Transglutaminase Catalysis of Modified Whey Protein Dispersions

被引:5
|
作者
Clare, Debra A. [1 ]
Daubert, Christopher R. [1 ]
机构
[1] N Carolina State Univ, Dept Food Bioproc & Nutr Sci, Raleigh, NC 27695 USA
关键词
enzyme modification; functionality; glycoprotein formation; rheology-apparent viscosity; transglutaminase; whey protein; TECHNO-FUNCTIONAL PROPERTIES; ENZYMATIC CROSS-LINKING; MICROBIAL TRANSGLUTAMINASE; MILK-PROTEINS; PHYSICAL-PROPERTIES; LOW PH; POLYMERIZATION; INGREDIENT; ISOLATE; GELATION;
D O I
10.1111/j.1750-3841.2010.01605.x
中图分类号
TS2 [食品工业];
学科分类号
0832 ;
摘要
Transglutaminase ( TGase) cross-linking reactions were accomplished using a heat-modified whey protein concentrate (mWPC) substrate after pH adjustment to 8. Based on earlier reports, the degree of lactosylation with respect to beta-lactoglobulin was lower in mWPC dispersions than measured in commercial whey concentrate (cWPC) protein solutions. In this study, a higher concentration of free sulfhydryl groups was detected in soluble supernatant fractions. Both factors potentially impact the availability of reactive lysine/glutaminyl residues required for TGase reactivity. The addition of 10 mM dithiothreitol (DTT) to the substrate mix, CBZ-glutaminyl glycine and hydroxylamine, revealed a 3.6-fold increase in TGase activity, likely due in part to maintenance of the catalytic cysteine residue in a reduced state. Furthermore, inclusion of DTT to mWPC dispersions significantly raised the apparent viscosity, independently of enzyme modification, while the rate of polymerization increased 2-fold based on OPA assay measurements. Limited cross-linking slightly increased the apparent viscosity, whereas extensive coupling lowered these values compared to equivalent nonenzyme-treated mWPC samples. Carbohydrate-staining revealed formation of glyco-polymers due to covalent linkages between glucosamine and mWPC proteins after TGase processing. Again, the apparent viscosity decreased after extensive enzymatic modification. Larger particles, sized 11.28 mu m, were observed in the structural matrix of TGase-mWPC-fixed samples compared to 8 mu m particles in control mWPC samples as viewed in scanning electron micrographs. Ultimately, the functional characteristics of TGase-mWPC ingredients may be custom-designed to deliver alternative functional attributes by adjusting the experimental reaction conditions under which catalysis is achieved. Practical Application: Taken together, these results suggest that unique TGase-mWPC and/or TGase-mWPC-glucosamine ingredients may be designed to provide novel, value-added, polymeric/glyco-polymeric protein products that afford added benefit for the milk industry.
引用
收藏
页码:C369 / C377
页数:9
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