein because of its kosmotropic effect under the Hofmeister series. The intention of the present review is to link together these recent findings and reappraise phytate interactions with proteins in pig and poultry diets and to consider their implications.
Protein–phytate interactions
Phytate is a reactive, polyanionic molecule potentially carrying twelve dissociable protons, with acid dissociation constants ranging from 1·5 to 10(Reference Costello, Glonek and Myers10). The capacity of phytate to interact with protein in cottonseed(Reference Jones and Csonka11), yellow peas(Reference Mattson12) and bean seed(Reference Bourdillon13) was reported decades ago. As reviewed by Cosgrove(Reference Cosgrove14), Cheryan(Reference Cheryan15) and Anderson(Reference Anderson, Finley and Hopkins16), it is generally accepted that negatively charged phytate molecules form binary protein–phytate complexes with proteins carrying a net positive charge at pH less than their isoelectric point. At pH exceeding their isoelectric point, with proteins carrying a net negative charge, a cationic bridge (usually Ca2+) links phytate and protein in ternary complexes. These interactions were demonstrated by Reddy & Salunkhe(Reference Reddy and Salunkhe17) in their investigations of phytate and albumin in black gram (Phaseolus mungo). Protein–phytate interactions were not detected at pH 6·40, which approximates the isoelectric point of black gram albumin. However, binary protein–phytate complex formation was observed at pH 2·80 and ternary complex formation was observed at pH 8·40, which was mediated by divalent cations.
Binary protein–phytate complexes
In the classic description of binary protein–phytate complexes Cosgrove(Reference Cosgrove14) concluded that protein–phytate interactions stem from phytate forming salt-like linkages with the basic amino acid residues of arginine, histidine and lysine at pH levels below protein isoelectric points. Cosgrove(Reference Cosgrove14) suggested that as a result of complex formation, protein molecules become closely packed around the relatively small and highly charged phytate anion leading to the formation of macromolecular aggregations or insoluble coacervates. Drawing on the investigations of Barré & Nguyen-van-Hout(Reference Barré and Nguyen-van-Hout18) into phytate and human serum albumin it appeared that phytate sequentially bound the terminal α-amino and ε-amino groups of lysine, the imidazole group of histidine and, finally, guanido groups of arginine. However, in a second study(Reference Barré and Nguyen-van-Hout19) with avian ovalbumin, the phytate-binding sequence differed to arginine, lysine and finally histidine.
Subsequently, Cheryan(Reference Cheryan15) suggested that the Barré & Nguyen-van-Hout(Reference Barré and Nguyen-van-Hout18, Reference Barré and Nguyen-van-Hout19) data contain several ambiguities. Similar solubility profiles for phytate and protein across a range of pH values where maximum insolubility coincides at a particular point are considered indicative of binary complex formation. From a series of soya protein studies(Reference Fontaine, Pons and Irving20–Reference De Rham and Jost23), Cheryan(Reference Cheryan15) concluded that the solubility of phytic acid ‘somewhat parallels’ that of soya protein. More recently, Anderson(Reference Anderson, Finley and Hopkins16) proposed that the extent of protein–phytate interactions is dependent on the number of unhindered cationic groups of the protein and that protein–phytate interactions were highly correlated with basic amino acid residues in several studies(Reference Barré and Nguyen-van-Hout18, Reference Barré and Nguyen-van-Hout19, Reference Okubo, Myers and Iacobucci24, Reference Prattley, Stanley and van der Voort25). This suggests that basic amino acid concentrations in proteins are critical to their propensity to be bound by phytate. Lysine monohydrochloride is frequently included in pig and poultry diets and this free basic amino acid has been shown to be bound by phytate from rice pollard(Reference Rutherfurd, Edwards, Selle and Cranwell26). Presumably, interactions between phytate and free lysine would reduce the extent of binary complex formation involving intact proteins.
Rajendran & Prakash(Reference Rajendran and Prakash27) investigated the kinetics and thermodynamics of sodium phytate and sesame α-globulin interactions. Sesame (Sesamum indicum L.) contains abundant phytate levels, as concentrations of 14·6 g phytate-P/kg or 51·8 g phytate/kg have been recorded in defatted sesame meal(Reference De Boland, Garner and O'Dell28). Sesame seed protein has an isoelectric point of 4·5 and a basic amino acid content of approximately 19·1% in which arginine is dominant(Reference Rivas, Dench and Caygill29). Specifically, the major sesame protein fraction, α-globulin, has a molecular weight of 2·5 × 105 Da and contains 18·7% basic amino acids(Reference Prakash and Nandii30). Rajendran & Prakash(Reference Rajendran and Prakash27) concluded that the interaction between sodium phytate and α-globulin was maximal at pH 2·3 and that complex formation was a biphasic process. In the rapid, first step sodium phytate binds with and changes the conformation of α-globulin. The slower, second step consists of progressive protein–protein associations to form polymers, ultimately resulting in precipitation when a critical mass is exceeded. The interaction requires a minimum sodium phytate:protein molar ratio of 10:1 and the number of α-globulin binding sites for sodium phytate was estimated to range from 11 to 20. Curiously, Rajendran & Prakash(Reference Rajendran and Prakash27) did not consider the complement of basic amino acids in sesame α-globulin in their discussion of protein–phytate interactions.
It is accepted that the propensity for proteins to be bound by phytate differs across feedstuffs. Mainly on the basis of reported protein–phytate solubility profiles, Champagne(Reference Champagne31) concluded that phytate is capable of binding proteins from soya(Reference Fontaine, Pons and Irving20, Reference De Rham and Jost23), wheat(Reference Hill and Tyler1), rapeseed(Reference Gillberg and Tornell32) and groundnut(Reference Fontaine, Pons and Irving20). Conversely, Champagne(Reference Champagne31) stated that proteins in cottonseed meal(Reference Fontaine, Pons and Irving20), maize germ(Reference O'Dell and de Boland33), sesame meal(Reference O'Dell and de Boland33) and rice bran(Reference Champagne, Rao and Liuzzo34) are not bound by phytate.
However, anomalies do appear to exist. The solubility profiles for total P and protein generated by Fontaine et al. (Reference Fontaine, Pons and Irving20) indicate that protein–phytate complexes are more likely to occur in groundnut meal and soyabean protein than cottonseed. However, cottonseed meal (19·7%)(Reference Ravindran, Cabahug and Ravindran35) has a higher proportion of basic amino acids than groundnut meal (14·9%)(Reference Ayres, Branscomb and Rogers36) and soyabean meal (16·6%)(Reference Ravindran, Cabahug and Ravindran35). Thus despite the relatively rich complement of basic amino acids in cottonseed meal, which contains an abundance of arginine, the propensity for phytate to bind cottonseed protein is considered to be less than either soya or groundnut proteins.
Recently, Kies et al. (Reference Kies, de Jonge and Kemme37) assessed protein–phytate interactions across a range of feedstuffs. The reductions in protein solubility generated by sodium phytate under in vitro conditions are shown in Table 1. At pH 2, phytate-induced reductions in protein solubility were substantial for casein (99%), soyabean meal (89%), sunflower-seed meal (84%) and maize (72%), intermediate for rapeseed meal (37%) and marginal for rice bran (6%). Importantly, at pH > 2, the effect of sodium phytate on protein solubility was diminished. The phytate-induced reductions in protein solubility were attributed to binary complex formation; however, it is evident from the tabulated values that there is no relationship between the basic amino acid content of test proteins and solubility reductions at pH 2. For example, rice bran protein has a relatively high proportion of basic amino acids but its solubility was barely altered by sodium phytate.
Table 1 Impact of pH on phytate-induced protein solubility reductions (%) of feedstuffs across a range of pH values in relation to their isoelectric point of protein and basic amino acid profile*
* Adapted from Kies et al. (Reference Kies, de Jonge and Kemme37).
† See Table 3.
‡ Casein, Vickery & White(Reference Vickery and White145); others, Ravindran et al. (Reference Ravindran, Cabahug and Ravindran35).
It is noteworthy that O'Dell & de Boland(Reference O'Dell and de Boland33) detected protein–phytate interactions in soya flakes but not in maize germ or sesame meal. In contrast Kies et al. (Reference Kies, de Jonge and Kemme37) reported protein–phytate interactions in maize at pH 2 and Rajendran & Prakash(Reference Rajendran and Prakash27) reported interactions between sesame α-globulin and phytate that peaked at pH 2·3. However, O'Dell & de Boland(Reference O'Dell and de Boland33) conducted their studies at pH levels of 4·4 and 9·0, so it appears that pH differences in the in vitro systems account for the apparent discrepancies in outcomes and emphasise the importance of pH to protein–phytate interactions. Further, the apparent limited capacity of phytate to bind protein feedstuffs such as cottonseed meal and rice bran is often dismissed on the grounds that the basic amino acid residues are inaccessible to phytate. However, basic amino acids are polar and hydrophilic and are normally found on the outer surface of a protein, particularly in the case of arginine(Reference Argos38, Reference Janin, Miller and Chothia39). Given this orientation, the likelihood is that the access of phytate to basic amino acids is largely unimpeded and the ‘inaccessibility’ argument may not be sound.
Numerous factors influence the intensity of binary protein–phytate interactions in addition to pH. Dietary Ca is one example and Ca has a broad impact on the phytate–phytase axis in pig and poultry nutrition(Reference Selle, Cowieson and Ravindran40). Ca is largely derived from limestone, which has a very high acid-binding capacity(Reference Lawlor, Lynch and Caffrey41) and increasing dietary Ca levels tend to elevate gut pH. As discussed previously(Reference Selle, Cowieson and Ravindran40), in the Ravindran et al. (Reference Ravindran, Cabahug and Ravindran42) study, seemingly small increases in analysed dietary Ca concentrations relative to both protein and phytate noticeably depressed amino acid digestibility responses to A. niger-phytase. That Ca can interact with phytate is established but Ca may also interact with protein including soya protein(Reference Scilingo and Anon43). Okuba et al. (Reference Okubo, Myers and Iacobucci24, Reference Okubo, Myers and Iacobucci44, Reference Okubo, Iacobucci and Myers45) investigated interactions between phytate and glycinin, the major soya protein. At pH 3, sufficient Ca was able to dissociate glycinin–phytate complexes, which was attributed to Ca competing with glycinin for access to negatively charged phytate molecules. The potential capacity of Ca to disrupt binary protein–phytate interactions may explain the diminished amino acid digestibility responses to supplemental phytase at higher Ca concentrations in the Ravindran et al. (Reference Ravindran, Cabahug and Ravindran42) study.
According to the Cosgrove(Reference Cosgrove14) and Rajendran & Prakash(Reference Rajendran and Prakash27) descriptions of binary complexes, the likelihood is that phytate is ‘protected’ by a shield of aggregated protein once complex formation takes place and would be less susceptible to hydrolysis by exogenous phytase. Thus phytase essentially prevents de novo complex formation via the prior hydrolysis of phytate and binary complexes may be an important limiting factor on the extent of enzymic degradation of phytate.
Ternary protein–phytate complexes
Ternary protein–phytate complexes are formed de novo in the small intestine where the major components are linked via a cationic bridge, usually Ca2+, the most prevalent divalent cation in digesta. More attention has been paid to the impact of ternary protein–phytate complexes on mineral bioavailability than protein/amino acid utilisation and this appears to have led to a consensus that ternary complexes are not important in respect of phytate reducing protein availability.
Nosworthy & Caldwell(Reference Nosworthy and Caldwell46, Reference Nosworthy and Caldwell47) reported precipitation of soya glycinin, phytate and Zn at pH 6·2 where 1 mol of glycinin was involved in a ternary complex with 7 mol of phytate and 39 mol of Zn. Thus phytate has a tremendous capacity to bind protein in ternary complexes under in vitro conditions. The affinity of phytate for Zn is established and the precipitation of Zn in ternary complexes may both reduce the activity of Zn-dependent proteases(Reference Jongeneel, Bouvier and Bairoch48) and compromise the integrity of the immune system(Reference Fraker, King and Laakko49).
The negative impact of phytate on Zn availability(Reference Wise4, Reference Zhou, Fordyce and Raboy50) has been seminal to the appreciation of protein–phytate interactions, particularly in relation to soya protein. Phytate has the capacity to bind Zn in both mineral–phytate and ternary protein–phytate complexes. This is reflected in pigs, where phytate is a key aetiological factor in parakeratosis, a manifestation of Zn deficiency(Reference Oberleas, Muhrer and O'Dell51). As demonstrated by Cranwell & Liebman(Reference Cranwell and Liebman52), the phytate content of soyabean, rather than the fibre content, reduces the bioavailability of Zn in humans. For this reason, the preparation of soya protein isolates and concentrates with reduced phytate contents to avoid Zn deficiencies in human infants has been a goal for decades(Reference McKinney, Sollars and Setzkorn53). As discussed by Erdman(Reference Erdman54), protein concentrates with reduced phytate contents can be prepared by exploiting the capacity of phytate to bind protein, which has been demonstrated in soya(Reference Erdman, Weingartner and Mustakas55) and rapeseed(Reference Tzeng, Diosady and Rubin56), and the fate of phytate following the preparation of soya protein concentrates/isolates has been reviewed(Reference Deak and Johnson57).
In relation to ternary complexes and protein availability, Champagne et al. (Reference Champagne, Fisher and Hinojosa58) suggested that the protein moiety of ternary complexes is comprised of either amino acids or small peptides and it then follows that the amount of protein bound in ternary complexes in the small intestine may not be sufficient to compromise amino acid digestibility(Reference Selle, Ravindran and Caldwell9). However, the validity of this interpretation depends on the molecular weights of protein present in small-intestinal digesta. In one of a series of studies, Montagne et al. (Reference Montagne, Crevieu-Gabriel and Toullec59) determined the molecular weights of protein along the small intestine of pre-ruminant calves. In diets in which either a soya protein concentrate or a soya protein isolate partially replaced skimmed milk powder, an average of nearly 60% of protein present in ileal digesta had a molecular weight in excess of 20 000 Da (Table 2). Protein fractions of this magnitude were even more dominant in the duodenum and jejunum as there is a declining gradient in the size of proteins along the gut. Consequently, it appears that sufficient protein may be bound as ternary protein–phytate complexes in the small intestine to disrupt protein digestion and amino acid absorption, and the importance of ternary complexes may have been dismissed prematurely.
Table 2 Distribution of protein and peptide fractions in ileal digesta from three diets according to molecular mass as a percentage of total crude protein*
* Adapted from Montagne et al. (Reference Montagne, Crevieu-Gabriel and Toullec59).
Of relevance is that Montagne et al. (Reference Montagne, Salgado and Toullec60) reported that the partial substitution of soya protein concentrate for skimmed milk powder increased alkaline phosphatase activity in the duodenum and jejunum by approximately 33%, which was more pronounced with soya protein isolate. Phytate was probably present in both soya preparations(Reference Deak and Johnson57) and may have triggered these increases in alkaline phosphatase activity. Therefore, it is noteworthy that Montagne et al. (Reference Montagne, Toullec and Formal61) found that both soya preparations substantially increased the flow of mucin protein in the duodenum, jejunum and ileum in pre-ruminant calves by approximately 70–90%. Moreover, Montagne et al. (Reference Montagne, Toullec and Lalles62) determined the effect of these partial substitutions on the apparent digestibility of cystine, lysine and threonine at the jejunal and ileal levels. With the soya protein concentrate, reductions in ileal digestibility of cystine (4·6%), lysine (4·1%) and threonine (7·2%) were modest in comparison with reductions in jejunal digestibility for cystine (49·4%), lysine (19·0%) and threonine (23·3%). The marked reduction in the jejunal digestibility of cystine may reflect its involvement in disulfide linkages within soya protein. Thus, relative to the control diet, soya protein concentrate depressed amino acid digestibility by an average of 30·6% at the level of the jejunum and by 5·3% at the ileal level. Thus the soya protein substitution both depressed and delayed small-intestinal uptakes of the three amino acids assessed and it is possible that the residual phytate content in soya concentrate contributed to this ‘distal shift’ in the site of amino acids absorption as a result of ternary complex formation.
An additional mechanism for protein–phytate interactions
The interaction of phytate with protein by forming binary and ternary complexes has been recognised for decades. Very recently, however, an additional or alternative mechanism has been suggested where phytate interacts with protein by acting as a ‘Hofmeister anion’. The mechanisms by which Hofmeister ions influence protein stability has been reviewed by Baldwin(Reference Baldwin63) and the Hofmeister or lyotropic series is a classification of cations and anions based on their capacity to stabilise or destabilise proteins. The reactions are complex but it appears that ions influence protein solubility mainly by changing the hydrogen-bonding properties of water in the surrounding medium. Ions may break hydrogen bonds in water systems and are classified as chaotropes that destabilise proteins; alternatively ions may form hydrogen bonds in water and stabilise proteins and these ions are kosmotropes(Reference Zhang, Furyk and Bergbreiter64). The impact of anions on protein solubility appears to be more potent than cations, and phosphate (HPO42–) is ranked as a kosmotrope(Reference Zhang, Furyk and Bergbreiter64). IP6 contains six HPO42– moieties and this suggests that the polyanionic IP6 phytate molecule has strong kosmotropic properties under the Hofmeister series that would tend to reduce protein solubility.
Cowieson & Cowieson(Reference Cowieson and Cowieson65) provided an indication that phytate does act as a kosmotropic anion in a study involving hen egg white lysozyme and sodium phytate. This in vitro assay was completed at pH 6·5, which is less than the isoelectric point of lysozyme (pH 9·4), and lysozyme has a basic amino acid complement of 15·5% on a molar basis(Reference Thompson66). These workers reported that increasing sodium phytate concentrations from 1 to 25 mm reduced lysozyme solubility from 100 to 50% but increasing phytate concentrations to 50–100 mm restored the solubility of lysozyme. However, X-ray crystallography did not detect any direct protein–phytate interactions to explain the reduction in protein solubility. Moreover, increasing the concentration of lysozyme against a fixed phytate concentration reduced protein solubility in the order of 85%. These outcomes would not be anticipated if phytate was directly binding protein in binary complexes. Finally, the effect of phytate on the solubility of five different proteins was not related to their isoelectric points, which ranged from pH 5·19 (ovalbumin) to 9·4 (lysozyme). Rather than phytate directly interacting with protein, Cowieson & Cowieson(Reference Cowieson and Cowieson65) proposed that phytate was indirectly influencing protein solubility via water thermodynamics as a kosmotropic anion. The magnitude of the protein solubility reduction was increased by protein concentration and this suggests that phytate is indirectly triggering protein aggregation. Phytate is negatively charged above pH 1·1(Reference Cosgrove14) and it may electrostatically attract a hydration shell in an aqueous media and compete with other molecules for water, reducing their solubility, as water potential is reduced with increasing phytate concentrations.
That dietary phytate may be acting as a kosmotropic anion raises wider issues. Numerous ‘Hofmeister ions’ are added to pig and poultry diets and it is not clear where a particular diet falls in the kosmotropic–chaotropic spectrum. Kosmotropic ions include various carbonates, phosphates, sulfates and chlorides; whereas Ca, Mg and Na are amongst the chaotropic ions(Reference Baldwin63, Reference Zhang, Furyk and Bergbreiter64). Limestone is routinely included in pig and broiler diets to supply approximately 10 g Ca/kg and this typical feed ingredient may have lyotropic effects. Limestone comprises about 370 g Ca/kg and Ca2+ is chaotropic; however, the balance is carbonate and CO32– is one of the strongest known kosmotropes(Reference Zhang, Furyk and Bergbreiter64). Thus, there is a need to investigate the net effect of a range of feed ingredients, including limestone or Ca2+ and CO32–, on protein solubility on the basis that, under the Hofmeister series, kosmotropic and chaotropic ions influence protein stability.
The proposal that phytate may indirectly influence protein solubility because it is a kosmotropic anion having an impact on the surrounding water medium differs radically from the accepted mechanisms of direct binary and ternary protein–phytate complex formation. However, it does not preclude the possibility that phytate influences protein solubility by interactions with both the protein per se and the surrounding water matrix. Where the effect of phytate on protein digestibility is dependent on binary or ternary complex formation and direct interaction with the protein surface then the amino acid composition and isoelectric point of the protein would be pivotal to the effect of phytate and, axiomatically, phytase. Alternatively, the polarity or hydrophobicity of protein may be the critical factor for phytate to influence its stability via indirect interactions under the Hofmeister series. If the kosmotropic properties of phytate are important, then an intriguing issue is raised. It is known that the capacity of phytate to bind Ca is disproportionately diminished as phytase degrades IP6 to lesser phytate esters(Reference Selle, Cowieson and Ravindran40); alternatively, it is not known if the phytase-induced degradation of IP6 increases or decreases the kosmotropic potency of the liberated phosphate anions.
Isoelectric points of protein
The pH along the gastrointestinal tract, relative to the isoelectric points of protein, should be pivotal to the integrity of binary protein–phytate complexes. Shafey et al. (Reference Shafey, McDonald and Dingle67) recorded pH values of 4·89 in the crop, 1·98 in the proventriculus, 3·14 in the gizzard, 5·53 in the duodenum, 6·06 in the jejunum, 6·62 in the ileum and 6·48 in the caecum in broiler chickens offered diets containing 10·7 g Ca/kg. Interestingly, Engberg et al. (Reference Engberg, Hedemann and Jensen68) found that pelleting broiler diets reduced intestinal pH, and they recorded average pH values of 6·01 in the duodenum, 6·10 in the jejunum and 6·94 in the ileum of chickens. In 32-d-old pigs offered maize–soya diets containing 8 g Ca/kg, Li et al. (Reference Li, Yi and Yin69) reported digesta pH of 3·27 in the stomach, 5·72 in the duodenum, 5·98 in the jejunum and 6·94 in the ileum.
Clearly, there is a substantial increase in pH as digesta transits from the stomach or gizzard into the duodenum, and binary protein–phytate complexes dissociate should this increase exceed the protein isoelectric point. Soyabean meal is the dominant protein source in pig and poultry diets and solvent-extracted soya protein has an isoelectric point of pH 4·1(Reference Monaghan-Watts70). Soya protein–phytate complexes will dissociate once digesta transits into the relatively alkaline pH of the duodenum and their ephemeral nature may limit their nutritional importance. However, structural changes to soya protein induced by its aggregation with phytate may still reduce its digestibility in the small intestine in its dissociated state.
Csonka et al. (Reference Csonka, Murphy and Jones71) determined the isoelectric point of a large number of proteins and a selection of these values is tabulated (Table 3). It is evident that the isoelectric point of proteins in cereal grains (5·90–6·45) is higher than proteins in oilseed meals (4·70–5·50); for example, wheat gliadin has an isoelectric point of pH 6·45 as opposed to pH 4·70 for soya glycinin. This comparison suggests that while binary complexes in soyabean, rapeseed and cottonseed meals will dissociate in the small intestine, this may not be the case in wheat, maize and sorghum. Consequently, phytate complexes with proteins from cereal grains may persist in the small intestine; this, as discussed later, may have interesting implications for starch digestibility.
Table 3 Isoelectric points of selected protein sources*
* Adapted from Csonka et al. (Reference Csonka, Murphy and Jones71).
† Vioque et al. (Reference Vioque, Sanchez-Vioque and Clemente146).
‡ Bau et al. (Reference Bau, Mohtadi-Ni and Mejean147).
Impact of phytase on amino acid digestibility in individual feedstuffs
Ravindran et al. (Reference Ravindran, Cabahug and Ravindran35) and Rutherfurd et al. (Reference Rutherfurd, Chung and Moughan72) reported that exogenous phytases increased the apparent ileal digestibility (AID) and true ileal digestibility (TID) of amino acids across a range of individual feedstuffs in broiler chickens, as shown in Table 4. In the first study, 1200 FTU A. niger-phytase/kg increased the AID of fourteen amino acids by averages of 2·67% in rapeseed meal, 3·40% in maize, 3·66% in wheat middlings, 4·16% in soyabean meal, 4·64% in sunflower-seed meal, 4·82% in cottonseed meal, 6·60% in sorghum, 7·52% in rice polishings and 9·26% in wheat. These data were largely confirmed in the second study where 750 U Peniophora lycii-phytase/kg increased TID coefficients of sixteen amino acids by averages of 3·90% in maize, 5·30% in rice bran, 6·39% in soyabean meal, 9·31% in rapeseed meal and 12·94% in wheat. Phytase responses in maize, wheat, soyabean meal and rice bran were similar in both studies and both research groups reported a substantial, three-fold difference in the magnitude of the phytase response between wheat and maize. The exception was rapeseed meal where different oil extraction processes may have contributed to the discrepancies in both amino acid digestibility and the magnitude of the phytase response.
Table 4 Impacts of 1200 phytase units Aspergillus niger-phytase/kg on the mean apparent ileal digestibility (AID) coefficient of fourteen amino acids(Reference Ravindran, Cabahug and Ravindran35) and 750 U Peniophora lycii-phytase/kg on the mean true ileal digestibility (TID) coefficient of sixteen amino acids(Reference Rutherfurd, Chung and Moughan72) in individual feedstuffs
It is instructive to consider the results of the study by Ravindran et al. (Reference Ravindran, Cabahug and Ravindran35) more closely (Table 5). The quantities of ileal digestible amino acids generated by phytase were not related to the amino acid composition of maize (P>0·85). In contrast, there were significant correlations (P < 0·001) for rapeseed meal, sunflower-seed meal, soyabean meal, wheat, cottonseed meal and sorghum. To illustrate this discrepancy, the relationships between the amino acid composition of maize and sorghum and the amino acids released by phytase are shown in Fig. 1. Moreover, for the last six feedstuffs mentioned, there was a significant relationship (r 0·913; P < 0·015) between the isoelectric points of protein and the magnitude of phytase responses. This may indicate that proteins with relatively high isoelectric points are more likely to be responsive to phytase because their binary protein–phytate complexes are more intact along the small intestine. It should be noted that had maize been included in this exercise the relationship would not be significant; however, maize responded very differently to phytase in comparison with the other six feedstuffs in this study.
Table 5 Data derived from the study by Ravindran et al. (Reference Ravindran, Cabahug and Ravindran35) which determined the effect of Aspergillus niger-phytase in broiler chickens on the apparent ileal digestibility of fourteen amino acids in individual feedstuffs
Fig. 1 Relationships between amino acid composition and amount of ileal digestible amino acids released by phytase in (a) maize (R 2 0·003) and (b) sorghum (R 2 0·987) (adapted from Ravindran et al.(Reference Ravindran, Cabahug and Ravindran35)).
Implications of binary protein–phytate complexes
Several research groups have concluded that complexed protein is refractory to pepsin digestion under in vitro conditions(Reference Barré and Nguyen-van-Hout18, Reference Camus and Laporte73–Reference Knuckles, Kuzmicky and Gumbmann76) and this may also apply to phytate-induced aggregations of protein under the alternative hypothesis that phytate acts as a kosmotropic anion. The key study by Vaintraub & Bulmaga(Reference Vaintraub and Bulmaga77) found that phytate reduced pepsin hydrolysis of bovine serum albumin by approximately 90% and Hb, casein and 11S soya protein by 65%. These maximal reductions were observed at pH 2–3 but reductions were not evident at pH 4·0–4·5; this indicates a narrow pH band for protein–phytate interactions. These reductions in pepsin hydrolysis were attributed to phytate binding with the substrate and rendering it refractory to digestion, presumably by phytate-induced alterations to protein structure and solubility.
Given this is the case, phytate has the potential to interfere with the initiation of protein digestion. Moreover, peptides generated by pepsin are regulators of the protein digestive processes(Reference Krehbiel, Matthews and D'Mello78), which suggests that this function may be compromised as well. However, if phytate complexes sufficient protein, rendering it refractory to pepsin digestion, then this could trigger gastric hypersecretions of pepsin and hydrochloric acid (HCl) as a compensatory mechanism. Condensed tannins have the capacity to bind protein, so it is relevant that repeated administrations of tannic acid to rats have been shown to increase gastric secretions of pepsin and HCl by approximately 60%(Reference Mitjavila, de Saint Blanquat and Derache79). Further indirect support of the concept of pepsin and HCl hypersecretion is provided by Decuypere et al. (Reference Decuypere, Knockaert and Henderickx80). These workers compared inclusions of soluble or insoluble soya isolates at 140 g/kg in diets for weaner pigs, and the in vitro pepsin digestibility of the soluble soya isolate was superior to the insoluble isolate. Higher peak pepsin activities were observed in pigs offered the insoluble isolate and the differences were significant at 135, 150 and 165 min post-feeding and pepsin activity was approximately 64% greater in pigs offered the insoluble soya isolate. Thus it is plausible that the presence of phytate-induced protein aggregations in the stomach that are refractory to pepsin digestion would promote gastric hypersecretion.
Both pepsin and HCl are described as endogenous aggressors(Reference Allen and Flemström81) and their hypersecretion would be countered by protective outputs of mucin and sodium bicarbonate (NaHCO3). For example, increased gastric mucin secretions in response to pepsin infusion have been demonstrated in rats(Reference Munster, Bagshaw and Wilson82). Importantly, as first reported by Cowieson et al. (Reference Cowieson, Acamovic and Bedford83), phytate increases mucin and Na excretion in broilers, which is ameliorated by phytase. It is possible that Na was secreted into the gut lumen as NaHCO3 to buffer excess HCl. Also in broiler chickens, Onyango et al. (Reference Onyango, Asem and Adeola84) reported that free phytic acid increased excretion of crude mucin by 50% but a Mg, K salt of phytic acid (Mg-K-phytate) increased crude mucin excretion by 162%. Mg-K-phytate is more akin to phytate naturally present in feedstuffs and it noticeably increased mucin secretions in poultry, and an Escherichia coli-derived phytase tended to stem this increase in mucin output.
Lien et al. (Reference Lien, Sauer and He85) reviewed the dietary influences on mucin secretion in the digestive tract of single-stomached animals where phytate was not specifically identified as an influential factor but considerable attention was paid to soluble and insoluble fibre. For example, Satchithanandam et al. (Reference Satchithanandam, Jahangeer and Cassidy86) reported that inclusions of wheat bran at 100 and 200 g/kg in a fibre-free diet for rats increased mucin levels in the small-intestinal lumen by approximately 200%. However, wheat bran and similar by-products are rich in phytate, as an average phytate content of 24·8 g/kg was recorded in seven samples(Reference Selle, Walker and Bryden87). Thus, there is the possibility that the large increase in mucin secretion recorded in this study was at least partially due to the phytate content of wheat bran in addition to its fibre content. Interestingly, Onyango et al. (Reference Onyango, Madsen and Gendler88) showed that phytate increased mucin gene expression (Muc1, Muc2) in jejunal and colonic mucosa in mice. Consequently, if phytate increases mucin secretion, as a response to hypersecretion of pepsin and HCl and/or direct ‘irritation’ of the gut mucosa, this has clear implications for the flow of endogenous amino acids because porcine mucin has a protein component of 343 g/kg and essentially remains undigested in the small intestine. Mucin protein contains little methionine and histidine but an abundance of threonine, proline and serine(Reference Lien, Sauer and Fenton89).
The impacts of phytate and phytase on the endogenous amino acid flows in broiler chickens have been investigated and reviewed(Reference Cowieson and Ravindran90–Reference Cowieson, Bedford and Selle92). Cowieson & Ravindran(Reference Cowieson and Ravindran90) found that increasing the phytate content of the diet from 8·5 to 11·5 and 14·5 g/kg generally increased endogenous amino acid flows at the ileal level. Overall, the increase from 8·5 to 11·5 g phytate/kg significantly increased (P < 0·001) the flow of seventeen amino acids by 27·2% (19 393 v. 15 247 mg/kg DM intake) and 500 FTU E. coli-phytase/kg reduced (P < 0·001) the flow by 20·0% (15 459 v. 19 327 mg/kg DM intake). Moreover, there was a positive correlation (r 0·762; P < 0·005) between the phytase-induced reductions in endogenous amino acid flows and the amino acid profile of mucin. The results followed a similar pattern in a second study(Reference Cowieson, Ravindran and Selle91) and, again, there was a positive correlation (r 0·556; P < 0·03) between the reductions in endogenous amino acid flows generated by phytase and the mucin amino acid profile. The implication of the significant regressions in both experiments is that phytate was exacerbating, and phytase attenuating, endogenous amino acid flows by making an impact on mucin secretions. However, the extent to which the protein component of mucin contributes to total endogenous protein/amino acids in the terminal ileum of poultry requires clarification, as it has been suggested that the mucin contribution is 19% in calves and 11% in pigs(Reference Montagne, Piel and Lalles93).
Bohak(Reference Bohak94) determined the amino acid composition of pepsin and pepsinogen in chickens. Pepsin has an unusual amino acid profile in that it contains a paucity of basic amino acids but considerable quantities of aspartic acid, serine, glycine and threonine. It is instructive to compare the pepsin amino acid profile with the variations in endogenous amino acid flows induced by phytate and phytase in the two studies(Reference Cowieson and Ravindran90, Reference Cowieson, Ravindran and Selle91) discussed. When the data are combined, there are significant correlations between phytate-induced increases (r 0·669; P < 0·001) and phytase-induced decreases (r 0·635; P < 0·001) in endogenous amino acid flows and the amino acid composition of pepsin. These significant relationships support the thesis that phytate increases the secretion of pepsin and mucin; both are potential sources of endogenous amino acids.
However, phytate may trigger extra-secretions of endogenous enzymes other than pepsin, by modifying substrates and rendering them less susceptible to hydrolysis, which would increase endogenous amino acids flows. Phytate is a potent inhibitor of α-amylase in vitro (Reference Desphande and Cheryan95), which may have in vivo relevance in pigs and poultry. As discussed later, it has been reported(Reference Sultan, Gan and Li96, Reference Sultan, Gan and Li97) that phytase increases the digestibility of sorghum starch, which implies that phytate has a negative effect. Phytate may interact with starch per se or with kafirin and glutelin, two proteins that are physically associated with starch granules in sorghum endosperm, and these interactions may modify the substrate leading to compensatory increases in outputs of α-amylase in order to digest starch.
Phytate has been shown to depress total tract digestibility of lipids in rats by 7·03%, from 0·910 to 0·846(Reference Nyman and Björk98); moreover, it has been reported that phytase increased the digestibility of fat and fatty acids in broilers(Reference Zaefarian, Romero and Ravindran99). As a main effect, 500 FTU E. coli-phytase/kg increased the ileal digestibility of fat in maize and wheat by 4·16% (0·827 v. 0·794; P < 0·001) and significantly increased the digestibility of specific fatty acids by up to 5·7%. Also, Liu et al. (Reference Liu, Ru, Wang and Xu100) reported that 1000 FTU E. coli-phytase/kg enhanced crude fat ileal digestibility by 5·64% (0·862 v. 0·816) in maize–soya broiler diets. These positive responses may have stemmed from the involvement of phytate, Ca and lipids in the de novo formation of metallic soaps in the gut lumen(Reference Ravindran, Cabahug and Ravindran42). Again, it is possible that phytate triggers compensatory increases in lipase outputs, which would contribute to endogenous amino acid flows.
Cowieson et al. (Reference Cowieson, Acamovic and Bedford83) reported that phytate increases, and phytase decreases, Na excretion in broilers on a total-tract basis. At the level of the ileum the impacts are more pronounced, as Ravindran et al. (Reference Ravindran, Morel and Partridge101) found that phytate decreased ileal Na digestibility (–0·38 v. − 0·24; P < 0·05) but phytase had a corresponding positive effect (–0·18 v. − 0·52; P < 0·001). Also, in broiler diets containing 11·0 g phytate/kg, 500 FTU E. coli-phytase/kg increased coefficients of ileal Na digestibility from − 0·52 to − 0·04(Reference Selle, Partridge and Ravindran102). Thus phytate has the capacity to drag Na into the small-intestinal lumen and this is counteracted by phytase; this transition of Na into the gut lumen may be as NaHCO3 to buffer HCl hypersecretions
Interactions between phytate and starch
Rickard & Thompson(Reference Rickard, Thompson and Shahidi103) nominated several mechanisms by which phytate may negatively influence starch digestion. Phytate may inhibit amylase activity either directly or via chelation of Ca, which is a requisite cofactor for amylase. Additionally, phytate may interact with starch directly or indirectly by binding proteins that are closely associated with starch granules. In a study of covalently bound P in starch granules Blennow et al. (Reference Blennow, Bay-Smidt and Olsen104) noted that considerable quantities of phytate in sorghum starch precluded analyses of glucose 3-phosphate and glucose 6-phosphate, which was not the case with potato and cassava starches. Thus, there is the inference that phytate-P also could be covalently bound to glucose in starch polymers and that starch–phytate complexes may depress energy utilisation. Theoretically, phytate may bind starch indirectly via interacting with proteins that are closely associated with starch. These interactions may be as binary complexes that persist in the small intestine due to the relatively high isoelectric points of protein in cereals, and phytate may bind starch-associated proteins in ternary protein–phytate complexes as well. Both mechanisms are consistent with the suggestion of Thompson(Reference Thompson105, Reference Thompson and Graf106) that phytate can indirectly bind starch.
Starch granules are enmeshed in a protein matrix in the endosperm of cereal grains(Reference Rooney and Pflugfelder107). This physical proximity would facilitate starch–protein interactions, and strong electrostatic attractions have been reported between potato starch and casein(Reference Takeuchi108). Anderson et al. (Reference Anderson, Levine and Levitt109) measured breath H2 levels in human subjects to assess wheat carbohydrate absorption and concluded that an appreciable proportion of starch was not absorbed, which was attributed to interactions between the starch and protein moieties in wheat flour. Subsequently, it was proposed that starch–protein interactions in food influence starch digestibility and the glycaemic response(Reference Thorne, Thompson and Jenkins110). It was reported(Reference Jenkins, Thorne and Wolever111) that removal of the protein composite gluten (gliandin and glutelin) from wheat flour significantly increased in vitro starch digestibility. Also, gluten removal increased glycaemic responses in vivo and increased starch absorption on the basis of breath H2 measurements. The presence of gluten in unprocessed wheat flour had the opposite effects and these decreases in glycaemic responses and starch absorption were attributed to starch–protein interactions.
As reviewed by Baldwin(Reference Baldwin112), proteins that are located in and on starch granules are described as starch granule-associated proteins (SGAP). Interactions between wheat starch granules and soya proteins were investigated(Reference Ryan and Brewer113) where protein binding was reduced by the removal of SGAP from the surface of starch granules. It was proposed that SGAP mediates the binding of exogenous protein to starch granules. Starch–protein interactions occur, including adsorption of wheat proteins by potato starch(Reference Eliasson and Tjerneld114), so it is possible that phytate may indirectly complex starch by binding SGAP. Therefore, it is relevant that Camden et al. (Reference Camden, Morel and Thomas115) reported that 250 U Bacillus subtilis phytase/kg enhanced ileal starch digestibility by 1·87% (0·982 v. 0·964) in broiler chickens offered maize–soya diets.
Starch granules are intimately associated with both protein bodies, which are composed of kafirin, and the glutelin protein matrix in sorghum endosperm. Sorghum differs from other cereal grains in that its nutritive value is vulnerable to ‘wet-cooking’, which is believed to be a consequence of disulfide linkage formation, particularly in kafirin(Reference Selle, Cadogan and Li116). Consequently, starch could interact with kafirin and/or glutelin, which may also involve phytate, as sorghum contains relatively high phytate concentrations(Reference Selle, Walker and Bryden87). Interestingly, Sultan et al. (Reference Sultan, Gan and Li96, Reference Sultan, Gan and Li97) investigated the effects of phytase in broilers offered diets containing sorghum at 918 g/kg. Phytase substantially increased the ileal digestibility coefficients of starch by 14·7% (0·86 v. 0·75) and crude protein by 8·3% (0·78 v. 0·72) at 21 d post-hatch. In the second study, phytase increased starch digestibility in the jejunum by 9·0% (0·607 v. 0·557), upper ileum by 4·5% (0·878 v. 0·840) and lower ileum by 2·4% (0·927 v. 0·905) at 42 d post-hatch. The digestibility of sorghum starch increases as it transits the small intestine, with corresponding reductions in responses to phytase. Axiomatically, the Sultan et al. (Reference Sultan, Gan and Li96, Reference Sultan, Gan and Li97) studies suggest that phytate depresses starch digestibility and delays its absorption from the small intestine, although the fermentative activity of the gut microflora would contribute to starch disappearance along the small intestine.
Phytase amino acid digestibility assays
The impact of phytate and phytase on protein utilisation has been mainly assessed by amino acid digestibility assays in pigs and poultry. One noteworthy exception is the Ketaren et al. (Reference Ketaren, Batterham and Dettmann117) study in grower pigs in which phytase significantly increased protein deposition and retention; however, these positive outcomes may have been in part a consequence of enhanced P availability. As reviewed by Selle & Ravindran(Reference Selle and Ravindran118, Reference Selle and Ravindran119), the effects of exogenous phytases on the AID of amino acids in pigs and poultry have been assessed in approximately fifty assays. These assays indicate that the influence of phytase is inconsistent, and the impact is marginal in the majority of reported studies, particularly in pigs. However, the straightforward adjudication that phytase does not improve ileal digestibility of amino acids in pigs and poultry seems justified but it may be misleading.
Phytase amino acid digestibility assays in poultry
In phytase amino acid digestibility assays involving complete broiler diets, there is a consistent pattern in which more robust responses have been recorded in studies using acid-insoluble ash or titanium oxide as dietary markers in comparison with chromic oxide(Reference Selle, Ravindran and Bryden120). If inert marker selection in phytase assays is a confounding factor, it has not been resolved. However, its potential importance is apparent from a comparison of three assays in which the one enzyme at the same inclusion rate (1000 FTU E. coli-phytase/kg) was added to maize–soya diets but different dietary markers were used. In the two chromic oxide assays(Reference Dilger, Onyango and Sands121, Reference Onyango, Bedford and Adeola122) the median phytase response across eighteen assessed amino acids was 2·40 and 1·06%, respectively. Threonine is almost invariably the most phytase-responsive essential amino acid and in these two assays the AID of threonine was increased by 1·99 and 2·49%. In contrast, in the titanium oxide assay(Reference Ravindran, Morel and Partridge101), the median phytase response was 5·38% and the AID of threonine was increased by 10·16%. In this study the control diets were supplemented with phytase at three inclusion levels. As a main effect, 500, 750 and 1000 FTU phytase/kg improved the average AID coefficient of eighteen amino acids from 0·798 to 0·833 (4·39%), 0·837 (4·89%) and 0·840 (5·26%), respectively. Moreover, in addition to the compelling Ravindran et al. (Reference Ravindran, Morel and Partridge101) study, there are several ‘non-chromic oxide’ assays in broiler chickens(Reference Ravindran, Cabahug and Ravindran42, Reference Selle, Partridge and Ravindran102, Reference Ravindran, Selle and Bryden123–Reference Selle, Ravindran and Ravindran127) in which phytase unequivocally enhanced amino acid digestibilities.
It would appear that the selection of chromic oxide for phytase amino acid digestibility assays may be contributing towards the equivocal outcomes, and the shortcomings of this marker have been discussed previously(Reference Selle and Ravindran118, Reference Selle, Ravindran and Bryden120). A consideration of the impact of exogenous phytases on gut passage rates is instructive, as phytase supplementation, particularly of low-P diets, frequently increases feed intake of broilers and, presumably, gut passage rates. In support of this, 600 FTU A. niger-phytase/kg has been shown to reduce gut transit times by 17·0% from 94·8 to 78·7 min in chicks offered maize–soya diets(Reference Watson, Matthews and Southern128).
Differences in feed intake rates can influence the outcomes of phytase amino acid digestibility assays. For example, Sebastian et al. (Reference Sebastian, Touchburn and Chavez129) evaluated the effect of phytase on amino acid digestibilities in male and female broilers in maize–soya diets that were low in either Ca or P. As shown in Table 6, the overall influence of 600 FTU A. niger-phytase/kg on digestibility of essential amino acids was negligible, with an average response of 0·3%. However, the minimum to maximum responses ranged from − 5·1 to +5·0% across the six categories of sex and diet type. Amino acid digestibilities were determined at day 28 and feed intakes to day 19 were recorded. Feed intakes of female chicks offered low-P diets remained unaltered (+0·2%) following phytase supplementation; in contrast, phytase increased feed consumption of the male counterparts by 15·0%. Remarkably, phytase increased the AID of nine amino acids by an average of 4·8% in female chicks but in the male chicks with increased feed consumption phytase reduced amino acid digestibility by 4·9%. There is an overall negative correlation (r − 0·832; P < 0·05) between phytase-induced percentage increases in feed intake and percentage responses in amino acid digestibility.
Table 6 Responses in the apparent ileal digestibility of essential amino acids to microbial phytase in male and female chicks offered diets with differing calcium and phosphorus levels in relation to feed intake rates*
* Adapted from Sebastian et al. (Reference Sebastian, Touchburn and Chavez129).
In addition, Yi et al. (Reference Yi, Kornegay and Denbow130) reported a similar pattern of results in turkey poults in which maize–soya diets with differing levels of non-phytate P and crude protein were supplemented with 750 FTU A. niger-phytase/kg. Overall, phytase increased feed intake by 6·1%, but intakes of poults offered the high-non-phytate P/low-crude protein diet were not altered (–0·2%). Although differences were subtle, phytase-induced numerical increases in the AID of amino acids were most evident in this treatment group, with an average increase of 2·7% for nine essential amino acids. In the remaining three treatment groups, phytase increased feed intakes by an average of 8·2%, but AID coefficients varied by only 0·8%. So, there is the distinct possibility that phytase-induced variation in feed intakes/gut passage rates is a confounding factor in amino acid digestibility assays, perhaps particularly those involving chromic oxide, as was the case in the two studies discussed.
Phytase amino acid digestibility assays in pigs
There are two key reports where the impact of phytase was clearly positive in grower and finisher pigs; however, they were not published in peer-reviewed journals. Firstly, Officer & Batterham(Reference Officer and Batterham131, Reference Officer and Batterham132) found that 1000 FTU A. niger-phytase/kg substantially increased the AID coefficients of ten amino acids in diets for grower pigs in which Linola meal, a variant of linseed meal, was the only protein source. In this study, phytase increased average amino acid AID coefficients by 14·0% (0·715 v. 0·627), which ranged from 5·6% (methionine) to 24·0% (threonine) for individual amino acids.
Second, Kornegay et al. (Reference Kornegay, Radcliffe and Zhang133) completed an instructive experiment in which ileal digesta samples were taken from both intact and cannulated finisher pigs offered low-protein diets. In cannulated pigs, 500 FTU A. niger-phytase/kg increased the average AID coefficients of seventeen amino acids by 3·7% (0·779 v. 0·751); in contrast, phytase increased AID coefficients by 9·8% (0·810 v. 0·738) in intact pigs. Further, phytase increased threonine digestibility by 16·2% in intact pigs, as opposed to 6·1% in cannulated pigs. Responses to phytase in the majority of amino acid digestibility assays completed in cannulated pigs, which are often weaners, are marginal(Reference Selle and Ravindran119) and generally less than those recorded by Kornegay et al. (Reference Kornegay, Radcliffe and Zhang133) A recent study in cannulated grower pigs by Zeng et al. (Reference Zeng, Piao and Wang134) is an exception, as these workers reported that 1000 FTU phytase/kg increased the average AID coefficients of eighteen amino acids by 6·2% (0·854 v. 0·804), with individual responses ranging from 1·3% (arginine) to 13·3% (glycine). It seems that more pronounced phytase responses have been recorded in grower–finisher pigs(Reference Officer and Batterham131–Reference Zeng, Piao and Wang134) than in weaners irrespective of the method of ileal digesta collection. These relatively pronounced responses may stem from lower gastric pH in older pigs promoting more intense binary protein–phytate complex formation.
Nearly all phytase–amino acid digestibility assays in pigs, including the studies discussed, have used chromic oxide as the marker. However, Kiarie et al. (Reference Kiarie, Owusu-Asiedu and Simmins135) used acid-insoluble ash in a cannulated study where 700 FTU E. coli-phytase/kg increased the average AID coefficient of nine essential amino acids by 3·6% from 0·687 to 0·712. Nitrayova et al. (Reference Nitrayova, Patras and Brestensky136) included both chromic oxide (3 g/kg) and acid-insoluble ash (Celite at 10 g/kg) in swine diets based on maize, barley and soyabean meal to evaluate a P. lycii-phytase in cannulated pigs. The responses to phytase did not differ greatly depending on the marker used, and the researchers concluded that marker selection is not the main factor for the ambiguous results recorded in the literature. However, marker selection may be more important in broiler assays than in pigs; a contributing factor could be the reverse peristalsis that takes place in the avian gut(Reference Sacrane, Iji and Millelsen137).
There is a need to establish the validity of the proposal that responses to phytase are more reliable when ileal digesta samples are taken from intact rather than cannulated animals and several factors that may be contributing to this apparent difference(Reference Selle and Ravindran119). The fact that cannulated pigs are usually fed twice daily on a restricted basis is at odds with practical, ad libitum feeding regimens. However, the intervention of cannulation procedures probably leads to a proliferation of amino acids of microfloral origin in the terminal ileum(Reference Rowan, Moughan and Wilson138) and the reduced motility of a surgically disrupted small intestine probably promotes this microbial proliferation(Reference Easter and Tanksley139). The protein of microbial origin in the ileum of pigs is rich in glutamic acid and aspartic acid but contains relatively low levels of methionine, cystine and histidine(Reference Miner-Williams, Moughan and Fuller140). Importantly, Brand et al. (Reference Brand, Badenhorst and Siebrits141) found that when offered protein-free diets, pigs that had undergone an ileo-rectal anastomosis had twice the endogenous protein flow (12·1 v. 5·8 g/d) in comparison with intact pigs. The surplus of amino acids of microfloral origin in the ileum of cannulated pigs may mask any phytase-induced increases in digestibility of dietary and endogenous amino acids.
From the Kornegay et al. (Reference Kornegay, Radcliffe and Zhang133) experiment, it is possible to quantity the ileal digestible amino acids generated by phytase in either cannulated or intact pigs and the difference in amounts. It is then possible to compare the differences with the amino acid profile of gut microbial protein(Reference Miner-Williams, Moughan and Fuller140), as shown in Table 7. There is a significant, positive correlation between the amino acid profile of microbial protein and the difference in amino acids generated by phytase in intact and cannulated pigs (r 0·514; P < 0·05). The abundant amino acids in gut microbial protein are also the amino acids for which the most pronounced differences in phytase responses were recorded between intact and cannulated pigs. This supports the contention that a proliferation of amino acids of gut microbial origin in the ileum of cannulated pigs may be masking the positive impact of phytase on the digestibility of dietary and endogenous amino acids.
Table 7 Quantity of ileal digestible amino acids generated by 500 phytase units Aspergillus niger-phytase/kg as determined in cannulated or intact pigs*
* Adapted from Kornegay et al. (Reference Kornegay, Radcliffe and Zhang133) and Miner-Williams et al. (Reference Miner-Williams, Moughan and Fuller140).
The ‘protein effect’ of phytase
Overall, the outcomes of phytase amino acid digestibility in pigs and poultry are conflicting and inconclusive. However, to support the contention that phytase has a positive impact on digestibility of amino acids, attention is drawn to two broiler studies. In the first study, Newkirk & Classen(Reference Newkirk and Classen142) incorporated rapeseed meal at 300 g/kg into maize–soya broiler diets that had been untreated, dephytinised or sham-treated. The average AID coefficient of seventeen amino acids in diets containing dephytinised rapeseed meal (0·725) was 11·9% greater than in diets containing sham-treated rapeseed meal (0·648) despite the fact that approximately only half the total dietary protein was derived from rapeseed meal. Presumably, the increase in amino acid digestibility would have been more pronounced had phytate also been removed from soyabean meal and maize to render a ‘phytate-free’ diet.
In the second study, Selle et al. (Reference Selle, Ravindran and Ravindran143) offered broilers diets containing lysine at either 10·0 or 11·8 g/kg, without or with 500 FTU A. niger-phytase/kg, from 7 to 28 d post-hatch. Both additional lysine and phytase increased (P < 0·001) weight gain by 7·22 and 3·37%, respectively. However, there was a significant (P < 0·05) phytase × lysine level interaction because the phytase response was more pronounced in lysine-deficient (5·47%) than lysine-adequate diets (1·56%). Therefore, it appears that phytase enhanced lysine bioavailability, and this effect was more evident in lysine-deficient diets. Surprisingly, however, significant phytase × lysine interactions (P < 0·05) were observed for the ileal digestibility of seven of the sixteen amino acids assessed including lysine; phytase increased the AID of lysine by 3·7% in deficient diets but by 2·7% in adequate diets. Lysine enrichment of broiler diets has been shown to up-regulate lysine transport across jejunal brush-border membranes(Reference Torras-Llort, Soriano-García and Ferrer144). It is possible that the phytase–lysine interactions in the digestibility of amino acids indicate that both phytase and lysine were having an impact on intestinal uptake rates of lysine and certain other amino acids.
Conceptual framework for protein–phytate interactions
Protein–phytate interactions contribute to the anti-nutritive properties of phytate in pig and poultry diets. These interactions may result in the formation of primary or ternary complexes depending on the isoelectric point of protein and the prevailing pH along the gut. Binary protein–phytate complexes are formed below protein isoelectric points by electrostatic attractions between polyanionic phytate molecules and proteins carrying a net positive charge. Above their isoelectric points, proteins carrying a positive charge are linked with phytate by divalent cationic bridges to form ternary protein–phytate complexes. Additionally, according to the Hofmeister series, phytate is a strong kosmotropic anion as it possesses up to six HPO42– moieties and can stabilise protein by making an impact on the surrounding water medium. In general terms, the likelihood is that these direct and indirect reductions in protein solubility induced by phytate depress protein utilisation. More specifically, protein bound in binary complexes is refractory to pepsin digestion at very low pH in the stomach, which interferes with the initiation of the protein digestive process, and while binary complexes dissociate at the protein isoelectric point they still may not be as readily digested in the small intestine due to structural changes induced by aggregation with phytate. Pepsin-refractory binary complexes may trigger both compensatory gastric hypersecretions and protective mucin outputs, which would increase endogenous amino acid flows. Phytate induces a marked transition of Na into the gut lumen, perhaps primarily as NaHCO3 to buffer HCl. However, this movement of Na into the gut lumen may reduce intestinal uptakes of dietary and endogenous amino acids by compromising Na-dependent transport systems and Na pump activity. Because of the relatively high isoelectric point of proteins in cereal grains, binary complexes may persist in the small intestine and binary and ternary interactions between phytate and proteins closely associated with starch granules in cereal grains may depress energy utilisation. The molecular weight of protein fractions, particularly in the proximal small intestine, may be sufficiently large to permit phytate to bind nutritionally important quantities of protein in ternary complexes and this would also hinder absorption of key minerals including Ca and Zn.
Future research
With emphasis on recent findings, the present review endeavours to provide a unified framework of the mechanisms underlying protein–phytate interactions and their nutritional consequences and to explain the ambiguous effects of phytase on amino acid digestibility. The capacity of phytate to interact with protein per se and with protein closely associated with other nutrients, including starch, appears to be pivotal. The possibility that phytate indirectly interacts with protein because it is a strong kosmotropic anion is a new concept that demands further investigation and perhaps a reassessment of binary and ternary complex formation in relation to protein–phytate interactions. The apparently differing propensities of proteins to be bound by phytate merit examination. Attention should be paid to the proposal that binary protein–phytate interactions reduce pepsin digestibility of aggregated protein, which in turn triggers gastric hypersecretion of pepsin and HCl coupled with increased protective outputs of mucin and NaHCO3. Investigations should also focus on the impact of phytate and phytase on the absorption kinetics of glucose and amino acids along the small intestine, given the likelihood that phytate-induced endogenous depletions of Na may compromise Na+-dependent transport systems and Na+-K+-ATPase activity. It even may be that phytate has a direct, negative impact on the Na pump and this possibility merits investigation. While the evidence is not conclusive, it is our contention that dietary phytate negatively influences protein and energy utilisation, probably to a greater extent in poultry than pigs. Ideally, the issues discussed in relation to the divergent outcomes of phytase amino acid digestibility assays in pigs and poultry should be clarified. The adoption of these recommendations should permit greater advantage to be taken of the ‘extra-phosphoric’ effects of exogenous phytases in respect of protein and energy utilisation in pigs and poultry, thereby facilitating more efficient and sustainable production of pig-meat, poultry-meat and eggs.
Acknowledgements
The authors do not have any conflict of interests and each of the four authors contributed to the compilation of the present review. This research did not receive specific grants from any funding agency in the public, commercial or not-for-profit sectors.
