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A M Fauzi

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Author-ID : 264772

Agriculture, Biological Sciences & Forestry

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Articles

Application of Electrical Properties to Differentiate Lard from Tallow and Palm Oil . Sucipto; T Djatna; . Irzaman; Tun Tedja I; A M Fauzi
Media Peternakan Vol. 36 No. 1 (2013): Media Peternakan
Publisher : Faculty of Animal Science, Bogor Agricultural University

This study aimed to differentiate lard from tallow and palm oil based on its electrical properties, namely conductance, impedance and capacitance. These properties were measured at spectra frequencies of 4.20 to 5.00 MHz in room temperature (26-27 oC). Statistic multivariate that consist on principal component analysis (PCA) and cluster analysis (CA) were used to evaluate the data. The results showed that lard and tallow can be differentiated using whole parameters electrical properties of materials. On the other hand, lard and palm oil can only be differentiated using part of the material electrical properties. Good performance of differentiation process was obtained using PCA model at 4.91 to 4.98 MHz. The first two components of PCA, which was derived from conductance, impedance and capacitance, contributed more than 90% of the total variances. CA showed that lard and tallow are different groups based on the Euclidean distance of each electrical properties. This technique can be potentially developed as an electrical sensor for differentiation lard to tallow and palm oil.

Produksi dan stabilisasi desaturase dari Absidia corymbifera Production and stabilization of desaturases from Absidia corymbifera . TRI-PANJI; . SUHARYANTO; A W PAULUS; K SYAMSU; A M FAUZI
E-Journal Menara Perkebunan Vol 70, No 2: Desember 2002
Publisher : INDONESIAN RESEARCH INSTITUTE FOR BIOTECHNOLOGY AND BIOINDUSTRY

SummaryDesaturases are enzymes which catalyze desaturation process on carbon chain of fatty acids into unsaturated fatty acids useful for healthy oil. Desaturases could be produced from Absidia corymbifera and applied for increasing unsaturation level and crude palm oil (CPO) quality. Desaturases have been known as very unstable enzymes. The objective this research was to determine carbon sources and culture time for optimum desaturase production, fatty acid composition resulted from desaturase bioconversion, and methods for stabilization of desaturase from A. corymbifera. Results showed that desaturases from A. corymbifera are intracellular enzymes that reached the highest activity in Serrano-Careon medium with C sources of a mixture of sucrose and paraffin (0.14 U/mL) and C sources of molasses (0.11 U/mL) incubated for 76 and 120 hours respectively. Activity of ∆6 and ∆12 desaturases have been detected in culture filtrate of A. corymbifera. Activiy of ∆12 desaturase was confirmed by increasing of linoleic acid in CPO incubated with culture filtrate and biomass extract, while activity of ∆6 was detected by its conversion as much as 66.48 % linoleic acid into gamma linolenic acid (GLA) that having high economic value. Precipitation of culture filtrate and lipid extraction of biomass were unable to stabilize desaturases. Desaturase degradation rate could be inhibited by isolation and washing of microsome fraction using high salt buffer. This method could stabilize desaturases 70-80% from initial activity at storage temperature 25o C and 50 o C for 6 hours. RingkasanDesaturase merupakan enzim yang berperan dalam proses desaturasi rantai karbon asam lemak menjadi asam lemak tak jenuh yang banyak manfaatnya bagi kesehatan. Desaturase dapat dihasilkan dari Absidia corymbifera dan diamplifikasikan untuk peningkatan ketidakjenuhan dan kualitas minyak sawit mentah (CPO). Enzim desaturase dikenal sangat tidak stabil. Penelitian bertujuan menetapkan sumber karbon dan waktu kultur yang memberikan aktivitas desaturase tertinggi, komposisi asam lemak hasil konversi desaturase dan cara menstabilkan desaturase dari A. corymbifera. Hasil penelitian menunjukkan bahwa desaturase dari A. corymbifera merupakan enzim intraselular yang mencapai aktivitas tertinggi pada medium Serrano-Careon dengan sumber karbon campuran sukrosa dan parafin (0,14 U/mL) dan sumber karbon molases (0,11 U/mL) masingmasing pada inkubasi selama 76 dan 120 jam. Aktivitas ∆6 dan ∆12 desaturase terdeteksi pada cairan fermentasi A. corymbifera. Aktivitas ∆12 desaturase terdeteksi dari peningkatan persentase asam linoleat pada CPO yang telah diinkubasi dengan cairan fermentasi atau ekstrak biomassa, sedangkan aktivitas ∆6 desaturase terdeteksi dari dikonversinya sebesar 66,48% asam linoleat menjadi asam gamma linolenat (GLA) yang memiliki potensi nilai ekonomis lebih tinggi. Pengendapan filtrat kultur fermentasi dan ekstraksi lipida biomassa tidak mampu menstabilkan desaturase. Laju degradasi desaturase dapat dihambat dengan cara isolasi dan pencucian fraksi mikrosom dengan bufer garam. Cara tersebut dapat mempertahankan aktivitas desaturase 70–80% pada penyimpanan suhu 25o C dan 50o C selama enam jam.

Produksi dan stabilisasi desaturase dari Absidia corymbifera Production and stabilization of desaturases from Absidia corymbifera . TRI-PANJI; . SUHARYANTO; A W PAULUS; K SYAMSU; A M FAUZI
Menara Perkebunan Vol. 70 No. 2: 70 (2), 2002
Publisher : INDONESIAN OIL PALM RESEARCH INSTITUTE

Show Abstract | Download Original | Original Source | Check in Google Scholar | DOI: 10.22302/iribb.jur.mp.v70i2.129

SummaryDesaturases are enzymes which catalyze desaturation process on carbon chain of fatty acids into unsaturated fatty acids useful for healthy oil. Desaturases could be produced from Absidia corymbifera and applied for increasing unsaturation level and crude palm oil (CPO) quality. Desaturases have been known as very unstable enzymes. The objective this research was to determine carbon sources and culture time for optimum desaturase production, fatty acid composition resulted from desaturase bioconversion, and methods for stabilization of desaturase from A. corymbifera. Results showed that desaturases from A. corymbifera are intracellular enzymes that reached the highest activity in Serrano-Careon medium with C sources of a mixture of sucrose and paraffin (0.14 U/mL) and C sources of molasses (0.11 U/mL) incubated for 76 and 120 hours respectively. Activity of ∆6 and ∆12 desaturases have been detected in culture filtrate of A. corymbifera. Activiy of ∆12 desaturase was confirmed by increasing of linoleic acid in CPO incubated with culture filtrate and biomass extract, while activity of ∆6 was detected by its conversion as much as 66.48 % linoleic acid into gamma linolenic acid (GLA) that having high economic value. Precipitation of culture filtrate and lipid extraction of biomass were unable to stabilize desaturases. Desaturase degradation rate could be inhibited by isolation and washing of microsome fraction using high salt buffer. This method could stabilize desaturases 70-80% from initial activity at storage temperature 25o C and 50 o C for 6 hours. RingkasanDesaturase merupakan enzim yang berperan dalam proses desaturasi rantai karbon asam lemak menjadi asam lemak tak jenuh yang banyak manfaatnya bagi kesehatan. Desaturase dapat dihasilkan dari Absidia corymbifera dan diamplifikasikan untuk peningkatan ketidakjenuhan dan kualitas minyak sawit mentah (CPO). Enzim desaturase dikenal sangat tidak stabil. Penelitian bertujuan menetapkan sumber karbon dan waktu kultur yang memberikan aktivitas desaturase tertinggi, komposisi asam lemak hasil konversi desaturase dan cara menstabilkan desaturase dari A. corymbifera. Hasil penelitian menunjukkan bahwa desaturase dari A. corymbifera merupakan enzim intraselular yang mencapai aktivitas tertinggi pada medium Serrano-Careon dengan sumber karbon campuran sukrosa dan parafin (0,14 U/mL) dan sumber karbon molases (0,11 U/mL) masingmasing pada inkubasi selama 76 dan 120 jam. Aktivitas ∆6 dan ∆12 desaturase terdeteksi pada cairan fermentasi A. corymbifera. Aktivitas ∆12 desaturase terdeteksi dari peningkatan persentase asam linoleat pada CPO yang telah diinkubasi dengan cairan fermentasi atau ekstrak biomassa, sedangkan aktivitas ∆6 desaturase terdeteksi dari dikonversinya sebesar 66,48% asam linoleat menjadi asam gamma linolenat (GLA) yang memiliki potensi nilai ekonomis lebih tinggi. Pengendapan filtrat kultur fermentasi dan ekstraksi lipida biomassa tidak mampu menstabilkan desaturase. Laju degradasi desaturase dapat dihambat dengan cara isolasi dan pencucian fraksi mikrosom dengan bufer garam. Cara tersebut dapat mempertahankan aktivitas desaturase 70–80% pada penyimpanan suhu 25o C dan 50o C selama enam jam.

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