S. Lamb rennet pastes were prepared by the procedure most commonly used by Idiazabal cheese manufacturers. We studied the effects on their coagulating and lipolytic activities of the state of the stomach at the time of death (full of milk or empty), the amount of NaCl added, the origin of the lambs and paste storage time. Coagulating activities were generally between 155 and 363 units\g tissue. Pastes prepared from stomachs of lambs from slaughterhouse flocks had significantly higher coagulating activities than those of lambs from separate flocks. No significant decrease in coagulating activity was observed after 1 year storage at 4 mC. Chymosin represented 75-80 % of the total coagulating activity with the remainder being pepsin. Rennet paste extracts with pH 4n7 did not have increased coagulating activities when their pH was lowered to 2n0, while those with pH 5n2 had activities 1n5-fold those before treatment. Lipase activity was higher in extracts of rennet pastes prepared using the stomachs of lambs that arrived at the slaughterhouse in the morning just prior to slaughter than in those prepared with the stomachs of lambs that had arrived on the previous evening. However, the reverse was the case for esterase activity. Activating the coagulating activity by pH cycling completely destroyed both lipolytic activities. Storage at 4 mC for 1 year did not affect esterase activity but lipase activity decreased substantially after 4-5 months. Lipase, but not esterase, activity was responsible for the liberation of short-chain free fatty acids from ovine milk fat.
Two methods were compared for the determination of free fatty acids
(FFA) from acetic to long-chain acids in samples with a large excess of
triacylglycerols (TG) (1[ratio ]200, w/w), such as cheese and other
dairy products. In
method 1, after fat extraction, FFA were separated from TG by aminopropyl-bonded
phase chromatography, injecting the fraction containing FFA directly into
the gas chromatograph. In method 2, extracted fat was treated with
tetramethylammonium hydroxide, the methyl ester derivatives being formed in the
injector. Cheese samples and standard mixtures of FFA and TG in different
proportions were analysed by both methods. The cheese sample contained 2·4
times more FFA when analysed by method 2 as compared with the result obtained with
method 1. The composition of the standard mixtures analysed by method 1 closely
reflected that of the original mixture and gave 90–100% recovery of FFA,
regardless
of their chain length and the ratio of FFA[ratio ]TG (1[ratio ]1 or 1[ratio ]200,
w/w). The composition
of samples with a FFA[ratio ]TG ratio of 1[ratio ]200 (w/v) was severely
distorted (as compared
with the original composition of the sample) when analysed by method 2. Varying
recoveries of FFA were also obtained, the largest differences being found for the
shorter-chain components. We conclude that the FFA fraction should be separated
from the TG fraction before derivatization and chromatographic analysis,
particularly for samples in which the FFA represent a minor fraction of the TG.
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