This study analysed the effect of cleaning intensity of the abdominal cavity and storage temperature from slaughter to the end of processing on the quality of farmed salmon (Salmo salar L.) fillets. These two parameters were manipulated in an experimental setup using in total thirty salmon with an average weight of 4.2 kg. The experiment was designed to imitate realistic scenarios in a normal production process in the Faroe Islands. The salmon stored at low temperatures had an average muscle temperature of 4.65°C, whereas the salmon stored at ambient temperature had an average muscle temperature of 11.27°C. After the salmon were gutted to remove all viscera except the kidney, the abdominal cavity was either rinsed lightly or meticulously cleansed of kidneys, all blood and bodily fluids. A wide range of quality and production parameters were measured either straight after cleaning or after the salmon had been stored in chipped ice at 1.5°C for 7 days. All measured parameters were analysed for possible correlations by principal component analysis (PCA). Blood and remains left in the abdominal cavity were shown to have a significant negative effect on fillet firmness (P < 0.01) and gaping (P < 0.01). The different storage temperatures between slaughter and gutting, tested in this experiment, did not significantly affect fillet firmness or gaping. However, the fillet colour showed significant negative correlation (P < 0.01) with the storage temperatures applied.
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In the Atlantic salmon (Salmo salar) aquaculture industry, gaping (the separation
of muscle bundles
from the connective tissue) is a major quality problem. This study
characterized chondroitin sulfate (CS) and heparan sulfate (HS) in
the connective tissue of intact and gaping salmon fillets from 30
salmon by mass spectrometry. Statistical difference was detected between
gaping and intact tissues only when comparing pairwise samples from
the same individual (n = 10). The gaping tissue had
a lower content of monosulfated CS disaccharides (p = 0.027), and the relative distribution of CS disaccharides was
significantly different (p < 0.05). The HS chains
were short (average = 14.09, SD = 4.91), and the intact tissue seemed
to have a more uniform HS chain structure compared to the gaping tissue.
Time-series samples from the same individuals are recommended for
future research to improve the understanding of reasons and implications
of these differences.
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