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Peptides reproducibly released by in vivo digestion of beef meat and trout flesh in pigs

Published online by Cambridge University Press:  01 December 2007

Caroline Bauchart
Affiliation:
INRA, UMR1019 Unité de Nutrition Humaine, F-63122St Genès Champanelle, France INRA, UR370 Qualité des Produits Animaux, F-63122St Genès Champanelle, France
Martine Morzel
Affiliation:
INRA, UR370 Qualité des Produits Animaux, F-63122St Genès Champanelle, France
Christophe Chambon
Affiliation:
INRA, UR370 Qualité des Produits Animaux, F-63122St Genès Champanelle, France
Philippe Patureau Mirand
Affiliation:
INRA, UMR1019 Unité de Nutrition Humaine, F-63122St Genès Champanelle, France
Christelle Reynès
Affiliation:
Laboratoire de Physique Moléculaire et Structurale, Faculté de Pharmacie, F-34060Montpellier, France
Caroline Buffière
Affiliation:
INRA, UMR1019 Unité de Nutrition Humaine, F-63122St Genès Champanelle, France
Didier Rémond*
Affiliation:
INRA, UMR1019 Unité de Nutrition Humaine, F-63122St Genès Champanelle, France
*
*Corresponding author: Dr Didier Rémond, fax +33 4 73 62 47 55, email [email protected]
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Abstract

Characterisation and identification of peptides (800 to 5000 Da) generated by intestinal digestion of fish or meat were performed using MS analyses (matrix-assisted laser desorption ionisation time of flight and nano-liquid chromatography electrospray-ionisation ion trap MS/MS). Four pigs fitted with cannulas at the duodenum and jejunum received a meal exclusively made of cooked Pectoralis profundus beef meat or cooked trout fillets. A protein-free meal, made of free amino acids, starch and fat, was used to identify peptides of endogenous origin. Peptides reproducibly detected in digesta (i.e. from at least three pigs) were evidenced predominantly in the first 3 h after the meal. In the duodenum, most of the fish- and meat-derived peptides were characteristic of a peptic digestion. In the jejunum, the majority of peptides appeared to result from digestion by chymotrypsin and trypsin. Despite slight differences in gastric emptying kinetics and overall peptide production, possibly in relation to food structure and texture, six and four similar peptides were released after ingestion of fish or meat in the duodenum and jejunum. A total of twenty-six different peptides were identified in digesta. All were fragments of major structural (actin, myosin) or sarcoplasmic (creatine kinase, glyceraldehyde-3-phosphate dehydrogenase and myoglobin) muscle proteins. Peptides were short ( < 2000 Da) and particularly rich in proline residues. Nineteen of them contained bioactive sequences corresponding mainly to an antihypertensive activity. The present work showed that after fish or meat ingestion, among the wide variety of peptides produced by enzymic digestion, some of them can be reproducibly observed in intestinal digesta.

Type
Full Papers
Copyright
Copyright © The Authors 2007

The concept of food-derived peptides possessing biological activity, or bioactive peptides, brings a completely new dimension that should be considered in the description of dietary protein quality. Bioactive peptides have been defined as protein fragments with specific sequences that have, in addition to their nutritional value, a positive impact on body functions and may ultimately influence healthReference Kitts and Weiler1. Once liberated in the body, they can exert different beneficial effects such as antihypertensive, antithrombotic, opioid, immunomodulating, antimicrobial and antioxidant activitiesReference Kitts and Weiler1, Reference Korhonen and Pihlanto2. Most dietary proteins contain bioactive sequences, but the corresponding peptides need to be released by proteolysis, during food processing or gastrointestinal digestion, in order to show a biological activity.

Many bioactive peptides have been identified in milk productsReference Clare and Swaisgood3, Reference Rutherfurd-Markwick and Moughan4; in comparison, less information is available for meat and fish products. Such products may nonetheless represent a valuable source of peptides with biological activitiesReference Arihara, Nollet and Toldrá5, Reference Vercruysse, Van Camp and Smagghe6. For example, two angiotensin-converting enzyme (ACE) inhibitory peptides, obtained by in vitro thermolysin digestion of porcine skeletal muscleReference Arihara, Nakashima, Mukai, Ishikawa and Itoh7, were shown to have an in vivo antihypertensive activity when administered orally to spontaneously hypertensive ratsReference Nakashima, Arihara, Sasaki, Mio, Ishikawa and Itoh8. However, there is evidence that peptides produced by in vitro digestion yield different peptides compared with those generated in vivo. For example, β-casomorphin fragments isolated from intestinal contents following ingestion of caseinReference Meisel9 are larger fragments than those found in in vitro digesta. To our knowledge, studies on the occurrence of bioactive peptides in digesta after ingestion of meat or fish have not been reported. More generally, and despite the central role of digestive events in the supply of nutrients or biologically active compounds to the organism, almost no information is available on peptides resulting from in vivo digestion of meat or fish, in particular their sizes and sequences, let alone the random or reproducible manner in which they are generated.

In this context, and following description of peptides present in ready-to-eat beef meat or troutReference Bauchart, Rémond, Chambon, Patureau Mirand, Savary-Auzeloux, Reynès and Morzel10, Reference Bauchart, Chambon, Patureau Mirand, Savary-Auzeloux, Rémond and Morzel11, the present study aimed at characterising and identifying peptides ( < 5 kDa) generated by intestinal digestion of such food products, using the pig as an animal model for man.

Materials and methods

Animals

The study involved four 3-month-old female pigs (40·5 (sd 5·2) kg). At 3 weeks before the experimentation, pigs were surgically fitted with T-shaped cannulas (silicone rubber; 12 mm internal diameter, 17 mm outer diameter) in the duodenum (10 cm downstream from the pylorus) and the mid-jejunum (about 4 m downstream from the pylorus), and a catheter (polyvinyl chloride; 1·1 mm internal diameter, 1·9 mm outer diameter) in the cava vein. Surgical procedures and post-surgical care were conducted in accordance with national legislation on the care and use of laboratory animals. Pigs were housed in individual pens (1 × 1·5 m) in a ventilated room with controlled temperature (19–23°C). They were given 800 g/d of a concentrate feed containing 18 % protein, 2 % fat, 5 % cellulose and 6 % ash (Porcyprima; Sanders Centre Auvergne, Aigueperse, France) distributed in two equal portions at 8.00 and 16.00 hours, and had free access to water. The daily ration was adjusted to cover 150 % of the maintenance requirementsReference Sève12.

Test meals

Three types of foods (beef, trout, protein-free food) were prepared. Beef meat was Pectoralis profundus from a 15-month-old Charolais bull, aged for 14 d, and cooked under vacuum for 90 min at 75°C in a water-bath. Trout was the dorsal part of rainbow trout (Oncorhynchus mykiss) fillets, stored for 7 d on ice, and cooked under-vacuum for 5 min at 70°C in a water-bath. Both types of muscle foods were frozen at − 20°C until use. The protein-free food, used for the purpose of monitoring the endogenous peptide composition of digesta in a postprandial situation, was made of 47 % free amino acids (in proportion close to the amino acid composition of muscle), 23 % wheat starch, 12 % fat and 18 % water. Each test meal provided 40 g crude protein, or the equivalent in amino acids, and was exclusively made of either beef (115 g; 44 g DM), trout (174 g; 44 g DM) or the control protein-free food mixture (85 g; 75 g DM). Meals were offered for 15 min and were always consumed entirely within that time.

Experimental procedures

The three types of foods were tested on each animal. Test meals were separated by at least 2 d. Duodenum and jejunum digesta sampling was performed on two distinct test meals. The test meal was given at 09.00 hours. Digesta were continuously collected from 08.00 to 15.00 hours in cold plastic bottles replaced each hour. Water intake was restricted to 250 ml/h. To prevent dehydration, 1 litre Ringer-lactate solution was intravenously infused at a rate of 150 ml/h throughout the sampling session.

Hourly collected digesta were immediately homogenised in a Waring Blender (VWR International SAS, Fontenay-sous-Bois, France) (twice 5 s at high speed, separated by 5 s). A first fraction of the homogenate (about 10 g) was used for DM determination (24 h at 104°C). A second fraction (about 100 g) was treated with perchloric acid at 170 mm (final concentration). After vigorous shaking, samples were kept on ice for 15 min, and then centrifuged at 10 000 g for 20 min at 4°C. For the postprandial period, fractions of supernatant fractions (2 % of hourly collected digesta) were pooled to yield two samples per animal: a first pool representative of the 3 h following the meal (PP1), and a second one representative of the period spanning from 3 to 6 h after the meal (PP2). Post-absorptive (sample collected before the meal), PP1 and PP2 supernatant fractions were filtered through 5000 Da cut-off filters (Vivaspin 15; Vivascience, Hanover, Germany) at 2000 g for 8 to 15 h at 4°C. Filtrates were stored at − 80°C until analysis.

Analytical methods

Chromatographic analysis of peptides in extracts was carried out using an HPLC system (Kontron Instruments, Bletchley, Bucks, UK). Separation was done in a Nucleodur® C18 pyramid (110 Å; 4·6 × 250 mm) with 5 μm particles (Macherey-Nagel, Düren, Germany) at 30°C in a column oven and at a flow rate of 0·9 ml/min. The gradient was performed using two solvents (A, 0·1 % trifluoroacetic acid in water; B, 0·1 % trifluoroacetic acid in 100 % acetonitrile) and formed as follows: 0 % B up to 5 min, 0–60 % B in 5–35 min and 60–100 % B in 35–38 min. Detection of peptide bonds was done at 220 nm.

Matrix-assisted laser desorption ionisation time-of-flight (MALDI-ToF) analysis and nano-liquid chromatography electrospray-ionisation ion trap MS/MS (nano-LC-ESI-IT MS/MS) analysis were performed as previously described by Bauchart et al. Reference Bauchart, Rémond, Chambon, Patureau Mirand, Savary-Auzeloux, Reynès and Morzel10. For MALDI-ToF analysis, masses were recorded in the m/z range 800 to 5000. Below 800, m/z may not be reliably monitored by MALDI-ToF because of interference with matrix-generated peaks.

Statistical analyses

DM flux, at each site, during the first 3 h after feeding (PP1) was examined by a two-way randomised-block ANOVA with food as factor and animal as block using SAS version 8.10 (SAS Institute Inc., Cary, NC, USA).

A statistical procedure, previously describedReference Bauchart, Rémond, Chambon, Patureau Mirand, Savary-Auzeloux, Reynès and Morzel10, was applied to MALDI-ToF data to determine whether peaks, at close m/z but originating from different spectra, were likely to correspond to the same compound. For one type of food and one sampling time (PP1, PP2), only the peaks gathered in a group consisting of data originating from at least three animals were considered. A similar procedure was subsequently applied to determine which groups of peaks corresponded to the same compound, across sampling times.

Results

Intestinal transit kinetics

DM collected at the duodenum after ingestion of protein-free food, trout or beef during the three first 3 h after feeding (PP1) accounted for 88·5 (sd 4·0), 90 (sd 1·2) and 74 (sd 10·2) % of the total DM collected in the whole postprandial period (data not shown). This proportion was lower for beef than for protein-free food and trout (P < 0·05). At the jejunum level, the proportion of DM collected in PP1 was not affected by test-meal composition, and averaged 77 (sd 14) % (data not shown).

Chromatographic profiles of digesta

Reverse-phase HPLC analysis of digesta extracts collected after the ingestion of protein-free food (Fig. 1(a) and (b)) revealed the presence of numerous endogenous peptides. Chromatographic profiles showed very few qualitative differences between duodenum and jejunum, with common peaks at retention times of about 5·0, 6·2, 8·3, 9·9, 15·3, 18·0, 19·5, 21·3, 23·4, 23·9, 24·2, 24·5, 24·9 and 27·4 min. These endogenous peptides were still observed after ingestion of trout (Fig. 1(c) and (d)) or beef (Fig. 1(e) and (f)) but in addition, absorbance at 220 nm globally increased across the retention times 15 to 25 min. This increase was more prominent for jejunum digesta than for duodenum digesta, and generally larger after a meal of trout than after a meal of beef.

Fig. 1 Reverse-phase HPLC chromatograms of digesta extracts from the duodenum (a, c and e) and the jejunum (b, d and f) collected in one pig over the first 3 h following ingestion of control protein-free food (a and b), trout (c and d) and beef (e and f).

Peptides evidenced by matrix-assisted laser desorption ionisation time of flight analysis

Although peptides up to 5000 Da should be extracted by the procedure we used (perchloric acid precipitation of proteins and ultrafiltration), MALDI-ToF analysis evidenced very few compounds between 2000 and 5000 m/z in the digesta (Fig. 2). Masses of peptides detected by MALDI-ToF in at least three of the four pigs (later called ‘reproducibly’ detected) in digesta extracts after ingestion of beef or trout are listed in Table 1. All endogenous compounds, i.e. detected at least once in the intestinal contents of the post-absorptive period or after a protein-free meal, were removed from the list in order to retain only peptides of an alimentary origin. The time of sampling had a major effect on the number of reproducibly detected peptides, since in the second 3 h period after the meal (PP2) only one peptide (m/z 1018·50) was listed, in the duodenum after ingestion of beef. Compounds listed in PP1 were more numerous in the duodenum than in jejunum (eight and seven for trout; nine and five for beef). Some food-derived peptides were common to the duodenum and jejunum digesta, four for trout (m/z 1115·89, 1148·44, 1182·44 and 1434·17) and two for beef (m/z 1115·89 and 1198·75). In PP1, there was a striking similarity in the masses of peptides reproducibly generated by digestion of either trout or beef. At the duodenum level, out of eight and nine reproducibly detected peptides, seven were common to trout and beef. At the jejunum level, five were common to trout and beef out of seven and five.

Fig. 2 Representative matrix-assisted laser desorption ionisation time of flight spectra of duodenum (a and c) and jejunum (b and d) digesta collected from one pig during the first 3 h after ingestion of cooked trout flesh (a and b) or cooked beef Pectoralis profundus (c and d).

Table 1 List of compounds (m/z 800 to 5000) detected by matrix-assisted laser desorption ionisation time of flight analysis in pig duodenum and jejunum digesta, collected during the first 3 h (PP1) and the subsequent 3 h (PP2) after ingestion of trout or beef*

* Listed compounds had an alimentary origin and were found in at least three of the four animals.

Identification of reproducibly generated food-derived peptides

Fish- and meat-derived peptides identified by nano-LC-ESI-IT MS/MS analysis in digesta extracts collected over PP1 are listed in Table 2. The identified peptides came from abundant muscle proteins, namely actin, myosins, creatine kinase and glyceraldehyde 3-phosphate dehydrogenase, and myoglobin specifically for beef. Again, there were some similarities between the intestinal contents after a meal of trout or beef, with six and four food-derived peptides common to the two types of muscle foods in the duodenum and jejunum, respectively. Overall, a particularity of the sequences was the high proportion of proline, accounting for approximately 12·0 % (fifteen of 125) and 13·1 % (fourteen of 107) of all residues in peptides identified at the duodenum level for trout and beef, respectively. At the jejunum level, the proportion was even higher and reached 15·0 % (twelve of eighty) and 19 % (eleven of fifty-eight) for trout and beef, respectively. After the protein-free meal (data not shown) several fragments of pepsin A, trypsin precursor, pancreatic α-amylase and salivary proline-rich proteins were identified in duodenum digesta. Fragments of trypsin (IKLSSPATL and LIKLSSPATL) and salivary proline-rich protein (ARPLPGPPPPGPPP) were common to duodenum and jejunum digesta. The jejunum content was also characterised by the presence of many more fragments of salivary proline-rich proteins.

Table 2 Peptides identified by nano-liquid chromatography-ion trap tandem mass spectrometry in duodenum and jejunum digesta extracts collected in pigs over the first 3 h following ingestion of trout or beef*

GA3PDH, glyceraldehyde 3-phosphate dehydrogenase.

* Peptides were identified by searching the National Center for Biotechnology Information nr protein database. Listed peptides had an alimentary origin and were found in at least three of the four animals.

A search of potential biological activity of identified peptides was carried out with the BioPep databaseReference Dziuba, Minkiewicz, Nalecz and Iwaniak13 and by comparison with sequences either reviewed in Vercruysse et al. Reference Vercruysse, Van Camp and Smagghe6 or described in Sentandreu & ToldráReference Sentandreu and Toldrá14. Some sequences with potential biological activity were found within nineteen of the identified peptide sequences (Table 3). They were mainly short sequences of two or three residues, except for the sequences IVGRPR, YALPHA and ALPHA, all contained in actin fragments. The most frequently found potential biological activity was an antihypertensive effect.

Table 3 Bioactive sequences contained within peptides identified in digesta in the first 3 h following ingestion of beef or trout

Discussion

The present study intended to characterise and identify peptides reproducibly generated by in vivo gastroduodenal digestion of fish or meat, focusing on peptides ranging from 800 to 5000 Da. The lower limit was dictated by technical considerations while the upper limit was chosen in relation to the generally reported size of bioactive peptides. Overall, we have identified nineteen and fifteen different food-derived peptides in digestive contents of pigs after a meal of fish or beef, respectively. Many of the identified peptides contained bioactive sequences.

DM flux measured at the duodenal level illustrates the rapidity of gastric emptying after the meal, even more for trout than for beef. Food texture has been recognised as a factor influencing gastric emptyingReference Santangelo, Perrachi, Conte, Fraquelli and Porrini15. Here, in the cooking conditions used for beef, meat was dry and compact. The looser structure and moister texture of trout is a plausible explanation for the accelerated kinetics. Compositional factors, in particular the high proportion of n-3 PUFA in trout, may also contribute to a faster gastric emptying as described by Robertson et al. Reference Robertson, Jackson, Fielding, Morgan, Williams and Frayn16. Values in the jejunum also evidence that transit throughout the anterior intestine proceeded rapidly.

After a meal of fish or meat, only one peptide was reproducibly detected in PP2 digesta, suggesting that peptides earlier generated by digestion were rapidly further processed by transformation or absorption. For these reasons, peptide identification was limited to samples collected in the first 3 h following the meal. Based on masses of peptides present in the two types of muscle foods constituting the mealsReference Bauchart, Rémond, Chambon, Patureau Mirand, Savary-Auzeloux, Reynès and Morzel10, Reference Bauchart, Chambon, Patureau Mirand, Savary-Auzeloux, Rémond and Morzel11, it appears that none of those dietary oligopeptides were found in digesta. This suggests that food-borne peptides were either degraded and/or that they were present in too low quantity to be detected. The latter is supported by the complex chromatographic profiles of digesta compared with the MS results, suggesting that only a fraction of the peptides was characterised and identified. It can reasonably be assumed that, within the size range studied, the identified peptides were those most important quantitatively, which is further reinforced by the fact that all identified peptides were fragments of abundant muscle proteins. Therefore, the relative contribution of peptides brought directly as constituents of cooked fish or meat to the peptide composition in digesta is likely to be very limited.

The size characteristics and identification of reproducibly detected peptides provided several types of information on digestive events and peptide release in digesta. First, a noteworthy characteristic of the detected peptides was their relatively small size, as indicated by MALDI-ToF spectra where very few compounds at m/z>2000 were found. Data on the size of peptides generated in vivo during digestion of proteins by gastric or intestinal enzymes are scarce. In human subjects, several peptides of six to twelve amino acids were identified in the stomach and in the duodenum after ingestion of milk or yogurtReference Chabance, Marteau, Rambaud, Migliore-Samour, Boynard, Perrotin, Guillet, Jolles and Fiat17. This peptide length corresponds well to sizes we observed. In an in vitro study focusing on bonito muscle treated by artificial gastric juiceReference Hasan, Kitagawa, Kumada, Hashimoto, Shiiba, Katoh and Terashima18, all proteins were converted into peptides ( < 10 kDa) after 5 min. Some peptides were identified in samples collected after 1 h of artificial digestion and, again, their lengths (eight to fifteen amino acids) were consistent with sizes we observed in vivo. In both studies, the analytical procedure involved separation of compounds by reverse-phase HPLC, which might create a bias in the size of separated and identified peptides. Nevertheless, the present results corroborate that, in the molecular weight range 0–5 kDa, mainly short peptides were released by digestive proteolytic enzymes. In other words, the first steps of protein intestinal digestion were fast and efficient enough to prevent accumulation of intermediary degradation products.

Another indication on digestive proteolytic functions resides in the number of reproducibly detected peptides. The larger number in duodenum digesta, i.e. after gastric digestion mainly performed by pepsin, results most probably from a more homogeneous digestion process. In the jejunum, where also several pancreatic enzymes intervene, the chromatographic profiles suggest that more peptides were produced, but the shorter list of reproducible peptides indicates a higher composition diversity.

Peptides identified in duodenum digesta were characteristic of pepsin hydrolysis: when combining results for trout and beef, out of eighteen different peptides, twelve possessed an N-terminal Y, F or L and nine peptides possessed a C-terminal residue M, F, or L, the most frequent amino acids after digestion by pepsinReference Kageyama19. In the luminal phase of the small intestine, products of peptic degradation are further cleaved by pancreatic proteases (trypsin, α-chymotrypsin, elastase and carboxypeptidase A and B) at more alkaline pH. We confirmed in the present study that reproducibly detected peptides in the jejunum were a mixture of peptides generated upstream and withstanding proteolysis entirely (for example, FRVPTPNVSV) or partly (for example, LFDKPVSPL, most probably issued from LFDKPVSPLL), and of newly generated peptides. Excluding FRVPTPNVSV which was not affected by pancreatic enzymes, out of nine peptides, three had a C-terminal leucine which is characteristics of hydrolysis by porcine chymotrypsin CReference Folk and Schirmer20 and four had a C-terminal arginine which is characteristics of tryptic hydrolysisReference Gray and Cooper21.

More generally, detected or identified peptides were probably among the most resistant to proteolysis. This is supported by the high proportion of proline in their sequences. Proline-containing peptides were reported to be generally resistant to degradation by digestive enzymesReference Hausch, Shan, Santiago, Gray and Khosla22Reference Vanhoof, Goosens, De Meester, Hendriks and Scharpé24. Accordingly, the proportion of proline in identified peptides was well above the average abundance in fish or meat proteinsReference Sosulski and Imafidon25.

Finally, the last information drawn from characterisation of peptides in digesta after a meal of trout or beef is a certain similarity regarding peptides release (six and four common peptides in the duodenum and jejunum, respectively). This is all the more remarkable since the two types of foods were chosen and prepared especially to show large differences in terms of collagen content, texture, structure etc. The difference between the two types of foods concerned the quantity of peptides released, which seemed slightly higher for trout as indicated by all methods, reverse-phase HPLC, MALDI-ToF and nano-LC-ESI-IT MS/MS. Similarly to DM flux, the difference between the two types of foods may be linked to the looser structure of trout, improving accessibility of proteolytic enzymes to their targets. However, resemblance in peptide release was in line with the previously mentioned efficiency of the digestive hydrolytic systems, able to some extent to function similarly on foods of different structures.

Most of bioactive sequences found within detected peptides in digesta corresponded to antihypertensive activity. Many muscle-derived ACE inhibitory peptides have been described. For example, LKPNM has been identified as an ACE inhibitor in thermolysin-digested dried bonitoReference Fujita and Yoshikawa26. Katayama et al. Reference Katayama, Tomatsu, Fuchu, Sugiyama, Kawahara, Yamaguchi, Kawamura and Muguruma27 isolated an ACE inhibitory peptide (RMLGQTPTK) from porcine troponin C hydrolysed with pepsin. In thermolysin digest of porcine skeletal muscle, Arihara et al. Reference Arihara, Nakashima, Mukai, Ishikawa and Itoh7 evidenced two myosin heavy chain fragments (MNPPK and ITTNP) with ACE inhibitory activity. More recently, Jang & LeeReference Jang and Lee28 purified an ACE inhibitory peptide (VLAQYK) from the hydrolysate of sarcoplasmic protein extracts from beef rump by using the combination of proteinases A and thermolysin. None of these fragments were identified in the digesta in the present study. Nevertheless, out of twenty-six identified peptides, nineteen contained sequences with potential bioactivity. ACE inhibitory sequences may be released by peptidases associated with the brush-border membrane of the enterocytes or to intracellular peptidasesReference Vermeirssen, Van Camp and Verstraete29. Under these conditions, our findings would confirm a previous suggestion that ACE inhibitory peptides may be generated in the gastrointestinal tract after ingestion of muscle foodsReference Arihara, Nakashima, Mukai, Ishikawa and Itoh7. To exert their biological activity, the ACE inhibitory peptides contained within oligopeptides we have described also have to reach the bloodstream. The possibility of absorption into the circulatory blood system of an antihypertensive dipeptide has been demonstrated in human subjectsReference Matsui, Tamaya, Seki, Osajima, Matsumoto and Kawasaki30. For larger peptides, although mechanisms of absorption have not been thoroughly studied, an ultimate impact on blood pressure has been demonstrated after oral administration to spontaneously hypertensive rats. This applies, for example, to peptides derived from porcine skeletal muscle myosinReference Nakashima, Arihara, Sasaki, Mio, Ishikawa and Itoh8 or to the bonito-derived peptide LKPNMReference Fujita, Yamagami and Ohshima31.

In conclusion, the present study showed that after fish or meat ingestion, among the wide range of peptides produced by enzymic digestion, some of them can be reproducibly observed in intestinal digesta. Some peptides have been shown to have a local action in the intestineReference Korhonen and Pihlanto2. However, the biological activity of peptides is generally peripheral, thereby implying peptide absorption. Although absorption has been occasionally proven for particular peptides, this topic deserves further studies.

Acknowledgements

The authors thank D. Durand for surgical preparation of the animals, and C. Lafarge for animal care.

References

1Kitts, DD & Weiler, K (2003) Bioactive proteins and peptides from food sources. Applications of bioprocesses used in isolation and recovery. Curr Pharm Des 9, 13091323.CrossRefGoogle ScholarPubMed
2Korhonen, H & Pihlanto, A (2006) Bioactive peptides: production and functionality. Int Dairy J 16, 945960.CrossRefGoogle Scholar
3Clare, DA & Swaisgood, HE (2000) Bioactive milk peptides: a prospectus. J Dairy Sci 83, 11871195.CrossRefGoogle ScholarPubMed
4Rutherfurd-Markwick, KJ & Moughan, PJ (2005) Bioactive peptides derived from food. J AOAC Int 88, 955966.CrossRefGoogle ScholarPubMed
5Arihara, K (2006) Functional properties of bioactive peptides derived from meat proteins. In Advanced Technologies for Meat Processing, pp. 245273 [Nollet, LML and Toldrá, F, editors]. New York: CRC Taylor & Francis Group.CrossRefGoogle Scholar
6Vercruysse, L, Van Camp, J & Smagghe, G (2005) ACE inhibitory peptides derived from enzymatic hydrolysates of animal muscle protein: a review. J Agric Food Chem 53, 81068115.CrossRefGoogle ScholarPubMed
7Arihara, K, Nakashima, Y, Mukai, T, Ishikawa, S & Itoh, M (2001) Peptide inhibitors for angiotensin I-converting enzyme from enzymatic hydrolysates of porcine skeletal muscle proteins. Meat Sci 57, 319324.CrossRefGoogle ScholarPubMed
8Nakashima, Y, Arihara, K, Sasaki, A, Mio, H, Ishikawa, S & Itoh, M (2002) Antihypertensive activities of peptides derived from porcine skeletal muscle myosin in spontaneously hypertensive rats. J Food Sci 67, 434437.CrossRefGoogle Scholar
9Meisel, H (1986) Chemical characterization and opioid activity of an exorphin isolated from in vivo digests of casein. FEBS Lett 196, 223227.CrossRefGoogle ScholarPubMed
10Bauchart, C, Rémond, D, Chambon, C, Patureau Mirand, P, Savary-Auzeloux, I, Reynès, C & Morzel, M (2006) Small peptides ( < 5 kDa) found in ready-to-eat beef meat. Meat Sci 74, 658666.CrossRefGoogle Scholar
11Bauchart, C, Chambon, C, Patureau Mirand, P, Savary-Auzeloux, I, Rémond, D & Morzel, M (2007) Peptides in rainbow trout (Oncorhynchus mykiss) muscle subjected to ice storage and cooking. Food Chem 100, 15661572.CrossRefGoogle Scholar
12Sève, B (1994) Alimentation du porc en croissance: intégration des concepts de protéine idéale, de disponibilité digestive des acides aminés et d'énergie nette (Feeding of growing pigs: integration of concepts of ideal protein, of digestive availability of amino acids and of net energy). INRA Prod Anim 7, 275291.CrossRefGoogle Scholar
13Dziuba, J, Minkiewicz, P, Nalecz, D & Iwaniak, A (1999) Database of biologically active peptide sequences. Nahrung-Food 43, 190195.3.0.CO;2-A>CrossRefGoogle ScholarPubMed
14Sentandreu, MA & Toldrá, F (2007) Evaluation of ACE inhibitory activity of dipeptides generated by the action of porcine muscle dipeptidyl peptidases. Food Chem 102, 511515.CrossRefGoogle Scholar
15Santangelo, A, Perrachi, M, Conte, D, Fraquelli, M & Porrini, M (1998) Physical state of meal affects gastric emptying, cholecystokinin release and satiety. Br J Nutr 80, 521527.CrossRefGoogle ScholarPubMed
16Robertson, MD, Jackson, KG, Fielding, BA, Morgan, LM, Williams, CM & Frayn, KN (2002) Acute ingestion of a meal rich in n-3 polyunsaturated fatty acids results in rapid gastric emptying in humans. Am J Clin Nutr 46, 232238.CrossRefGoogle Scholar
17Chabance, B, Marteau, P, Rambaud, JC, Migliore-Samour, D, Boynard, M, Perrotin, P, Guillet, R, Jolles, P & Fiat, AM (1998) Casein peptide release and passage to the blood in humans during digestion of milk or yogurt. Biochimie 80, 155165.CrossRefGoogle ScholarPubMed
18Hasan, F, Kitagawa, M, Kumada, Y, Hashimoto, N, Shiiba, M, Katoh, S & Terashima, M (2006) Production kinetics of ACE inhibitory peptides from bonito meat in artificial gastric juices. Process Biochem 41, 505511.CrossRefGoogle Scholar
19Kageyama, T (2002) Pepsinogens, progastricsins, and prochymosins: structure, function, evolution, and development. Cell Mol Life Sci 59, 288306.CrossRefGoogle ScholarPubMed
20Folk, JE & Schirmer, EW (1965) Chymoptrypsin C – I. Isolation of the zymogen and the active enzyme: preliminary structure and specificity studies. J Biol Chem 240, 181192.CrossRefGoogle Scholar
21Gray, GM & Cooper, HL (1971) Protein digestion and absorption. Gastroenterology 61, 535544.CrossRefGoogle ScholarPubMed
22Hausch, F, Shan, L, Santiago, NA, Gray, GM & Khosla, C (2002) Intestinal digestive resistance of immunodominant gliadin peptides. Am J Physiol 283, G996G1003.Google ScholarPubMed
23Kaspari, A, Diefenthal, T, Grosche, G, Schierhorn, A & Demuth, HU (1996) Substrates containing phosphorylated residues adjacent to proline decrease the cleavage by proline-specific peptidases. Biochim Biophys Acta 1293, 147153.CrossRefGoogle ScholarPubMed
24Vanhoof, G, Goosens, F, De Meester, I, Hendriks, D & Scharpé, S (1995) Proline motifs in peptides and their biological processing. FASEB J 9, 736744.CrossRefGoogle ScholarPubMed
25Sosulski, FW & Imafidon, GI (1990) Amino acid composition and nitrogen-to-protein conversion factors for animal and plant foods. J Agric Food Chem 38, 13511356.CrossRefGoogle Scholar
26Fujita, H & Yoshikawa, M (1999) LKPNM: a prodrug-type ACE-inhibitory peptide derived from fish protein. Immunopharmacology 44, 123127.CrossRefGoogle ScholarPubMed
27Katayama, K, Tomatsu, M, Fuchu, H, Sugiyama, M, Kawahara, S, Yamaguchi, K, Kawamura, Y & Muguruma, M (2003) Purification and characterization of an angiotensin I-converting enzyme inhibitory peptide derived from porcine troponin C. Anim Sci J 74, 5358.CrossRefGoogle Scholar
28Jang, A & Lee, M (2005) Purification and identification of angiotensin converting enzyme inhibitory peptides from beef hydrolysates. Meat Sci 69, 653661.CrossRefGoogle ScholarPubMed
29Vermeirssen, V, Van Camp, J & Verstraete, W (2004) Bioavailability of angiotensin I converting enzyme inhibitory peptides. Br J Nutr 92, 357366.CrossRefGoogle ScholarPubMed
30Matsui, T, Tamaya, K, Seki, E, Osajima, K, Matsumoto, K & Kawasaki, T (2002) Val-Tyr as a natural antihypertensive dipeptide can be absorbed into the human circulatory blood system. Clin Exp Pharmacol Physiol 29, 204208.CrossRefGoogle ScholarPubMed
31Fujita, H, Yamagami, T & Ohshima, K (2001) Effects of an ACE-inhibitory agent, katsuobushi oligopeptide, in the spontaneously hypertensive rat and in borderline and mildly hypertensive subjects. Nutr Res 21, 11491158.CrossRefGoogle Scholar
Figure 0

Fig. 1 Reverse-phase HPLC chromatograms of digesta extracts from the duodenum (a, c and e) and the jejunum (b, d and f) collected in one pig over the first 3 h following ingestion of control protein-free food (a and b), trout (c and d) and beef (e and f).

Figure 1

Fig. 2 Representative matrix-assisted laser desorption ionisation time of flight spectra of duodenum (a and c) and jejunum (b and d) digesta collected from one pig during the first 3 h after ingestion of cooked trout flesh (a and b) or cooked beef Pectoralis profundus (c and d).

Figure 2

Table 1 List of compounds (m/z 800 to 5000) detected by matrix-assisted laser desorption ionisation time of flight analysis in pig duodenum and jejunum digesta, collected during the first 3 h (PP1) and the subsequent 3 h (PP2) after ingestion of trout or beef*

Figure 3

Table 2 Peptides identified by nano-liquid chromatography-ion trap tandem mass spectrometry in duodenum and jejunum digesta extracts collected in pigs over the first 3 h following ingestion of trout or beef*

Figure 4

Table 3 Bioactive sequences contained within peptides identified in digesta in the first 3 h following ingestion of beef or trout