Methods for Analysis of Conjugated Linoleic Acids and trans-18:1 Isomers in Dairy Fats by Using a Combination of Gas Chromatography, Silver-Ion Thin-Layer Chromatography/Gas Chromatography, and Silver-Ion Liquid Chromatography

Author:

Cruz-Hernandez Cristina1,Deng Zeyuan2,Zhou Jianqiang3,Hill Arthur R4,Yurawecz Martin P5,Delmonte Pierluigi5,Mossoba Magdi M5,Dugan Michael E R6,Kramer John K G3

Affiliation:

1. Agriculture and Agri-Food Canada, Food Research Program, 93 Stone Rd West, Guelph, Ontario, Canada, and University of Guelph, Department of Food Science, Guelph, Ontario, Canada

2. Agriculture and Agri-Food Canada, Food Research Program, 93 Stone Rd West, Guelph, Ontario, Canada, and University of Nanchang, Department of Food Science, Nanchang, China

3. Agriculture and Agri-Food Canada, Food Research Program, 93 Stone Rd West, Guelph, Ontario, Canada

4. University of Guelph, Department of Food Science, Guelph, Ontario, Canada

5. U.S. Food and Drug Administration, 5100 Paint Branch Pkwy, College Park, MD

6. Agriculture and Agri-Food Canada, Lacombe Research Center, Lacombe, Alberta, Canada

Abstract

Abstract Conjugated linoleic acids (CLA) are octadecadienoic acids (18:2) that have a conjugated double-bond system. Interest in these compounds has expanded since CLA were found to be associated with a number of physiological and pathological responses such as cancer, metastases, atherosclerosis, diabetes, immunity, and body fat/protein composition. The main sources of these conjugated fatty acids are dairy fats. Rumen bacteria convert polyunsaturated fatty acids, especially linoleic and linolenic acids, to CLA and numerous trans- containing mono- and diunsaturated fatty acids. It has been established that an additional route of CLA synthesis in ruminants and monogastric animals, including humans, occurs via Δ9 desaturation of the trans-18:1 isomers. To date, a total of 6 positional CLA isomers have been found in dairy fats, each occurring in 4 geometric forms (cis,trans; trans,cis; cis,cis; and trans,trans) for a total of 24. All of these CLA isomers can be resolved only by a combination of gas chromatography (GC), using 100 m highly polar capillary columns, and silver-ion liquid chromatography, using 3 of these 25 cm columns in series. Complete analysis of all the trans-18:1 isomers requires prior isolation of trans monoenes by silver-ion thin-layer chromatography (TLC), followed by GC analysis using the same 100 m capillary columns operated at low temperatures starting from 120°C. These analytical techniques are required to assess the purity of commercial CLA preparations, because their purity will affect the interpretation of any physiological and/or biochemical response obtained. Prior assessment of CLA preparations by TLC is also recommended to determine the presence of any other impurities. The availability of pure CLA isomers will permit the evaluation and analysis of individual CLA isomers for their nutritional and biological activity in model systems, animals, and humans. These techniques are also essential to evaluate dairy fats for their content of specific CLA isomers and to help design experimental diets to increase the level of the desired CLA isomers in dairy fats. These improved techniques are further required to evaluate the CLA profile in monogastric animals fed commercial CLA preparations for CLA enrichment of animal products. This is particularly important because absorption and metabolism will alter the ingested-CLA profile in the animal fed.

Publisher

Oxford University Press (OUP)

Subject

Pharmacology,Agronomy and Crop Science,Environmental Chemistry,Food Science,Analytical Chemistry

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