Test procedures were developed for measuring the residual milk clotting activity of a protease produced by Endothia parasitica in curd and viii whey separated from freshly coagulated milk. A substrate was prepared by reconstituting 6 g low heat nonfat dry milk in 500 ml buffer containing 50 ml 0.5M cacodylic acid, 50 ml 0.2M CaCl2 , 30 ml 0.2M triethanolamine and 370 ml double distilled water. The substrate was stored at 2 to 4 C for 20 hours before use. Two milliliters of whey or supernatant from centrifuged curd-water slurries were inoculated into 25 ml of substrate at 30 C and the coagulation time noted, and compared with that produced by a known dilution of a standard enzyme solution.
Endothia parasitica curd formed at pH 6.7 contained 45 per cent of the enzyme activity added to 454 g milk hut when formed at pH 5.2 the curd contained only 25 per cent. ix The recovery of Endothia parasitica protease in curd was made by preparing a 1:5 curd-water slurry, adjusting to pH 5.4, filtering and testing the filterate.
| Identifer | oai:union.ndltd.org:UTAHS/oai:digitalcommons.usu.edu:etd-6180 |
| Date | 01 May 1974 |
| Creators | Patel, Raman B. |
| Publisher | DigitalCommons@USU |
| Source Sets | Utah State University |
| Detected Language | English |
| Type | text |
| Format | application/pdf |
| Source | All Graduate Theses and Dissertations |
| Rights | Copyright for this work is held by the author. Transmission or reproduction of materials protected by copyright beyond that allowed by fair use requires the written permission of the copyright owners. Works not in the public domain cannot be commercially exploited without permission of the copyright owner. Responsibility for any use rests exclusively with the user. For more information contact digitalcommons@usu.edu. |
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