Common Molecular Features among Amaranth Storage Proteins

Abstract: The structure of albumin 2 protein fraction of amaranth was investigated. It was formed by several major polypeptide subunits of molecular masses of 52.3 ± 0.8, 54 ± 2, and 56 ± 1 kDa. The former and the latter subunits were composed of a peptide of molecular mass between 31 and 38 kDa linked by S−S bonds with another peptide of molecular mass between 19 and 23 kDa. The 54 kDa subunit together with the 31−38 and 19−23 kDa subunits formed S−S-linked aggregated polypeptides. Lyophilized albumin 2 was highly poly… Show more

“…Table 2 depicts the denaturation temperatures and enthalpies (T d y ΔH d ) of amaranth protein isolates in either native state (0.1 MPa) or treated with HP (200, 400 and 600 MPa) at different protein concentrations (1%, 5% and 10%). The native isolate exhibited the two characteristic endotherms, one at 70.7°C with an enthalpy of 4.1 J g − 1 that can be attributed to the denaturation of albumins and a minor globulin fraction (globulin-7S), and a second one at 98.6°C with an enthalpy of 5.7 J g − 1 corresponding to the denaturation of the protein fractions globulin-11S, globulin-P and glutenins (Avanza & Añón, 2007;Martínez et al, 1997).…”

“…The polypeptide composition of samples was analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) using a separating gel (12% w/v in polyacrylamide) with a stacking gel (4% w/v in polyacrylamide) in a minislabs system (Bio-Rad Mini-Protean II Model) (Martínez, Castellani, & Añón, 1997). The following continuous buffers system were used: 0.375 mol L − 1 Tris-HCl, 1 g L − 1 SDS, pH 8.8, for the separating gel; 0.025 mol L − 1 Tris-HCl, 0.192 mol L − 1 glycine and 1 g L − 1 SDS, pH 8.3, for the running buffer; and 0.125 mol L − 1 Tris-HCl, 200 ml L − 1 glycerol, 10 g L − 1 SDS, 0.5 g L − 1 bromophenol blue (p.a., Sigma Chemical Co.), pH 6.8, as sample buffer.…”

Physicochemical and structural properties of amaranth protein isolates treated with high pressure

“…Table 2 depicts the denaturation temperatures and enthalpies (T d y ΔH d ) of amaranth protein isolates in either native state (0.1 MPa) or treated with HP (200, 400 and 600 MPa) at different protein concentrations (1%, 5% and 10%). The native isolate exhibited the two characteristic endotherms, one at 70.7°C with an enthalpy of 4.1 J g − 1 that can be attributed to the denaturation of albumins and a minor globulin fraction (globulin-7S), and a second one at 98.6°C with an enthalpy of 5.7 J g − 1 corresponding to the denaturation of the protein fractions globulin-11S, globulin-P and glutenins (Avanza & Añón, 2007;Martínez et al, 1997).…”

“…The polypeptide composition of samples was analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) using a separating gel (12% w/v in polyacrylamide) with a stacking gel (4% w/v in polyacrylamide) in a minislabs system (Bio-Rad Mini-Protean II Model) (Martínez, Castellani, & Añón, 1997). The following continuous buffers system were used: 0.375 mol L − 1 Tris-HCl, 1 g L − 1 SDS, pH 8.8, for the separating gel; 0.025 mol L − 1 Tris-HCl, 0.192 mol L − 1 glycine and 1 g L − 1 SDS, pH 8.3, for the running buffer; and 0.125 mol L − 1 Tris-HCl, 200 ml L − 1 glycerol, 10 g L − 1 SDS, 0.5 g L − 1 bromophenol blue (p.a., Sigma Chemical Co.), pH 6.8, as sample buffer.…”

Physicochemical and structural properties of amaranth protein isolates treated with high pressure

“…There was a significant presence of peptides with molecular mass lower than 10 kDa in Is (about a 78% of the total protein mass), including very small peptides (about a 3.5% of the total protein mass) ( Table 5). The polypeptide composition of the Is fraction cannot be compared with those currently described for amaranth isolates (Martinez & Añón, 1996, Martínez, Castellani and Añón 1997, Scilingo, Molina-Ortiz, Martínez and Añón, 2002 because it contains only proteins and polypeptides soluble in phosphate buffer at pH 7.8.…”

Amaranth proteins as a source of antioxidant peptides: Effect of proteolysis

“…Así, las fracciones mayoritarias constituidas por proteínas de peso molecular altos fueron de 300 kDa (fracción A), alrededor de 180 kDa (fracción B), 120 kDa (fracción C), entre 40 y 50 kDa (fracción D), entre 20 y 30 kDa (fracción E) y otras por debajo de 10 kDa (fracciones F, G y H). Se ha descrito la presencia en las semillas de amaranto de una proteína de reserva semejante a la legumina de las leguminosas con un peso mayor de 300 kDa y denominada amarantina (Martinez et al, 1997). Esta proteína tiene la …”

“…Por un lado un grupo bien definido entre 50 y 64 kDa. Se ha sugerido que estos péptidos pueden representar una forma inmadura de subunidades α−β componentes de la amarantina que, por causas desconocidas, no se disocia en los péptidos α y β tras el tratamiento con β-mercaptoetanol (Martinez et al, 1997). Otro grupo de péptidos está constituido por moléculas con un peso entre 33 y 37 kDa.…”

Seed protein characterisation of eleven species of amaranthus