Metal-catalyzed lipid oxidation and changes of proteins in fish |
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Authors: | Charles H. Castell |
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Affiliation: | (1) Halifax Laboratory, Fisheries Research Board of Canada, Halifax, Nova Scotia, Canada |
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Abstract: | The addition of metals to pure fats and model systems has given us a picture of the part they play in lipid oxidation. But
in complex substrates such as fish flesh the same metal ions catalyze reactions in other components of the muscle as well.
A more complete picture of deterioration is obtained when we also examine the effect of metals on the other components of
the muscle.
Although lean fish muscle contains 0.5% to 1% unsaturated lipids, during frozen storage it rarely goes rancid, as indicated
by thiobarbituric acid (TBA) values or rancid odors. The lipids do oxidize, but instead of forming carbonyls and other compounds
associated with rancidity, they become bound up in lipid-protein complexes, which accounts for the toughened texture of overstored
or poorly stored frozen fish. It has been generally accepted that the formation of these lipid-protein polymers is brought
about by a reaction between the proteins and oxidizing fatty acids. For fish of the gadoid or cod family, this is further
complicated by the enzymic production of formaldehyde, which forms in the muscle during cold storage. The direct addition
of formaldehyde to give concentrations of 0.001% to 0.05% caused marked reductions in the extractable protein of cod muscle.
Because formaldehyde and dimethylamine (DMA) are produced in the stored muscle by the same reaction, the accumulation of the
DMA can be used as a measure of this process which leads to protein insolubility. Removal of the dark lateral muscle from
the fillets before freezing reduced the production of DMA and formaldehyde during storage and resulted in less loss of extractable
protein.
One of 28 papers presented at the Symposium “Metal-Catalyzed Lipid Oxidation” presented at the ISF-AOCS, World Congress, Chicago,
September 1970. |
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