ASSESSMENT OF THE HEMOAGLUTINANT AND DIGESTIVE ENZYME INHIBITORY ACTIVITY OF EXTRACTS OBTAINED FROM DIFFERENT PARTS OF ATEMOIA

Serquiz, Alexandre Coelho; Serquiz, Raphael Paschoal; Peixoto, Thayane Kerbele Oliveira das Neves; Santos, Elizeu Antunes dos; Rocha, Hugo Alexandre Oliveira

doi:10.1590/0100-29452018098

ABSTRACT

The benefits of various foods, such as fruits and vegetables, have been the focus of several studies aimed at improving welfare, health, and reducing the incidence of diseases. Therefore, the present paper objectified to investigate the presence of molecules of biotechnological and pharmacological interest in peel, seed, and pulp of Annona x atemoya Mabb. Aqueous extracts of the fruit parts were obtained with different buffers and assessed as to their protein and phenolic compounds content. The three parts of the fruit presented different proportions of these compounds when subject to different extraction conditions, with the highest concentrations of proteins being found in the seed and phenolic compounds in the peel of the studied fruit. Bioactive proteins (protease inhibitors and lectins) were detected through inhibitory tests for trypsin and chymotrypsin and hemagglutinating activity tests with human erythrocytes. A variation of 400 to 9600 inhibition units for the trypsin in the analyzed extracts, whereas for chymotrypsin a variation of 200 to 2500 in the inhibition units for the three fruit parts, considering the different extraction conditions were identified. The extracts obtained from the seeds and the peel presented titers higher than 0.9 hemagglutination units, suggesting that the by-products from the processing of A. x atemoya are potential sources of bioactive molecules.

Index terms
Annona x atemoya; residues; protease inhibitors; lectins

RESUMO

Os benefícios de diversos alimentos, como frutas e hortaliças, têm sido foco de vários estudos que visam a melhorar o bem-estar, a saúde e a reduzir a incidência de doenças. Dessa forma, no presente estudo, averiguou-se a presença de moléculas de interesse biotecnológico e farmacológico em casca, semente e polpa de Annona x atemoya Mabb. Extratos aquosos das três partes do fruto foram obtidos com diferentes tampões e avaliados quanto a seu conteúdo de proteínas e compostos fenólicos. As três partes do fruto apresentaram proporções diferentes destes compostos quando submetidos a distintas condições de extração, sendo que as maiores concentrações de proteínas foram encontradas na semente, e as de fenólicos na casca, do fruto estudado. Proteínas bioativas (inibidores de proteases e lectinas) foram detectadas por ensaios inibitórios para tripsina e quimotripsina, e ensaios de atividade hemaglutinante com eritrócitos humanos. Identificou-se variação de 400 a 9.600 unidades de inibição para a tripsina nos extratos analisados; já para a quimotripsina foi vista variação nas unidades de inibição de 200 a 2.500 unidades nas três partes do fruto e nas diferentes condições de extração. Os extratos obtidos das sementes e da casca apresentaram títulos superiores a 0,9 unidades de hemaglutinação, sugerindo que os resíduos do processamento de produtos derivados de A. x atemoya são potenciais fontes de moléculas bioativas.

Termos para indexação
Annona x atemoya; resíduos; inibidores de proteases; lectinas

Introduction

Urbanization, industrialization and globalization had great influence on the lifestyle, diet and, consequently, the nutritional status of Brazilians (TARDIDO, FALCÃO, 2006 TARDIDO, A.P.; FALCÃO, M.C. O impacto da modernização na transição nutricional e obesidade. Revista Brasileira de Nutrição Clinica, São Paulo, v.21, n.2, p.117-124, 2006. ; BRASIL, 2012 BRASIL. Ministério da Saúde. Secretaria de Atenção à Saúde. Departamento de Atenção Básica. Política nacional de alimentação e nutrição - Série B. Textos Básicos de Saúde. Brasília, DF: Ministério da Saúde, 2012. ). This influence led to a decrease in poverty and social exclusion, bringing in a decrease in figures related to hunger and malnutrition among the poor population. On the other hand, a vertiginous increase in weight excess is observed in all the layers of the population, pointing towards a new scenario of problems related to food and nutrition, such as chronic non-communicable diseases (BRASIL, 2012 BRASIL. Ministério da Saúde. Secretaria de Atenção à Saúde. Departamento de Atenção Básica. Política nacional de alimentação e nutrição - Série B. Textos Básicos de Saúde. Brasília, DF: Ministério da Saúde, 2012. ). In view of this, the role of Nutrition today is to maximize physiological functions and ensure increased health and well-being with reduced risk of disease (SMET; VOSSEN, 2016 SMET, D.S; VOSSEN, E. Meat balance between nutrition and health.A review. Meat Science, Thailand, v.120, n.62, p.145-156, 2016. ).

Given these facts, a large number of novel products which supposedly provide health improvement ha e been presented by the food industry, due to the concern on food and nutrition (ANJO, 2004 ANJO, D.L.C. Alimentos funcionais em angiologia e cirurgia vascular. Jornal Vascular Brasileiro, São Paulo, v.3, n.2, p.145-154, 2004. ). The growing speed at which this occurs gives rise to new terms in this field as, for instance, functional foods. There is still no consensus regarding the concept of “functional food” by the National Agency for Sanitary Surveillance (ANVISA), however, its records state that “a claim of functional property is that concerning the metabolic or physiological role played by the nutrient or non-nutrient in the growth, development, maintenance and other normal functions of the human organism” (ANVISA, 1999). The concept of functional foods is broad and still advocates the assumption that the diet can reduce the risk of involvement by morbidities (BORGES, 2000 BORGES, P.Z. Avaliação nutricional de concentrados proteicos obtidos do leite bovino. 2000. 83 f. Dissertação (Mestre em Engenharia de Alimentos) - Faculdade de Engenharia de Alimentos, Universidade Estadual de Campinas, Campinas, 2000. ).

According to Roberfroid (2002) ROBERFROID, M.B. Global view on functional foods: European perspectives. British Journal of Nutrition, Cambridge, v.88, p.133-138, 2002. , the functional food can be: 1. Natural food. 2. Food to which a component has been added. 3. Food from which a component has been removed. 4. Food in which the nature of one or more components has been modified. 5. Food in which the bioavailability of one or more components has been modified.

Therefore, functional property is present in several foods, such as fruits and vegetables.

Fruits are the subject of studies worldwide, aiming to elucidate the properties and effects of substances in these foods, including certain phenolic compounds, lectins and trypsin inhibitors (VASCONCELOS; OLIVEIRA, 2004 VASCONCELOS, I.M.; OLIVEIRA, J.T. Antinutritional properties of plant lectins. Toxicon, Oxford, v.44, n.4, p.385-403, 2004. ). Phenolic compounds have an antioxidant function which attracts a special attention to fruits regarding the treatment and prevention of various diseases, including degenerative diseases (GARDNER et al., 2000 GARDNER, P.T.; WHITE, T.A.; MCPHAIL, D.B.; DUTHIE, G.G. The relative contributions of vitamin C, carotenoids and phenolics to the antioxidant potential of fruit juices. Food Chemistry, Barking, v.68, n.4, p.471-474, 2000. , LEONG ;SHUI, 2002 LEONG, L.P.; SHUI, G. An investigation of antioxidant capacity of fruits in Singapore markets. Food Chemistry, Barking, v.76, n.1, p.69-75, 2002. ; KUSKOSKI et al., 2006 KUSKOSKI, E.M.; ASUERO, A.; MORALES, M.; FETT, R. Frutos tropicais silvestres e polpas de frutas congeladas: atividade antioxidante, polifenóis e antocianinas. Ciência Rural, Santa Maria, v.36, n.4, p.1283 - 1287, 2006. ).Lectins are proteins capable of binding to glycogen and glycoconjugates (HATAKEYAMA et al., 1995 HATAKEYAMA, T.; NAGATOMO, H.; YAMASAKI, N. Interaction of the hemolytic lectin CEL-III from the marine invertebrate Cucumaria echinata with the erythrocyte membrane. The Journal of Biological Chemistry, Bethesda v.270, n.8, p.3560-3564, 1995. ), and by doing so those can modulate the function of these molecules. As an example, by associating with the glycoproteins in the surface of certain tumor cells, lectins can lead to a change in cellular metabolism, by modulating various intracellular signal transduction pathways (PARK et al., 2000 PARK, R.; KIM, M.S.; SO, H.S.; JUNG, B.H.; MOON, S.R.; CHUNG, S.Y.; KO, C.B.; KIM, B.R.; CHUNG, H.T. Activation of c-Jun N-terminal kinase 1 (JNK1) in mistletoe lectin II-induced apoptosis of human myeloleukemic U937 cells. Biochemical Pharmacology, Kansas, v.60, n.11, p.1685-1691, 2000. ) and, as shown by several in vitro and in vivo studies, lectins can inhibit various stages of the carcinogenesis process (HOLLMAN, KATAN, 1997 HOLLMAN P.C.H.; KATAN M.B. Absorption, metabolism and health effects of dietary flavonoids in man. Biomedicine &Pharmacotherapy, Paris, v.51, n.8, p.305-310, 1997. ; RABELO et al., 2012 RABELO, L.M.A.; MONTEIRO, N.; SEQUIZ, R.P.; SANTOS, P.I.M.; OLIVEIRA, R.; OLIVEIRA, A.S.; ROCHA, H.A.; HELONEIDA, A.; UCHOA, A.; SANTOS, E.A. A lactose-binding lectin from the marine sponge Cinachyrella apion (Cal) induces cell death in human cervical adenocarcinoma cells. Marine Drugs, Basel, v.10, n.4, p.727-743, 2012. ; MAESTRI, 2014 MAESTRI, C.A. Avaliação da importância da concentração de lectina ligante de manose (MBL) na evolução das lesões escamosas de baixo grau, alto grau e câncer de colo uterino. 2014. 44 f. Dissertação (Mestrado) - Universidade Federal do Paraná, Curitiba, 2014. ).

Nevertheless, despite the efforts, the “functional” properties of many fruits are still unknown (RIBEIRO et al., 2015 RIBEIRO, J.A.; SERQUIZ, A.C.; SILVA, P.F.; BARBOSA, P.B.; SAMPAIO, T.B.; ARAUJO JUNIOR, R.F.; OLIVEIRA, A.S.; MACHADO, R.J.; MACIEL, B.L.; UCHOA, A.F.; SANTOS, E.A.; MORAIS, A.H. Trypsin inhibitor from tamarindus indica L. seeds reduces weight gain and food consumption and increases plasmatic cholecystokinin levels. Clinics, São Paulo, v.70, p.136-143, 2015. ). One of them is atemoya (Annona x atemoya Mabb.). This is a hybrid fruit resulting from the cross between cherimolia (Annoma cherimola Mill.) and sugar apple (also known as earl fruit or ata) (Annoma squamosa L.) (STENZEL et al., 2003 STENZEL, N.M.C; MURATA, I.M.; NEVES, C.S.V.J. Superação da dormência em sementes de atemóia e fruta-do-conde. Revista Brasileira Fruticultura, Jaboticabal, v.25, n.2, p.305-308, 2003. ). It is intentionally produced because it is easy to plant and highly adaptable to the tropical climate, further to being described as tastier, containing fewer seeds and having a longer post-harvest life when compared to cherimolia and sugar apple (MARCELLINI et al., 2003 MARCELLINI, P.S.; CORDEIRO, C.E.; FARAONI, A.S.; BATISTA, R.A.; RAMOS, A.L.D.; LIMA, A.S. Comparação físico-química e sensorial da atemóia com a pinha e a graviola produzidas e comercializadas no estado de Sergipe. Alimentos e Nutrição, São Paulo, v.14, n.2, p.187-189, 2003. ; RABLLO et al., 2014 RABÊLO, S.V.; COSTA, M.M.D.; LIBÓRIO, R.C.; ALMEIDA, J.R.G.D.S. Antioxidant and antimicrobial activity of extracts from atemoia (Annona cherimola Mill.x A.squamosa L.). Revista Brasileira de Fruticultura, Jaboticabal, v.36, p.265-271, 2014. Número especial. ). The main destination of atemoya fruits is in natura consumption. Although considered very tasty fruits, their production and commercialization are still limited and there is little availability of fresh fruits in the Brazilian and world markets. Moreover, there are few studies about their benefits to human health (PEREIRA et al., 2011 PEREIRA, M.C.T.; NIETSCHE, S.; COSTA, M.R.; CRANE, J.H.; CORSATO, C.D.A.; MIZOBTSI, E.H. Anonáceas: pinha, atemoia e graviola. Informe Agropecuário, Belo Horizonte, v.32, n.264, 2011. ).

If little is known about the atemoya fruit, to date, there are no data referring to atemoya wastes: peel and seed. They account for about 40% of the fruit’s weight and are discarded by consumers.

Discarded waste from food could have a beneficial purpose for man and the environment.

Some fruits, during processing, have their seeds discarded. However, they could be used, minimizing this waste. One way this could be done would be to obtain higher added value products of the seeds, like, for instance, vegetable oils (KOBORI; JORGE,2005 KOBORI, C.; JORGE, N. Caracterização dos óleos de algumas sementes de frutas como aproveitamento de resíduos industriais. Ciência e Agrotecnologia, Lavras, v.29, p.1008-1014, 2005. ). In addition, some researchers have shown the presence of phytochemicals in fruit peel and seed (AL-DAIHAN; BHAT, 2012 AL-DAIHAN, S; BHAT, R.S. Antibacterial activities of extracts of leaf, fruit, seed and bark of Phoenix dactylifera. African Journal of Biotechnology, Nairobe, v.11, n.42, p.10021-10025, 2012. ), which brings functional value to these types of food residues.

The properties of atemoya and its residues are still unknown, thus the importance to explore and investigate their biotechnological and pharmacological potentials. Thereby, for this work, extracts of atemoya peel, pulp and seed were obtained and the protein and phenolic compound contents of the extracts were evaluated, as well as their hemagglutinating agents and protease inhibitors activities, in order to initiate filling the gap regarding the knowledge about the potential of atemoya and its residues.

Materials and Methods

The atemoya (Annona cherimola Mill. X A. squamosa L.) fruit samples were obtained in supermarkets in the city of Natal-RN in February 2014 and their parts (seed, pulp and peel) were manually separated.

Extraction - to obtain the extracts of the different parts of atemoya, fruits were selected and those containing signs of infestation, poor state of conservation or advanced maturation were discarded.

The fruits chosen were opened and divided into three parts: pulp, peel and seed. The first two were frozen (-20ºC) and only defrost at the time of obtaining the extracts. The seeds were dried in a ventilated oven at 60^oC, peeled for tegument removal, and the cotyledon was then ground in an industrial mill until the seed meal, which was then cooled, was formed.

All samples were through extraction proceses in three buffers, separately - 0.05 M sodium acetate, pH 4.3; 0.05 M tris-HCl, pH 7.5 and 0.05 M tris added to 0.05 M glycine, pH 11.5 – at 1:10 (w/v) ratio, for seed extraction, and 1:2 (w/v) for peel and pulp, and maintained for four hours under constant stirring. Subsequently, the samples were centrifuged at 4oC for 30 minutes at 8000 x g. The precipitate was discarded and the supernatant obtained was named crude extract.

Protein Dosage - all protein determinations were performed by the method of Bradford (1976) BRADFORD, M.M. A rapid and sensitive method for the quantification of microgram quantities of protein utilizing the principle of protein-dye binding. Analytical Biochemistry, New York, v.72, n.1/2, p.248-254, 1976. with modifications. In a 96-well flat bottom plate, 10 μL of the extracts was placed in different titrations.

Subsequently, 200 μl of the Bradford reagent was added and the plate was rested for approximately ten minutes before being read on a microplate reader at 595 nm. Bovine albumin was used to determine the standard curve and wells containing only 10 μL of the extraction buffers were used as white.

Total phenolic compounds assessment - the total phenolic content was measured in duplicate, and the tests were repeated three times for each extract as described by Melo-Silveira et al. (2014) MELO-SILVEIRA, R.F.; FIDELIS, G.P.; VIANA, R.L.S.; SOEIRO, V.C.; SILVA, R.A.D.; MACHADO, D.; COSTA, L.S.; FERREIRA, C.V.; ROCHA, A.O. Antioxidant and antiproliferative activities of methanolic extract from a neglected agricultural product: corn cobs. Molecules, Basel, v.19, n.5, p.5360-5378, 2014. .

An analytical curve containing 500, 400, 300, 200, 100, 50, 10 and 0 mg/ml of gallic acid was used as an equivalence reference. 200 μl of extracts was then separately added to the test tubes, then 1400 μl of ultrapure water, and 100 μl of Folin reagent. The tubes were then shaken in a tube shaker and rested for ten minutes at room temperature. Sequentially, 50 μl of 20% sodium bicarbonate was added to the tubes, which were again stirred and placed in a water bath at 40°C for 20 minutes. Whites containing only the respective extraction buffers from each crude extract were made to exclude residual absorbance.

The absorbance readings were performed at 765 nm in a spectrophotometer. The results were expressed as gallic acid equivalents (EAG)/g of sample dry weight.

Trypsin inhibitory activity - the trypsin inhibitory activity test, for the three fruit parts, was performed in triplicate, being repeated three times and determined as described by Migliolo et al. (2010) MIGLIOLO, L.; de OLIVEIRA, A.S.; SANTOS, E.A.; FRANCO, O.L.; MAURÍCIO, P. Structural and mechanistic insights into a novel non-competitive Kunitz trypsin inhibitor from Adenanthera pavonina L. seeds with double activity toward serine-and cysteine-proteinases. Journal of Molecular Graphics and Modelling, New York, v.29, n.2, p.148-156, 2010. . Thus, 10 μL of the enzyme was added into the tubes and then 120 μL of 2.5 mM hydrochloric acid and 100 μL of the extracts, separately. Subsequently, 0.05 mM Tris-HCl buffer, pH 7.5 was added to obtain the final volume of 790 μl. An extract free tube was determined as the standard for enzymatic activity. After this procedure, the tubes were kept in a water bath at 37^oC for 10 minutes, and 500 μL of 1.25 mM BAPNA substrate was added to the water bath. The reaction was then halted with the addition of 120μl of 30% acetic acid. The whites were made into sample tubes, where the substrate was only added after the reaction stopped. The result was measured by spectrophotometer reading at 410 nm.

The results were expressed in specific inhibitory activity obtained in three sequential assays with the same samples. The specific activity was calculated as the ratio between the sample’s inhibition units and the amount of proteins or phenolic compounds present in the test samples. An inhibitory unit was defined as the amount of inhibitor decreasing enzyme activity by 0.01 of the absorbance at 410 nm.

Inhibitory activity for chymotrypsin - the inhibitory activity on chymotrypsin was measured according to the methodology proposed by Oliveira et al. (2007) OLIVEIRA, A.S.; MIGLIOLO, L.; AQUINO, R.O.; RIBEIRO, J.K.C.; MACEDO, L.L.P.; ANDRADE, L.B.S.; BEMQUERER, M.P.; SANTOS, E.A.; KIYOTA, S.; SALES, M.P. Purification and characterization of a trypsin-papain inhibitor from Pithecelobium dumosum seeds and its in vitro effects digestive enzymes from insect pests. Plant Physiology and Biochemistry, Amsterdam, v.45, p.858-865, 2007. with adaptations. Thus, 20 μL of bovine chymotrypsin (0.1 mg / mL in 50 mM Tris-HCL, pH 7.5, containing 20 mM CaCl2) was added to 100 μL of the inhibitor and incubated for 15 minutes at 37°C.

After this, the reaction was started by adding 200 mL of 1% azocasein. After 30 minutes, the reaction was halted by adding 300 mL of 20% TCA solution.

The reaction mixture was centrifuged at 12,000 x g for 10 minutes and the supernatant basified with 2M NaOH at 1:1 ratio. The absorbance was measured in a spectrophotometer at 440 nm. White tests were performed and the tests were done in triplicate. The results were expressed in specific activity, calculated in the same manner as for the trypsin testes.

Hemagglutinating activity - the hemagglutinating activity was verified following the methodology adapted by Medeiros et al. (2010) MEDEIROS, D.S.; MEDEIROS, T.L.; RIBEIRO, J.K.; MONTEIRO, N.K.; MOGLIOLO, L., UCHOA, A.F.; SANTOS, E.A. A lactose specific lectin from the sponge Cinachyrella apion: purification, characterization, N-terminal sequences alignment and agglutinating activity on Leishmania promastigotes. Comparative Biochemistry and Physiology Part B: Biochemistry and Molecular Biology, Amsterdam, v.155, n.3, p.211-216, 2010. . Three 1 mL aliquots of human types A, B and O erythrocytes were washed with 12 mL of 0.9% saline solution and centrifuged at 3500 rpm for five minutes until a serum free erythrocyte mass was obtained. Two aliquots of each blood type were subjected to enzymatic treatment - one with papain and one with trypsin - to increase exposure of the red blood cell binding sites and the other was maintained as native blood. The treated aliquots were rewashed for complete removal of the enzymes. The hematocrit was performed and 4% erythrocytes solutions were prepared in saline.

Hemagglutination tests were performed by serial dilution in “V’ bottom 96-well plates. In each well 25μl of saline solution, 25μl of the 12 titrations serially diluted samples were added. Thus 25μL of a 4% erythrocyte suspension was added and the reaction was incubated at room temperature for 1 hour and visually analyzed after that period.

Each sample was tested with type A, B and O blood – trypsin treated, papain treated and native - separately.

The specific hemagglutinating activity (HU/μg) was determined by the ratio between the hemagglutinating units and the amount of protein or phenolic compounds contained in the evaluated sample. The hemagglutinating unit was obtained as the maximum titer at which agglutination of the red blood cells was noted.

Statistical analysis – the data were tabulated and analyzed using descriptive statistics, through central trend and dispersion measures (mean and standard deviation) with the Microsoft Excel® program, version 2015.

Results and discussion

The results presented in Table 1 refer to the quantification data of soluble proteins and phenolic compounds present in the atemoya extracts.

Regarding the content of phenolic compounds, it was observed that the three extracts obtained from the peel are the ones with the greater content of this component, followed by the pulp extracts. When comparing the three buffers studied, the largest quantities of phenolic compounds, regardless of source, were always extracted using the tris-glycine buffer. It is believed that the peel extracts stand out because they are the main reservoirs of phenolic compounds in most of the studied fruits (Heim et al., 2002 HEIM, K.E; TAGLIAFERRO, A.R.; BOBILYA, D.J. Flavonoid antioxidants: chemistry, metabolism and structure-activity relationships. The Journal of Nutritional Biochemistry, Stoneham, v.13, p.572-584, 2002. ).These molecules are considered as one of the main responsible for the antioxidant action of fruits and are indicated as preventive agents of chronic-degenerative diseases and other biological processes related to oxidative stress (ALMEIDA et al., 2011 ALMEIDA, M.M.B.; DE SOUZA, P.H.M.; ARRIAGA, Â.M.C.; DO PRADO, G.M.; DE CARVALHO, C.E.; MAIA, G.A.; DE LEMOS, T.L.G. Bioactive compounds and antioxidant activity of fresh exotic fruits from northeastern Brazil. Food Research International, London, v.44, n.7, p.2155-2159, 2011. ). Finding them in atemoya, especially in the peel, is a display of the potential lost by the population when using the fruit, since it is common not to use that part of atemoya as food.

Regarding proteins (Table 1), when comparing the amount of protein obtained from each part of the fruit using the same buffer, it is verified that, regardless of the buffer, more protein is always obtained from the seed than from other parts This occurred mainly when the tris-glycine buffer was used, a condition at which ten times more proteins were obtained from the seeds than from the pulp and the peel. Also with respect to such buffer it has been found that the amounts of proteins extracted from the pulp and the peel are similar. In the other conditions, the amount of protein extracted from the peel was higher than those extracted from the pulp.

These data corroborate with those obtained by Cruz (2011) CRUZ, L.S. da. Caracterização física e química da casca, polpa e semente de atemoia “gefner”. 2011. Dissertação (Mestrado) - Universidade Federal de Lavras, Lavras, 2011. , since they show that the seed, followed by the peel, would be the main protein reservoirs of atemoya. This would reflect, therefore, the higher amount of proteins found in the extracts obtained from these parts in comparison to the extracts obtained from the pulp. With the trisglycine buffer, regardless of the fruit part used, more proteins were always extracted than with the other buffers. An explanation for these facts is probably the characteristic of the proteins extracted and of their amino acids. The tris-glycine buffer was the only one to maintain the basic pH, around 11. This value enables the ionization of basic amino acids, which increases the solubility of their proteins (HOVING et al., 2002 HOVING, S.; GERRITS, B.; VOSHOL, H.; MULLER, D.; ROBERTS, R.C.; OOSTRUM, J.V. Preparative two-dimensional gel electrophoresis at alkaline pH using narrow range immobilized pH gradients. Proteomics, Weinheim, v.2, p.127-134, 2002. ). Therefore, it is believed that more proteins were extracted with the tris-glycine buffer because atemoya would be rich in proteins comprising basic amino acids in their constitution, which favors their solubilization at basic pH.

Figure 1 shows the specific inhibition activity of the trypsin enzyme in IU/μg of protein (Figure 1A) and IU/μg of phenolic compounds (Figure 1B).

With respect to the seed extracts it can be observed that with those rich in proteins, i.e. extracts obtained with tris-glycine and tris-HCl (Table 1), no detectable rates of trypsin enzyme inhibition were observed when the protein component was analyzed.

This index was only observed when the phenolic component was analyzed. For the acetate extract, the best trypsin inhibition rates were obtained both with respect to the protein and phenolic components (Figure 1A and Figure 1B). It is also worth noting that this extract had a high specific activity for phenolic compounds, which is an unusual fact, given the fact that this extract, among the three, has the lowest content of phenolic compounds, indicating a high specificity of the phenolic compounds extracted.

Considering the peel, it was possible to inhibit the trypsin activity with all of its extracts.

Amongst them, it was with the peel extract obtained with acetate that the best specificity of trypsin inhibition was verified, considering the specific activity of the protein component.

For the pulp extract obtained with the trisglycine buffer, very low rates of trypsin inhibition were observed for both the protein and phenolic components. The pulp extract obtained with the Tris-HCl buffer presented high specific activity of the protein components, the highest obtained among all the extracts evaluated herein (Figure 1).

Trypsin inhibitors of protein origin have already been found in various vegetable sources, such as peanuts (ARAUJO, 2014 ARAÚJO, J.M.; ALVES, J.C.; PEIXOTO, T.O.N.; MEDEIROS, A.F.; MACHADO, R.J.DE A.; SERQUIZ, A.C.; SANTOS, E.A.; UCHOA, A.F.; MORAIS, A.H.A. Determination of antitryptic activity in proteins from peanut products isolated by affinity chromatography. Química Nova, São Paulo, v.37, n.10, 2014. ), in pulps and seeds of tropical fruits, such as white and red varieties of guava, passion fruit, watermelon (BEZERRA, 2014 BEZERRA, A.D.L,; BARBOSA, C.R.M.; CARVALHO, F.M.C.D.; SERQUIZ, A.C.; MORAIS, A.H.D.A. Antitryptic activity of proteins from pulps and seeds of tropical fruits. Revista Brasileira de Fruticultura, Jaboticabal, v.36, n.2, p.408-416, 2014. ), and tamarind (RIBEIRO et al., 2015 RIBEIRO, J.A.; SERQUIZ, A.C.; SILVA, P.F.; BARBOSA, P.B.; SAMPAIO, T.B.; ARAUJO JUNIOR, R.F.; OLIVEIRA, A.S.; MACHADO, R.J.; MACIEL, B.L.; UCHOA, A.F.; SANTOS, E.A.; MORAIS, A.H. Trypsin inhibitor from tamarindus indica L. seeds reduces weight gain and food consumption and increases plasmatic cholecystokinin levels. Clinics, São Paulo, v.70, p.136-143, 2015. ).With regard to atemoya, only one other study evaluating extracts of this fruit as trypsin inhibitors was identified. In this case, pulp and peel extracts have proven to possess trypsin inhibitory activity. However, the individual influence of both the protein and phenolic components in this inhibition was not determined (CRUZ, 2011 CRUZ, L.S. da. Caracterização física e química da casca, polpa e semente de atemoia “gefner”. 2011. Dissertação (Mestrado) - Universidade Federal de Lavras, Lavras, 2011. ).

In these foregoing studies, the use of different extraction conditions for inhibitors of existing sources was not evaluated. However, it can be stated that use of the tris-glycine buffer, at least in the case of atemoya, decreases the extraction of trypsin inhibitors.

Trypsin inhibitors are known as antinutritional substances because they have inhibitory action of digestive enzymes. This inhibition results in decreased protein digestion, compromising the absorption of amino acids, and leading to loss of peptides through feces. This generates negative nitrogen balance, a fact that leads to losses to individuals (VAZ PATTO et al., 2015 VAZ PATTO, M.C.; AMAROWICZ, R.; ARYEE, A.N.; BOYE, J.L.; CHUNG, H.J.; MARTIN-CABREJAS, M.A.; DOMONEY, C. Achievements and challenges in improving the nutritional quality of food legumes. Critical Reviews in Plant Sciences, London, v.34, n.1-3, p.105-143, 2015. ).Trypsin inhibitors are described in several plant sources, including beans, the most consumed pulses in Brazil (Vaz Patto et al., 2015 VAZ PATTO, M.C.; AMAROWICZ, R.; ARYEE, A.N.; BOYE, J.L.; CHUNG, H.J.; MARTIN-CABREJAS, M.A.; DOMONEY, C. Achievements and challenges in improving the nutritional quality of food legumes. Critical Reviews in Plant Sciences, London, v.34, n.1-3, p.105-143, 2015. ; Yamamoto, IKENAKA, 1967 YAMAMOTO, M.;IKENAKA, T. Studies on soybean trypsin inhibitors i.purification and characterization of two soybean trypsin inhibitors. The Journal of Biochemistry, Tokyo, v.62, n.2, p.141-149, 1967. ; GU et al., 2014 GU, C.; SONG, X.; ZHAO, L.; PAN, S.; QIN, G. Purification and characterization of bowman-birk trypsin inhibitor from soybean. Journal of Food and Nutrition Research, Newark, v.2, n.9, p.546-550, 2014. ). Phenolic compounds are also reported as being trypsin inhibitors in three grape varieties (CARVALHO et al., 2014 CARVALHO, F.M.C ; BEZERRA, A.D.L.; SANTOS, E.A.; MACHADO, R.J.A.; DANTAS, M.B.V.C.; ARAUJO, A.H. Phenolic compounds and antitryptic activity from pulpls and seeds of three varieties of grapes. Revista Brasileira de Inovação Tecnologica em Saúde, Natal, v.4, p.39-50, 2014. ).

The low trypsin concentration in foods may contribute to the bioavailability of the protein nutrients found in these foods, favoring their digestion and absorption processes, thus contributing to the added nutritional value of the food (Silva et al., 2000 SILVA, M.R.; DA SILVA, M.A.A.P. Fatores antinutricionais: inibidores de proteases e lectinas. Annual Review of Nutrition, Palo Alto, v.13, n.1, p.3-9, 2000. ). However, from the studies carried out with inhibitors, there is still little practical knowledge on how to reduce the amount of these antinutritional factors. Therefore, it is of paramount importance to find extraction media that allow the acquisition of smaller inhibitor amounts, which is the case observed when the tris-glycine buffer was used. Based on the data obtained, it is suggested that studies to be carried out with fruits evaluate different conditions for the extract obtention, in order to identify their real nutraceutical potential.

The seed extracts obtained with acetate and the pulp extracts obtained with tris-HCl, in their turn, contain a greater specific inhibitory activity of trypsin (Figure 1) and can be used in research aimed at the purification and characterization of trypsin inhibitors. These molecules are identified as possessing properties such as anticancer, antiinflammatory and anticoagulant (KENNEDY, 1998 KENNEDY, A.R. The chemopreventive agents: protease inhibitors. Pharmacology &Therapeutics, Kansas, v.78, n.3, p.167-209, 1998b. ; OLIVA et al., 2000 OLIVA, M.L.; SOUZA-PINTO, J.C.; BATISTA, I.F.; ARAUJO, M.S.; SILVEIRA, V.F.; AUERSWALD, E.A.; MENTELE, R.; ECKERSKORN, C.; SAMPAIO, M.U.; SAMPAIO, C.A. Leucaena leucocephala serine proteinase inhibitor: primary structure and action on blood coagulation, kinin release and rat paw edema. Biochimica et Biophysica Acta, Amsterdam, v.1477, n.1-2, p.64-74, 2000. ). They may help to control glycemia (SERQUIZ et al., 2016 SERQUIZ, A.C., MACHADO, R.J., SERQUIZ R.P., LIMA, V.C., CARVALHO, F.M.C., CARNEIRO, M.A, MACIEL, B.L.L., UCHÔ, A.F, SANTOS, E.A, MORAIS, A.H. Supplementation with a new trypsin inhibitor from peanut is associated with reduced fasting glucose, weight control, and increased plasma CCK secretion in an animal model. Journal of Enzyme Inhibition and Medicinal Chemistry, Basingstoke, v.31, n.6, p.1261-1269, 2016. ) and suppress the regulation of pancreatic secretion with greater release of the cholecystokinin hormone (CCK) through the intestinal mucosa, a hormone known as satietyogenic (LIENER, 1994 LIENER, I.E. Implications of antinutritional components in soybean foods. Critical Reviews of Food Science &Nutrition, Cleveland, n.34, p.31-67, 1994. ; SERQUIZ, 2012 SERQUIZ, A.C. Efeito sacietogênico de um novo inibidor de tripsina da paçoca do amendoim com aumento plasmático de colecistocinina (cck). 2012. 97 f. Dissertação (Mestrado em Bioquímica) - Universidade Federal do Rio Grande do Norte, Natal, 2012. ). However, not all of them have the same activities or the same efficiency as bioactive agents. This drives the search for the discovery of new trypsin inhibitors which may have different or more efficient physiological actions, even presenting less side effects. The extraction of these compounds in different buffers is fast, reproducible and inexpensive, and can also be used to select fruits presenting higher indexes of inhibitors in the peel and seed in order to select cultivars that are more resistant to pests.

Chymotrypsin inhibitors, as for the trypsin inhibitors, were extracted in different amounts for each extract (Figure 2).

Regarding the protein inhibitors (Figure 2A), it was verified that the seed is the source with the least amount of these inhibitors, as well as for trypsin, whereas in the peel and in the pulp the highest values were observed. In this case, with the acetate buffer and the Tris-HCl buffer, respectively.

For the phenolic compounds, it was with the seed extract that the highest value of specific inhibition of the enzyme was obtained (Figure 1B and 2B), however, the phenolic composition was not elucidated. It is assumed that these extracts would have the presence of alkaloids and tannins (SANTOS, 2007 SANTOS, A.G. Estudo fitoquímico e atividade leishmanicida de Annona impressivenia Safford (Annonaceae). 2007. Dissertação (Mestrado) - Universidade Federal do Amazonas, Manaus, 2007. ) and, therefore, the predominance of the specific activity in the seed extract may be a compensatory effect for the specific activity of these molecules. Regardless, it is worth noting that inhibitory activity was found for all extracts.

To date, chymotrypsin inhibitors have, admittedly, a range of possibilities of diverse functions and properties for living organisms and previously unexplored biotechnological applications, of which biomedicine and environmental applications can be highlighted.

Several plants were selected for generations in order to choose the cultivars with the greatest number of chymotrypsin inhibitors, which would therefore be more resistant to insect-plague attack (PADUL et al., 2012 PADUL, M.V.; RAJESH, D.T.; MANVENDRA S.K. Protease inhibitor (PI) mediated defense in leaves and flowers of pigeonpea (protease inhibitor mediated defense in pigeonpea). Plant Physiology and Biochemistry, Kalyani, v.52, p.77-82, 2012. ). In the biomedical field, it is possible to highlight the potential of these inhibitors in the control of diseases - of which AIDS and cancer are highlighted - due to coagulation as well as to the immune system related effects (GUPTA et al., 2013 GUPTA, A.; SHARMA, S.; REICHENBACH, P.; MARJAVAARA, L.; NILSSON, A.K.; LINGNER, J.; CHABES, A.; ROTHSTEIN, R.; CHANG, M. Telomere length homeostasis responds to changes in intracellular dNTP pools. Genetics, Baltimore, v.193, n.4, p.1095-105, 2013. ).

The tris-glycine extracts of the peel, seed and pulp of the atemoya fruit, despite presenting a great amount of protein in relation to the other components evaluated (Table 1), showed low specific inhibition activity, both for trypsin and chymotrypsin, when compared to other fruits described in the literature (BEZERRA, 2014 BEZERRA, A.D.L,; BARBOSA, C.R.M.; CARVALHO, F.M.C.D.; SERQUIZ, A.C.; MORAIS, A.H.D.A. Antitryptic activity of proteins from pulps and seeds of tropical fruits. Revista Brasileira de Fruticultura, Jaboticabal, v.36, n.2, p.408-416, 2014. ). This indicates that these extracts have a high nutritional value, since they present a higher amount of protein and lower amount of inhibitors, favoring their digestion and absorption process. Future studies of digestibility for these extracts could confirm this hypothesis.

The presence of proteins in the extracts indicated the existence of lectins in them. Lectins are carbohydrate-recognizing proteins with high biotechnological potential (SHIMOKAWA et al., 2016 SHIMOKAWA, M.; HARAGUCHI, T.; MINAMI, Y.; YAGI, F.; HIEMORI, K.; TATENO, H.; HIRABAYASHI, J. Two carbohydrate recognizing domains from Cycas revolute leaf show the distinct sugar-binding specificity – A unique mannooligo saccharide recognition by N-terminal domain. The Journal of Biochemistry, Tokyo, v.11, n.3, p.06-24, 2016. ) and a rapid way to identify their presence is to use the blood cell agglutination test, since several lectins are known as agglutinins (POP et al. al., 2015b POP, A.; CORNEA, C.P.; IORDACHE, F.; FAFANEATA, C.; PISOSCHI, A.M. Spectroscopic and molecular modeling investigations on structural changes of food grade proteins. Journal of Biotechnology, New York, v.208, p.S5-S120, 2015b. Abstracts. ).

Table 2 shows the specific hemagglutinating activity of the extracts obtained from the seed, peel and pulp of atemoya. Using tris-glycine buffer, the haemagglutinating activity molecule was not extracted.

Another noteworthy fact was the absence of hemagglutinating activity in the three extracts obtained from the atemoya seeds (Table 2). This data does not agree with others in the literature, which show that seeds are good sources of lectins (NG TZI BUN et al, 2015 NG TZI BUN; SANG, C.Y.; ASA, N.C.C.; HO, W.J. Purification and Characterization of a Lectin from Green Split Peas (Pisum sativum). Applied Biochemistry and Biotechnology, Totowa, v.177, n.6, p.1374-1385, 2015. ), and can lead to two notices.

There are actually no lectins in the atemoia seed, after all three extraction conditions were used, and in the three conditions no agglutinating activity was identified. Another thing Is that the possibility of agglutinating lectins or other agglutinating agents in the atemoia seed can not be totally excluded, since there is a possibility that the extraction conditions were not favorable to extract those, or disadvantage their activities, fact which has already been described by other authors when studying other fruits (POP et al., 2015a POP, A.; CLENCIU, D.; ANGHEL, M.; RADU, S.; MOTA, E.; MOTA, M.; PANDURU, N.M. Insulin resistance is associated with all chronic complications in type 1 diabetes. Journal of Diabetes, Richmond, v.8, n.2, p.220-8, 2015a. ). It is hoped to use other conditions in the future to clarify whether or not there are agglutinants in atemoya seeds.

In the pulp and the peel (Table 2), the binding activity was evidenced in different intensities. It stands out that, when obtained with the sodium acetate or tris-HCl buffers, they were able to agglutinate all three types of blood (treated or native), which highlights the possibility of having one more binding molecule and/or of aglutinin binding nonspecificity.

This data also points to the existence of lectins in the extracts. Lectins are molecules with great potential, as for example, being apoptosis inducing agents in tumor cells (PARK et al., 2000 PARK, R.; KIM, M.S.; SO, H.S.; JUNG, B.H.; MOON, S.R.; CHUNG, S.Y.; KO, C.B.; KIM, B.R.; CHUNG, H.T. Activation of c-Jun N-terminal kinase 1 (JNK1) in mistletoe lectin II-induced apoptosis of human myeloleukemic U937 cells. Biochemical Pharmacology, Kansas, v.60, n.11, p.1685-1691, 2000. ; RABELO et al., 2012 RABELO, L.M.A.; MONTEIRO, N.; SEQUIZ, R.P.; SANTOS, P.I.M.; OLIVEIRA, R.; OLIVEIRA, A.S.; ROCHA, H.A.; HELONEIDA, A.; UCHOA, A.; SANTOS, E.A. A lactose-binding lectin from the marine sponge Cinachyrella apion (Cal) induces cell death in human cervical adenocarcinoma cells. Marine Drugs, Basel, v.10, n.4, p.727-743, 2012. ).

The other component of the extracts are the phenolic compounds. There are authors who show that some phenolic compounds may have agglutinating action (CAROCHO, 2013 CAROCHO, M., FERREIRA, I. A review on antioxidants, prooxidants and related controversy: natural and synthetic compounds, screening and analysis methodologies and future perspectives. Food and Chemical Toxicology, Oxford, v.51, p.15-25, 2013. ; CALUETE, et al., 2015 CALUÊTE, M.E.E., DE SOUZA, L.M.P., FERREIRA, E., FRANÇA, A.P., GADELHA, C.A., AQUINO, S.J., SANTI-GADELHA, T. Nutritional, antinutritional and phytochemical status of okra leaves (Abelmoschus esculentus) subjected to different processes. African Journal of Biotechnology, Nairobi, v.14, n.8, p.683-687, 2015. .)Therefore, the possibility that the phenolic compounds of the atemoya extracts can act as agglutinins can not be ruled out. It is hoped to subject these extracts to purification steps in the future in order to characterize the phenolic compounds and the lectins present in the atemoya.

The molecules discussed in this paper, probably present in the pulp, peel and seed extracts of atemoya, have great interest both for biomedical research and for environmental science studies.

Acquiring knowledge about them has the effect of increasing the added value of atemoya and its residues (peel and seed), thus strengthening the production chain around the production and use of this fruit.

Figure 1
Specific inhibitory activity of the seed, peel and pulp extracts of the atemoya fruit for three extraction buffers, tested against trypsin, calculated based on the amount of proteins (A) and phenolic compounds (B). IU – inhibition unit.

Figure 2
Specific inhibitory activity of the seed, peel and pulp of the atemoia fruit extracts for different extraction buffers, tested against chymotrypsin, calculated on the basis of the amount of proteins (A) and phenolic compounds (B). IU - inhibition unit .

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Table 1
Soluble proteins and phenolic compounds in aqueous extracts of three parts of the atemoya fruit, for three extraction buffers. ND - levels lower than the Bradford reaction sensitivity.

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Table 2
Specific Hemagglutinating Activity (UH/µg) in extracts obtained from the seed, peel and pulp of atemoya for different extraction buffers; calculated based on the amount of proteins and phenolic compounds. Each blood type (A, B and O) was evaluated natively (N), papain treated (P) and trypsin treated (T), separately.

Conclusion

The atemoya, including its currently neglected parts, has several biological molecules, from which trypsin and chymotrypsin inhibitors, and haemagglutinating molecules can be highlighted.

Acknowledgements

This research was presented to the Graduate Program in Health Sciences of the Federal University of Rio Grande do Norte as part of the thesis of Alexandre Coelho Serquiz. Hugo A O Rocha thanks CNPq for his productivity grant.

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RABELO, L.M.A.; MONTEIRO, N.; SEQUIZ, R.P.; SANTOS, P.I.M.; OLIVEIRA, R.; OLIVEIRA, A.S.; ROCHA, H.A.; HELONEIDA, A.; UCHOA, A.; SANTOS, E.A. A lactose-binding lectin from the marine sponge Cinachyrella apion (Cal) induces cell death in human cervical adenocarcinoma cells. Marine Drugs, Basel, v.10, n.4, p.727-743, 2012.
RABÊLO, S.V.; COSTA, M.M.D.; LIBÓRIO, R.C.; ALMEIDA, J.R.G.D.S. Antioxidant and antimicrobial activity of extracts from atemoia (Annona cherimola Mill.x A.squamosa L.). Revista Brasileira de Fruticultura, Jaboticabal, v.36, p.265-271, 2014. Número especial.
RIBEIRO, J.A.; SERQUIZ, A.C.; SILVA, P.F.; BARBOSA, P.B.; SAMPAIO, T.B.; ARAUJO JUNIOR, R.F.; OLIVEIRA, A.S.; MACHADO, R.J.; MACIEL, B.L.; UCHOA, A.F.; SANTOS, E.A.; MORAIS, A.H. Trypsin inhibitor from tamarindus indica L. seeds reduces weight gain and food consumption and increases plasmatic cholecystokinin levels. Clinics, São Paulo, v.70, p.136-143, 2015.
ROBERFROID, M.B. Global view on functional foods: European perspectives. British Journal of Nutrition, Cambridge, v.88, p.133-138, 2002.
SANTOS, A.G. Estudo fitoquímico e atividade leishmanicida de Annona impressivenia Safford (Annonaceae). 2007. Dissertação (Mestrado) - Universidade Federal do Amazonas, Manaus, 2007.
SERQUIZ, A.C. Efeito sacietogênico de um novo inibidor de tripsina da paçoca do amendoim com aumento plasmático de colecistocinina (cck). 2012. 97 f. Dissertação (Mestrado em Bioquímica) - Universidade Federal do Rio Grande do Norte, Natal, 2012.
SERQUIZ, A.C., MACHADO, R.J., SERQUIZ R.P., LIMA, V.C., CARVALHO, F.M.C., CARNEIRO, M.A, MACIEL, B.L.L., UCHÔ, A.F, SANTOS, E.A, MORAIS, A.H. Supplementation with a new trypsin inhibitor from peanut is associated with reduced fasting glucose, weight control, and increased plasma CCK secretion in an animal model. Journal of Enzyme Inhibition and Medicinal Chemistry, Basingstoke, v.31, n.6, p.1261-1269, 2016.
SHIMOKAWA, M.; HARAGUCHI, T.; MINAMI, Y.; YAGI, F.; HIEMORI, K.; TATENO, H.; HIRABAYASHI, J. Two carbohydrate recognizing domains from Cycas revolute leaf show the distinct sugar-binding specificity – A unique mannooligo saccharide recognition by N-terminal domain. The Journal of Biochemistry, Tokyo, v.11, n.3, p.06-24, 2016.
SILVA, M.R.; DA SILVA, M.A.A.P. Fatores antinutricionais: inibidores de proteases e lectinas. Annual Review of Nutrition, Palo Alto, v.13, n.1, p.3-9, 2000.
SMET, D.S; VOSSEN, E. Meat balance between nutrition and health.A review. Meat Science, Thailand, v.120, n.62, p.145-156, 2016.
STENZEL, N.M.C; MURATA, I.M.; NEVES, C.S.V.J. Superação da dormência em sementes de atemóia e fruta-do-conde. Revista Brasileira Fruticultura, Jaboticabal, v.25, n.2, p.305-308, 2003.
TARDIDO, A.P.; FALCÃO, M.C. O impacto da modernização na transição nutricional e obesidade. Revista Brasileira de Nutrição Clinica, São Paulo, v.21, n.2, p.117-124, 2006.
VASCONCELOS, I.M.; OLIVEIRA, J.T. Antinutritional properties of plant lectins Toxicon, Oxford, v.44, n.4, p.385-403, 2004.
VAZ PATTO, M.C.; AMAROWICZ, R.; ARYEE, A.N.; BOYE, J.L.; CHUNG, H.J.; MARTIN-CABREJAS, M.A.; DOMONEY, C. Achievements and challenges in improving the nutritional quality of food legumes. Critical Reviews in Plant Sciences, London, v.34, n.1-3, p.105-143, 2015.
YAMAMOTO, M.;IKENAKA, T. Studies on soybean trypsin inhibitors i.purification and characterization of two soybean trypsin inhibitors. The Journal of Biochemistry, Tokyo, v.62, n.2, p.141-149, 1967.

Publication Dates

Publication in this collection
2018

History

Received
03 Oct 2016
Accepted
11 May 2017

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[52] VAZ PATTO, M.C.; AMAROWICZ, R.; ARYEE, A.N.; BOYE, J.L.; CHUNG, H.J.; MARTIN-CABREJAS, M.A.; DOMONEY, C. Achievements and challenges in improving the nutritional quality of food legumes. Critical Reviews in Plant Sciences, London, v.34, n.1-3, p.105-143, 2015.

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Fruit Part	Extraction Buffer	Soluble Proteins mg∙mL^-1	Phenolic Compounds EAG/g
Seed	Tris-Glycine	19,072 (± 0,022)	0,117 (± 0,001)
	Tris-HCl	14,506 (± 0,039)	0,042 (± 0,004)
	Sodium Acetate	0,501 (± 0,007)	0,047 (± 0,001)
Pulp	Tris-Glycine	1,898 (± 0,021)	0,391 (± 0,057)
	Tris-HCl	0,093 (± 0,01)	0,124 (± 0,068)
	Sodium Acetate	ND	0,117 (± 0,009)
Peel	Tris-Glycine	1,865 (± 0,044)	1,375 (± 0,005)
	Tris-HCl	0,608 (± 0,017)	0,328 (± 0,009)
	Sodium Acetate	0,435 (± 0,008)	0,717 (± 0,018)

Protein				Blood Type
				A				B					O
Part		Extract		N		P	T	N		P	T		N	P	T
Semente		Sodium Acetate		-		-	-	-		-	-		-	-	-
		Tris-HCl		-		-	-	-		-	-		-	-	-
		Tris-Glycine		-		-	-	-		-	-		-	-	-
Polpa		Sodium Acetare		-		-	-	-		-	-		-	-	-
		Tris-HCl		-		19,9	1,2	-		39,8	5,08		-	9,9	2,5
		Tris-Glycine		-		-	-	-		-	-		-	-	-
Casca		Sodium Acetate		71,8		287,1	287,1	143,5		287,1	287,1		143,5	287,1	143,5
		Tris-HCl		140,0		140,0	140,0	140,0		140,0	140,0		140,0	140,0	140,0
		Tris-Glycine		-		-	-	-		-	-		-	-	-

Phenolic Compounds			A						B				O
Part	Extract		N		P		T		N	P		T	N	P	T
Seed	Sodium Acetate		-		-		-		-	-		-	-	-	-
	Tris-HCl		-		-		-		-	-		-	-	-	-
	Tris-Glycine		-		-		-		-	-		-	-	-	-
Pulp	Sodium Acetate		3,2		103,7		25,9		6,5	207,3		25,9	3,2	207,3	13,0
	Tris-HCl		-		14,8		0,9		-	29,6		3,7	-	7,4	1,9
	Tris-Glycine		-		-		-		-	-		-	-	-	-
Peel	Sodium Acetate		14,3		57,1		57,1		28,6	57,1		57,1	28,6	57,1	28,6
	Tris-HCl		124,9		124,9		124,9		124,9	124,9		124,9	124,9	124,9	124,9
	Tris-Glycine		-		-		-		-	-		-	-	-	-

Brasil