Amylase production studies and partial purification of amylolytic enzyme from Enterococcus Faecium DMF78 / Glaiza L. Tabanao

By: Material type: TextTextLanguage: English Publication details: 2008Description: 45 leavesSubject(s): Dissertation note: Thesis (BS Food Technology) -- University of the Philippines Mindanao, 2008 Abstract: The amylolytic enzyme of Enterococcus faecium DMF78 was isolated and partially purified from the fermentation broth. Amylase production and enzyme assay conditions were optimized prior to purification. Amylase production was found to be better at the following cultural conditions: raw sago starch as carbon source and incubation without shaking. The highest productivity of amylases was obtained at the first hour of incubation and generally declined thereafter. Prior to the purification protocol was sequenced as follows: ammonium sulfate precipitation at 90% saturation, dialysis and anion-exchange chromatography (DEAE-cellulose). The partially purified amylase preparation had a purification-fold of 1.57, a recovery of 24.69% and specific activity of 115.31 U/mg. Purity was monitored using SDS-PAGE analysis but distinct protein bands were not observed probably due to very dilute samples.
List(s) this item appears in: BS Food Technology
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Item type Current library Collection Call number Status Date due Barcode
Thesis Thesis University Library Theses Room-Use Only LG993.5 2008 F62 T32 (Browse shelf(Opens below)) Available 3UPML00012216
Thesis Thesis University Library Archives and Records Non-Circulating LG993.5 2008 F62 T32 (Browse shelf(Opens below)) Preservation Copy 3UPML00032438

Thesis (BS Food Technology) -- University of the Philippines Mindanao, 2008

The amylolytic enzyme of Enterococcus faecium DMF78 was isolated and partially purified from the fermentation broth. Amylase production and enzyme assay conditions were optimized prior to purification. Amylase production was found to be better at the following cultural conditions: raw sago starch as carbon source and incubation without shaking. The highest productivity of amylases was obtained at the first hour of incubation and generally declined thereafter. Prior to the purification protocol was sequenced as follows: ammonium sulfate precipitation at 90% saturation, dialysis and anion-exchange chromatography (DEAE-cellulose). The partially purified amylase preparation had a purification-fold of 1.57, a recovery of 24.69% and specific activity of 115.31 U/mg. Purity was monitored using SDS-PAGE analysis but distinct protein bands were not observed probably due to very dilute samples.

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