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Karakterisasi enzim α-amilase dari isolat bakteri termofil CW-1
Universitas Indonesia, 2003
TA1203
UI - Tugas Akhir  Universitas Indonesia Library
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Dewi Apriliani
Karakterisasi enzim a-Amilase ekstraseluler isolat bakteri termofil dari pusat pengolahan kompos, BSD, tangerang
"Filtrat biakan yang diperoleh dlpekatkan, kemudian dilakukan
pengujian anatisa karakterisasinya. Penelitian ini bertujuan untuk
mengisolasi dan mengkarakterisasr enzim a-amilase ekstraseluler yang
dihasilkan dari isolat bakteri SW2. Isolasi dilakukan setelah bakteri tersebut
difermentasi pada media pati kentang selama 39 jam pada temperatur 60°C,
pH 7,5 di dalam shaker incubator yang berkecapan 150 rpm. Uji karakterisasi
enzim meliputi; penentuan temperatur dan pH optimum, penentuan stabilitas
i'
termal enzim, penentuan aktivator dan inhibitor, penentuan berat molekul,
pengaruh penyimpanan terhadap stabilitas enzim serta penentuan produk
hidrolisis substrat yang dikatalisis enzim. Enzim a-amilase yang diperoleh
memiliki aktivitas optimum pada temperatur 70°C dan pH 6,0. Enzim tersebut
merupakan a-amilase logam yang bersifat termofil dan termostabil. Ion
logam yang meningkatkan aktivitas enzim adalah Na"^, \C, Ca^* dan Mn^"^
sedangkan ion logam yang menghilangkan aktivitas enzim adalah Ni^"^, Zn^*
dan Fe^"^, aktivitas enzim berkurang dengan adanya SDS dan urea. Berat
molekul enzim kasar a-amilase ekstraseluler SW2 diperkirakan sekitar 180
kDa. Reaksi hidrolisis yang dikatalisis a-amilase ini pada berbagai
polisakarida menghasilkan produk utama G1, G2, G3, G4 dan cabang
dekstrin. Uji stabilitas, terhadap penyimpanan selama 4 bulan, menunjukkan
aktivitas enzim mengalami penurunan sebesar ±29% bila disimpan pada temperatur 4°C dan penurunan sebesar ±50% bila disimpan pada temperatur
30°C."
Depok: Fakultas Matematika dan Ilmu Pengetahuan Alam Universitas Indonesia, 2003
S-Pdf
UI - Skripsi Membership  Universitas Indonesia Library
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Wibowo Mangunwardoyo
Isolasi bakteri termofil dari tanah
Depok: Fakultas Matematika dan Ilmu Pengetahuan Alam Universitas Indonesia, 1983
LP-pdf
UI - Laporan Penelitian  Universitas Indonesia Library
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Wangi Firdausi
Karakterisasi nzim sukrase dari isolat-isolat bakteri asam laktat penghasil eksopoliskarida dengan sds-page
"Eksopolisakarida (EPS) yang diproduksi dari bakteri asam laktat (BAL) memiliki nilai ekonomis yang penting karena berguna bagi industri makanan, farmasi dan kesehatan. Untuk mensintesis EPS dari substrat berupa sukrosa, BAL menggunakan suatu enzim ekstraselular berukuran besar yaitu enzim sukrase. Dari penelitian terdahulu, telah diketahui bahwa beberapa isolatisolat BAL mengandung gen-gen sukrase seperti gtf dan ftf yang berturutturut menyandikan glukansukrase dan fruktansukrase. Penelitian ini bertujuan untuk melihat aktivitas dari enzim-enzim sukrase pada beberapa isolat-isolat BAL yang secara molekuler telah diketahui memiliki gen-gen sukrase. Supernatan dan pelet sel dari isolat-isolat BAL tersebut dianalisis dengan menggunakan elektroforesis gel SDS poliakrilamid (SDS-PAGE).
Dengan melakukan SDS-PAGE menggunakan penanda protein, ukuran molekuler dari enzim dapat diperkirakan, dan dengan menginkubasi gel dalam buffer sukrosa dan staining dengan pereaksi Schiff asam periodat, EPS yang berupa glukan dan/atau fruktan yang diproduksi oleh enzim-enzim tersebut dapat diamati. Semua isolat BAL yang digunakan dalam penelitian ini, yaitu Weisella confusa MBF 8-1, W. confusa MBF 8-2, Leuconostoc mesenteroides MBF 3-1 dan W. confusa MBF PDG10(1) menunjukkan adanya aktivitas-aktivitas sukrase pada ukuran yang bervariasi, mulai dari 10 hingga 43 kDa."
Depok: Fakultas Matematika dan Ilmu Pengetahuan Alam Universitas Indonesia, 2009
S32657
UI - Skripsi Open  Universitas Indonesia Library
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R. Nida Sopiah
Isolasi, Identifikasi, dan Karakterisasi Isolat Bakteri dari Limbah Cangkang Udang (Penaeus Merguensis) dan Rajungan (Portunus Pelagicus)
Depok: Fakultas Matematika dan Ilmu Pengetahuan Alam Universitas Indonesia, 2002
T39898
UI - Tesis Membership  Universitas Indonesia Library
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Suwarti
Isolasi bakteri dan karakterisasi parsial enzim oksidoreduktase dari Situ Agathis, Kampus Universitas Indonesia, Depok
"Oxydoreductases are enzymes which catalyze oxidation-reduction reaction of their corresponding substrates. Oxydoreductase enzymes from many microorganisms had become major focus of research during last decades. This reaction had been utilized in biosensor (Yuhashi et al. 2005), biotransformation and biofuel (Zu et al. 2006). In the field of biosensor, glucose dehydrogenase application as self-blood glucose monitoring had evolved through several generation to enhance its sensitivity and specificity (Witarto et al. 1997).
Oxydoreductase involve cofactor in their active sites. According to Anthony (1996) among several known cofactors such nicotinamide, flavonoid, and quinone, Pyrollo Quinoline Qinone (PQQ) as the member group of quinon is one of the latest known-cofactors. PQQ differs from other cofactor since it is not covalently bond to its enzyme (Oubrie et al. 1999). PQQ ubiquitously found in all organisms from prokaryote to eukaryote (Bishop et al. 1998). Bacteria is the largest group of PQQ-oxydoreductase producing microorganisms. They successfully isolated from many habitats such: soil, water (Toyama et al. 1995), fruits (Adachi et al. 2003), plants, and in human mouth (Anesti et al. 2005). However, study on PQQ-oxydoreductase producing bacteria isolation had never been reported in Indonesia.
PQQ-Oxydoreductase bacteria are able to utilize organic substrates such glucose, ethanol, methanol, up to polyvinyl alcohol (Ameyama et al. 1985). One of the habitats which provides such organic substrates is Situ Agathis located in University of Indonesia Depok. Situ Agathis contain humic substances that could be degraded in to glucose, ethanol, methanol, also quinone.
In this study, isolation of oxydoreductase-producing bacteria from Situ Agathis University of Indonesia, Depok and characterization of oxydroreductases of selected isolates were performed. The objectives of this research are: to investigate the presence of oxydoreductase-producing bacteria, to isolate the oxydoreductases -producing bacteria, and to partially characterize oxydoreductases from Situ Agathis University of Indonesia Depok. This is the first study on bacteria isolation performed in Situ Agathis UI, Depok. Hence, this study can provide information about the oxydoreductases- producing bacteria from Situ Agathis, which located in UI, Depok. The study consists of two part: first part describe the isolation of oxydoreductase-producing bacteria from Situ Agathis. Second part describe the partial characterization of oxydoreductases which covers enzyme activity, molecular weight, and PQQ effects on the enzymes activity.
The research was carried out at the Protein Engineering Laboratory, Biotechnology Research Centre, Indonesian Institute of Science, Cibinong and the Laboratory of Microbiology, Department of Biology, University of Indonesia, Depok during February ? September 2007. The isolation of bacteria was conducted in three methods i.e : dilution, filtration using filter paper Milipore membran (0.2 μm) based on Cappucino and Sherman (2002). Isolation of oxydoreductase-producing bacteria was carried out by using selective media based on Toyama et al. (1995). The assay of oxydoreductases was performed by using Native-PAGE based on Khodijah (2002).
The result showed that 83 isolates were obtained from Situ Agathis which we assumed could produce oxydoreductase enzymes. Among those isolates, 15 isolates were randomly selected for further study e.g : five isolates which could grow in glucose as sole carbon sources by producing glucose dehdyrogenase, six isolates which could grow on ethanol as sole carbon sources by producing ethanol dehydrogenase and four isolates which could grow on methanol as sole carbon sources by producing methanol dehydrogenase. The selected isolates showed various morphotypes indicating no specific morphological character in oxydoreductase-producing bacteria.
Two oxydoreductases from selected isolates were selected to be analyzed further in second part this thesis. Those enzymes were examined for their possibility to have intracellular PQQ cofactor. Those enzymes were obtained from isolate G1H1D30 (glucose dehydrogenase) and isolate A1H2D60 (ethanol dehydrogenase). Native-PAGE result confirmed that crude extract fraction, dialyzed fraction and elution of open column chromatography of isolate G1H1D30 can produce glucose dehydrogenase and isolate A1H2D60 can produce ethanol dehdyrogenase. The molecular weight of glucose dehydrogenase subunit is about 46 kDa using SDS-PAGE.
SDS-PAGE of ethanol dehydrogenase did not show any protein band in acrylamide gel. We assumed that the amount of protein extracted from cell cytoplasm was not sufficient enough to be detected in SDS-PAGE. Cell of isolate A1H2D60 should be treated by other destruction method such as French pressure or ultrasonicator since this isolate is Gram positive bacteria which had thicker peptydoglycan layer than isolate G1H1D30 which is Gram negative bacteria.
Other characterization performed was addition of PQQ as the cofactor to investigate its effect on enzymes activity. Glucose dehydrogenase from isolate G1H1D30 was known to be PQQ dependent enzymes from its activity increased after addition of PQQ. The addition of PQQ raised the indicating no specific morphological character in oxydoreductase-producing bacteria.
Two oxydoreductases from selected isolates were selected to be analyzed further in second part this thesis. Those enzymes were examined for their possibility to have intracellular PQQ cofactor. Those enzymes were obtained from isolate G1H1D30 (glucose dehydrogenase) and isolate A1H2D60 (ethanol dehydrogenase). Native-PAGE result confirmed that crude extract fraction, dialyzed fraction and elution of open column chromatography of isolate G1H1D30 can produce glucose dehydrogenase and isolate A1H2D60 can produce ethanol dehdyrogenase. The molecular weight of glucose dehydrogenase subunit is about 46 kDa using SDS-PAGE.
SDS-PAGE of ethanol dehydrogenase did not show any protein band in acrylamide gel. We assumed that the amount of protein extracted from cell cytoplasm was not sufficient enough to be detected in SDS-PAGE. Cell of isolate A1H2D60 should be treated by other destruction method such as French pressure or ultrasonicator since this isolate is Gram positive bacteria which had thicker peptydoglycan layer than isolate G1H1D30 which is Gram negative bacteria.
Other characterization performed was addition of PQQ as the cofactor to investigate its effect on enzymes activity. Glucose dehydrogenase from isolate G1H1D30 was known to be PQQ dependent enzymes from its activity increased after addition of PQQ. The addition of PQQ raised theindicating no specific morphological character in oxydoreductase-producing bacteria.
Two oxydoreductases from selected isolates were selected to be analyzed further in second part this thesis. Those enzymes were examined for their possibility to have intracellular PQQ cofactor. Those enzymes were obtained from isolate G1H1D30 (glucose dehydrogenase) and isolate A1H2D60 (ethanol dehydrogenase). Native-PAGE result confirmed that crude extract fraction, dialyzed fraction and elution of open column chromatography of isolate G1H1D30 can produce glucose dehydrogenase and isolate A1H2D60 can produce ethanol dehdyrogenase. The molecular weight of glucose dehydrogenase subunit is about 46 kDa using SDS-PAGE.
SDS-PAGE of ethanol dehydrogenase did not show any protein band in acrylamide gel. We assumed that the amount of protein extracted from cell cytoplasm was not sufficient enough to be detected in SDS-PAGE. Cell of isolate A1H2D60 should be treated by other destruction method such as French pressure or ultrasonicator since this isolate is Gram positive bacteria which had thicker peptydoglycan layer than isolate G1H1D30 which is Gram negative bacteria.
Other characterization performed was addition of PQQ as the cofactor to investigate its effect on enzymes activity. Glucose dehydrogenase from isolate G1H1D30 was known to be PQQ dependent enzymes from its activity increased after addition of PQQ. The addition of PQQ raised theenzyme activity to eight fold from 0.102 U/mL to 0.94 U/mL of crude enzyme extract. In contrast, addition of PQQ did not give significant effect to EDH enzyme activity (activity of crude enzyme remain 0.082 U/mL in the presence and absence of PQQ). However, further study should be performed to analyze the real cofactor of EDH from isolate A1H2D60. EDH differs from GDH since it had disulphide ring which stabilize PQQ bound to its enzyme.
Hence, PQQ could remain bound to EDH as purification procedure performed. PQQ-GDH do not have any disulphide ring which could stabilize PQQ bound. This fact implicated unstable PQQ bound to GDH while isolation and purification performed."
Depok: Fakultas Matematika dan Ilmu Pengetahuan Alam Universitas Indonesia, 2008
T39491
UI - Tesis Open  Universitas Indonesia Library
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Miftahul Ilmi
Isolasi dan karakterisasi enzim kitinolitik dari bakteri asal limbah pengolahan udang
2007
T39458
UI - Tesis Membership  Universitas Indonesia Library
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Mas Gunawan Haryanto
Purifikasi dan karakterisasi enzim selulase dari isolat eschericia coli BPPTCC-EGRK2 = Purification and characterization of cellulase enzyme from eschericia coli BPPTCC-EGR2 / Mas Gunawan Haryanto
"ABSTRAK
Enzim selulase banyak digunakan dalam berbagai industri seperti industri deterjen, bioethanol, pakan ternak, tekstil dan kertas. Akan tetapi saat ini kebutuhan enzim selulase paling banyak didapat dari impor. Salah satu bakteri penghasil enzim selulase adalah Eschericia coli BPPT-CC EgRK2. Bakteri hasil rekombinasi yang dapat memproduksi enzim protein endo- 𝜷-1,4-glukanase, diteliti di dalam kultur batch untuk ditentukan parameter-parameter kinetikanya seperti konstanta Michaelis-Menten (Km) dan kecepatan maksimum (Vmax). Eschericia coli BPPT-CC EgRK2 dikultur di dalam media cair Luria Bertani. Selanjutnya dilakukan purifikasi dan karakterisasi dari enzim selulase. Purifikasi menggunakan metode kromatografi penukar ion dan filtrasi gel setelah itu dianalisis aktifitas enzim dengan substrat carboxymethyl cellulose (CMC), kadar protein menggunakan metode Bradford, berat molekul menggunakan sodium deodecyl sulfate (SDS-PAGE) dan kinetika enzim menggunakan plot Michaelis-Menten. Hasilnya menunjukkan aktivitas enzim tertinggi adalah 3.114 U/ml dan konsentrasi selulase 0.723 mg/ml. Konstanta Michaelis-Menten (Km) dan kecepatan maksimum (Vmax) untuk hidrolisis substrat CMC adalah 0.314 μmol/ml and 3.511 μmol/ml/sec. Hasil dari analisis berat molekul selulase menggunakan metode SDS-PAGE adalah 58 kDa pada 7.5% stacking gel. Hasil dari penelitian ini membuktikan bahwa Eschericia coli BPPT-CC EgRK2 menjadi sebuah sumber terbarukan dari enzim selulase untuk aplikasi pada skala industrial
ABSTRACT
Cellulase enzymes are widely used in various industries such as detergent industry, bioethanol, animal feed, textile and paper. This research is focused on characterization cellulase enzyme from bacteria. One of the bacteria producing cellulase enzyme is Eschericia coli BPPT-CC EgRK2. Recombinant bacteria that can produce protein enzymes endo- β-1,4-glucanase. Eschericia coli BPPT-CC EgRK2 is cultured in 1 litre liquid medium Luria Bertani. Because the bacteria is intracellular, need sonication to break the cell to get the cellulase enzyme. Then purification with ion exchange chromatography and gel filtration to purified the enzyme. After that analyzed the enzyme activity with carboxymethyl cellulose (CMC) substrate at different concentration, protein content analysis using Bradford method, molecular weight analysis using sodium deodecyl sulfate (SDS-PAGE) and enzyme kinetics using Michaelis-Menten plot. This results showed the highest enzyme activity is 3.11 U/ml at 2% CMC and the cellulase concentration is 0.723 mg/ml. The Michaelis-Menten constant (Km) and maximum velocity (Vmax) for CMC substrate hydrolysis is 0.314 μmol/ml and 3.511 μmol/ml/sec. The results of cellulae enzyme molecular weight is 58 kDa using SDS-PAGE with 7.5% stacking gel. The result of this research have known that Eschericia coli BPPT-CC EgRK2 become a promising renewable source for cellulase enzyme for industrial application."
2018
T51406
UI - Tesis Membership  Universitas Indonesia Library
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Sitaresmi
Ativitas amilolitik bakteri termofil bacillus sp th4
"ABSTRAK
Penggunaan mikroorganisme sebagai. sumber enzim dalam industri rneningkat, sehingga masih terus dicari strain-strain penghasil enzim yang baik. Bacillus sp. Th4 hasil isolasi dari Timur Tengah diuji aktivitas enzimnya pada suhu 45oC.
Pengujian aktivitas amilolitik dilakukan dengan mengukur kadar gula pereduksi yang terbentuk dengan menggunakan pereaksi DNS. Aktivitas proteolitik dilakukan dengan mengukur tingginya pencairan gelatin, sedangkan aktivitas lipolitik dilakukan dengan mengukur diameter zona bening yang terbentuk di sekitar koloni bakteri yang ditumbuhkan pada medium Tributirin Agar.
Hasil penelitian adalah, pada suhu 45oC: Bacillus sp. Th4 tidak memiliki aktivitas lipolitik, aktivitas proteolitik lemah, serta aktivitas amilolitik yang kuat. Hasil uji-t pada α=0,05 menunjukkan bahwa ada beda nyata antara aktivitas amilolitik pada suhu 45 dan 50°C. Pengukuran aktivitas amilolitik pada suhu 50°C menunjukkan bahwa aktivitas amilolitik lebih rendah daripada di suhu 45°C.
ABSTRACT
"
Depok: Fakultas Matematika dan Ilmu Pengetahuan Alam. Universitas Indonesia, 1990
S-Pdf
UI - Skripsi Membership  Universitas Indonesia Library
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Rossy Fitria
Optimasi produksi enzim lignolitik oleh isolat A-1 dan G. lucidum serta pemurnia parsial dan karakterisasi lakase
"Jamur pelapuk putih (JPP) isolat A-1 dan Ganoderma lucidum yang
merupakan koleksi Balai Penelitian Bioteknologi Perkebunan Indonesia
diketahui memiliki kemampuan dalam mendegradasi Tandan Kosong Kelapa
Sawit(TKKS). Sehubungan hal tersebut dilakukan pengujian terhadap A-1
dan Ganoderma lucidum untuk menghasilkan enzim lignolitik. Pengujian
aktivitas enzim lignin peroksidase (LiP), mangan peroksidase (MnP)dan
lakase eksoseluler dilakukan selama masa pertumbuhannya didalam
beberapa variasi media. Hasil pengamatan menunjukan bahwa tidak ada aktivitas MnP eksoseluler yang terdeteksi pada masing-masing isolat di
dalam medium uji, meskipun pada uji pendahuluan ekstrak miselium
Ganoderma lucidum menghasilkan aktivitas MnP endoseluler sebesar 0,66
U/mL pada media PDA. Dari seluruh medium yang diuji isolat A-1 hanya
menghasilkan lakase dengan aktivitas tertinggi pada media yang
mengandung 2% Energen cereal sebesar 1.162 U/mL pada inkubasi hari ke-
6 dengan pH pertumbuhan 5,0. Sedangkan Ganoderma lucidum hanya
menghasilkan LiP dengan aktivitas tertinggi pada media glukosa-melt-yeast
(GMY) sebesar 1.720 U/mL pada inkubasi hari ke-2 dengan pH pertumbuhan
5.5. Uji peningkatan aktivitas lakase isolat A-1 lebih lanjut terjadi pada media
yang mengandung 2% TKKS sebesar 0.38 U/mL pada inkubasi hari ke-10
dengan pH pertumbuhan 6,54. Purifikasi parsial pada kolom Sephacryl S-200
HR terhadap ekstrak enzim lakase pada medium 2%TKKS hari ke-15
menunjukan bahwa enzim lakase ter-recovery sebesar 58,23% dengan
kemurniaan 2 kalinya. Isolat A-1 menghasilkan aktivitas lakase maksimum
pada pH optimum 4,5. Aktivitas lakase tetap stabil setelah pemanasan
selama 30 menit pada temperatur kamar hingga 50oC dan menurun tajam
pada suhu 60oC. Pengaruh konsentrasi substrat ABTS terhadap aktivitas
lakase isolat A-1 menghasilkan harga KM dan Vmaks masing-masing 0.15mM
dan 0.56 U/mL."
Depok: [Fakultas Matematika dan Ilmu Pengetahuan Alam. Universitas Indonesia, Universitas Indonesia], [2005, 2005]
S-Pdf
UI - Skripsi Membership  Universitas Indonesia Library
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