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ning reactions during storage of low‐moisture Australian sultanas: Effects of vine nitrogen nutrition on subsequent arginine‐mediated Maillard reactions during storage of dried fruit
Author(s) -
FRANK DAMIAN,
GOULD IAN,
MILLIKAN MARY
Publication year - 2005
Publication title -
australian journal of grape and wine research
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.65
H-Index - 77
eISSN - 1755-0238
pISSN - 1322-7130
DOI - 10.1111/j.1755-0238.2005.tb00275.x
Subject(s) - browning , chemistry , maillard reaction , food science , nitrogen , horticulture , organic chemistry , biology
Ten‐year old Vitis Vinifera L. cv. Sultana (Thompson Seedless) grape vines were transferred into large cement pots in low nitrate soil and supplemented with four levels of nitrogen application in the form of ammonium nitrate as follows: 0 g ( N 0 ), 8.5 g ( N 1 ), 17.0 g ( N 2 ) and 25.0 g ( N 3 ). Grapes were harvested from each nitrogen treatment, dipped and dried to low moisture (˜11.4%) and subsequently stored for 10 months at 10 o C and at 30 o C in either the presence or absence of oxygen. The pre‐storage concentration of free arginine, free‐proline and total protein in the dried sultanas increased with soil nitrogen application. Skin‐polyphenoloxidase (PPO) activity was higher in sultanas with added soil nitrogen ( N 1 , N 2 , N 3 ), however pre‐storage differences in total phenolics, and the PPO substrate, trans‐ caftaric acid, were not significantly different. After 10 months storage at 30 o C significant browning was observed in both the presence and absence of oxygen. Greater browning corresponded to higher soil‐nitrogen application rates. The concentration of skin trans‐ caftaric acid did not decrease in N 0 , N 1 or N 2 after 10 months at 30 o C, in either the presence or absence of oxygen, although some decreases were measured in the highest nitrogen sultanas ( N 3 ). While PPO oxidation of the phenolic substrate trans‐ caftaric acid was not the primary route to browning, a number of Maillard reaction products (MRP) were present in both sultanas and arginine‐glucose model systems. Those products were separated via reverse phase HPLC and partially characterised by UV‐diode array spectroscopy. The lack of oxidation of trans‐ caftaric acid observed in the nitrogen storage trial was confirmed in an accelerated browning experiment in low‐moisture sultanas, where despite browning at 50 o C after 12 days, no decreases in this primary substrate for PPO‐mediated oxidation were measured.