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"The purification of recombinant proteins is an important stage in biopharmaceutical research. A commonly used technique is immobilized metal affinity chromatography (IMAC). One of the main advantages of this type of chromatography is that the column can easily be regenerated for subsequent purification work. The mechanism of IMAC is based on bonding between metal ions immobilized on a matrix with a specific amino acid. Because of the strong interactions of the electron donor group on the imidazole ring, histidine is often used in the IMAC purification system. Two types of commercial IMAC resin use a nitrilotriacetic acid (NTA) matrix: a nickel-based (Ni-NTA) and cobalt-based (Co-NTA), better known as TALON. This study was aim to investigate the effect of the metal ions Ni2+ and Co2+ to purify recombinant human erythropoietin (rhEPO) expressed in yeast system Pichia pastoris. The results indicated that both Ni-NTA and Co-TALON gave almost the same level of protein purity; however, Ni-NTA has a higher binding affinity than Co-TALON might be due to the higher stability complex of Ni+. The average amount of protein bound by Ni-NTA and Co-TALON was 183.5 and 38.7 μg/mL, respectively."

"Perkembangan teknologi penyuntingan genom clustered regularly interspaced short palindromic repeat (CRISPR) memberikan kemampuan pada ilmuwan untuk memodifikasi sekuens genom pada sebagian besar sel eukariot. Selain untuk insersi dan delesi gen, penelitian sistem CRISPR-Cas9 juga telah menuju ke arah perkembangan represor transkripsional artifisial CRISPR interference (CRISPRi) dengan sistem dCas9 untuk rekayasa metabolisme melalui penyuntingan metabolic pathways.  dCas9 yang merupakan turunan dari Cas9 saat ini umumnya diproduksi oleh bakteri Streptococcus pyogenes yang merupakan bakteri mesofilik dan menyebabkan Cas9 dan dCas9 yang berasal dari Sterptococcus pyogenes memiliki limitasi terhadap suhu tinggi.  Saat ini eksplorasi terhadap bakteri termofilik sebagai sumber gen Cas9-dCas9 sedang berkembang. Salah satunya adalah bakteri Geobacillus kaustophilus yang tumbuh pada suhu optimal 60˚C dan dapat hidup hingga suhu 74˚C. Dalam penelitian ini, produksi enzim dCas9 dilakukan menggunakan Escherichia coli BL21 sebagai host dan dipurifikasi Immobilized metal affinity chromatography (IMAC). Variasi pemanasan supernatant dilakukan untuk suhu 50˚C, 60˚C, dan 70˚C sebelum purifikasi. Terdapat penurunan konsentrasi protein total dengan semakin tinggi suhu pemanasan, dengan konsentrasi protein total tertinggi pada suhu 50˚C. Purifikasi dilakukan menggunakan 3 buffer elusi dengan konsentrasi imidazole berbeda (250 mM, 350 mM, dan 450 mM). Konsentrasi imidazole 350 mM pada buffer elusi menghasilkan protein dengan konsentrasi total paling tinggi. SDS PAGE silver staining dilakukan untuk melihat berat molekul protein rekombinan yang telah dipurifikasi, dan protein terpurifikasi muncul pada pita ~50 kDa.

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The development of clustered regularly interspaced short palindromic repeat (CRISPR) genome editing technology has given scientists the ability to modify the genome sequences of most eukaryotic cells. In addition to gene insertion and deletion, research on the CRISPR-Cas9 system has also led to the development of artificial transcriptional CRISPR interference repressors (CRISPRi) with the dCas9 system for metabolic engineering through editing of metabolic pathways. dCas9 which is a derivative of Cas9 is currently generally produced by Streptococcus pyogenes which is a mesophilic bacterium and causes Cas9 and dCas9 derived from Streptococcus pyogenes to have limitations against high temperatures. Currently, exploration of thermophilic bacteria as a source of Cas9-dCas9 genes is rising. One of them is the bacterium Geobacillus kaustophilus which grows at an optimal temperature of 60˚C and can live up to 74˚C. In this study dCas9 recombinant production was carried out using Escherichia coli BL21 as the host and Immobilized Metal Affinity Chromatography (IMAC) purification. Variation of supernatant heating was carried out for temperatures of 50˚C, 60 ˚C, and 70 ˚C before purification. There was a decrease in total protein concentration with higher heating temperature, with the highest total protein concentration at 50 ˚C. Purification was carried out using 3 elution buffers with varying imidazole concentrations (250 mM, 350 mM, and 450 mM). The imidazole concentration of 350 mM in the elution buffer produced fractions with the highest total protein concentration. SDS PAGE silver staining was performed to determine the molecular weight the purified fraction, and bands appeared in the ~50 kDa band."

"Sistem CRISPR-Cas9 merupakan mekanisme perlindungan bakteri terhadap materi genetik asing yang diaplikasikan secara luas dalam rekayasa genetika. Kombinasi enzim Cas9 dengan gRNA pada CRISPR-Cas9 memungkinkan terjadinya pengeditan genom terhadap target yang spesifik. Meskipun demikian, Cas9 yang dikembangkan saat ini berasal dari bakteri mesofilik sehingga rentan terdegradasi dan tidak cocok untuk aplikasi pada temperatur tinggi. Di sisi lain, bakteri termofilik Geobacillus kaustophilus telah diisolasi dari mata air panas di Cisolong, Banten, dan diidentifikasi mengandung enzim Cas9. Untuk memperoleh enzim Cas9 yang tidak terdenaturasi pada temperatur tinggi (termostabil), dilakukan uji coba produksi Cas9 rekombinan dari Geobacillus kaustophilus. Gen Cas9 yang telah dikloning pada plasmid pET43.1a ditransformasikan ke dalam Escherichia coli BL21 dan dikultur dengan konsentrasi penambahan IPTG yang bervariasi—0,05 mM, 0,20 mM, dan 0,50 mM. Hasil kultur bakteri dipanaskan pada temperatur yang bervariasi (50 °C, 60 °C, dan 70 °C) untuk mendenaturasi enzim non-termofilik. Setelah itu, sampel dipurifikasi dengan mmobilized Metal Affinity Chromatography untuk memperoleh enzim Cas9. Hasil uji Lowry menunjukkan sampel heated supernatant dengan konsentrasi IPTG 0,05 mM dan temperatur pemanasan 50 °C memiliki konsentrasi protein tertinggi dan hasil purifikasinya memiliki konsentrasi Cas9 sebesar 42,6 μg/mL. Identifikasi protein dengan uji SDS-PAGE menunjukkan ukuran protein hasil purifikasi sebesar 52,61 kDa.

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The CRISPR-Cas9 system is a bacterial defense mechanism against foreign genetic material that is broadly applied in genetic engineering. The combination of Cas9 enzyme and gRNA in CRISPR-Cas9 allows genome editing of specific targets. However, the currently developed Cas9 originated from mesophilic bacteria, making it susceptible to degradation and unsuitable for applications requiring elevated temperatures. On the other hand, the thermophilic bacterium, Geobacillus kaustophilus, was isolated from a hot spring in Cisolong, Banten, and identified as containing the Cas9 enzyme. To obtain undenatured Cas9 enzymes at high temperatures (thermostable), a production test of recombinant Cas9 from Geobacillus kaustophilus was carried out. The Cas9 gene cloned on the pET43.1a plasmid was transformed into Escherichia coli BL21 and cultured under various IPTG addition concentrations—0.05 mM, 0.20 mM, and 0.50 mM. The bacterial cultures were heated at various temperatures (50 °C, 60 °C, and 70 °C) to denature unwanted non-thermophilic enzymes. Thereafter, the samples were purified using Immobilized Metal Affinity Chromatography to obtain Cas9 enzyme. Lowry protein assay results showed that the heated supernatant sample with 0.05 mM IPTG addition and 50 °C heating temperature has the highest protein concentration, and the purified sample yielded a Cas9 concentration of 42.6 μg/mL. Protein identification with SDS-PAGE revealed a purified protein size of 52.61 kDa"

"ABSTRACTFor clinical purposes, pure protein and identification of carbohydrate structure from recombinant erythropoietin are needed. Purification was done by Immobilized Metal Affinity Chromatography (IMAC) column charged with Ni2+(His-Trap affinity chromatography) and continued with gel filtration chromatogram phy column to get purer protein. The carbohydrate group which is o ligosaccharide from the resulting pure protein then can be recognized by using N- and O-glycosidase. Pure oligosaccharide was hydrolyzed to produce various monosaccharide through incubation with 4 N HCl in 100oC temperature for 6 hours and the result was applied on High Performance Liquid Chromatography (HPLC) column to learn the composition of its monosaccharide."

"Protein apoptin dari virus anemia ayam telah diteliti memiliki potensi yang baik sebagai pendeteksi dini sel kanker. Keberhasilan produksi apoptin yang tidak lagi berupa badan inklusi telah memberikan harapan lebih besar untuk melakukan optimasi produksi protein apoptin rekombinan ini. Sel rekombinan apoptin yang berhasil diproduksi dalam skala besar dengan menggunakan inang Bacillus subtilis 168 pOXGW-apop-2His8Arg, pOGW-apop-12His dalam berbagai variasi kondisi kultivasi (konsentrasi substrat penginduksi, laju aerasi, dan laju agitasi) kemudian dipurifikasi menggunakan metode IMAC dalam kolom afinitas (HisTrap FF 5 mL) yang berisi ion logam transisi Ni2+ dengan menggunakan instrumen AKTA Prime Plus. Secara rata-rata, hasil purifikasi menunjukkan bahwa elusi apoptin rekombinan terjadi ketika nilai konduktivitas berada pada angka 15,85 mS/cm, dengan konsentrasi imidazole berada pada kisaran nilai 76% - 88% (384,8-442,4 mM), yang terlihat dari grafik gradien elusi. Pengukuran konsentrasi protein apoptin dengan menggunakan metode Bradford menujukkan bahwa konsentrasi terbesar diperoleh pada sampel dengan sistem agitasi 250 rpm dan laju aerasi 0,5 Nl/menit, dengan besar konsentrasi 0,0507 mg/ml. Hasil purifikasi berhasil dideteksi menggunakan SDS-PAGE 12% dengan hasil pita protein terlihat di area 15 kDa dan 58,5 kDa untuk semua sampel.

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Apoptin has been known to be having a great potency for cancer detection. The success of apoptin production which is not in inclusion body form anymore has given a bigger hope to optimize its production. Recombinant apoptin cells which was succesful to be cultivated in large scale using Bacillus subtilis 168 pOXGW-apop-12His8Arg, pOGW-apop-12His vector in various cultivation condition (aeration rate, agitation rate) then purified using IMAC method in Ni2+-loaded affinity column (HisTrap FF 5ml) and proceeded in AKTA Prime Plus instrument. Averagely, purifcation result showed that the elution of apoptin recombinant protein happened when the conductivity value at 15,85 mS/cm, with imidazole concentration lied around 76%-88% (384,8-442,4 mM), which could be seen from elusion gradient curve. The measurement of apoptin protein concentration using Bradford method showed that the biggest concentration was obtained from the sample with agitation rate 250 rpm and aeration rate 0,5 Nl/min, and the value is 0,0507 mg/ml. Purification yield was succesfully detected using SDS-PAGE 12%, with protein band was seen on 15 kDa and 58,5 kDa area for all samples."

"Penerapan antibodi monoklonal (mAb) anti-spike untuk digunakan dalam diagnosis SARS-CoV-2 memerlukan suatu proses purifikasi untuk mendapatkan suatu antibodi yang murni dan homogen sehingga dapat mendeteksi suatu patogen spesifik secara optimal. Penelitian ini bertujuan untuk memurnikan mAb terhadap protein spike SARS-CoV-2 dan membandingkan hasil purifikasi terbaik dari metode kromatografi afinitas dengan protein G dan kromatografi penukar ion sehingga diperoleh metode yang paling optimal dalam purifikasi mAb terhadap protein spike SARS-CoV-2. Purifikasi mAb anti-spike SARS-CoV-2 dilakukan menggunakan kromatografi afinitas dengan protein G dan kromatografi penukar ion. Hasil purifikasi dari kedua metode kromatografi dikarakterisasi dan diuji fungsionalitasnya menggunakan SDS-PAGE, pengukuran konsentrasi protein, ELISA indirect, dan western blot (WB). Hasil profil SDS-PAGE menunjukkan mAb hasil purifikasi menggunakan protein G pada fraksi 19GD dan 20GD memiliki profil pita protein dengan dua pita, yaitu heavy chain ~50 kDa dan light chain ~25 kDa dengan tingkat kemurnian mencapai 96%. Uji fungsionalitas dengan ELISA indirect menunjukkan fraksi 19GD dan 20GD memiliki nilai absorbansi sebesar 1,015 dan 1,021. Uji fungsionalitas dengan WB menunjukkan adanya pengikatan mAb fraksi 19GD terhadap protein RBD pada ukuran ~38 kDa. Hasil karakterisasi dan uji fungsionalitas mAb fraksi hasil purifikasi dengan resin penukar ion menunjukkan profil pita protein kontaminan, nilai absorbansi dari 0,49—0,82 , dan tidak terbentuk pita protein pada uji WB. Berdasarkan hasil tersebut, mAb anti-spike SARS-CoV-2 berhasil dimurnikan menggunakan kromatografi afinitas dengan protein G secara optimal.

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The application of anti-spike monoclonal antibody (mAb) for use in the diagnosis of SARS-CoV-2 requires a purification process to obtain a pure and homogeneous antibody so that it can detect a specific pathogen optimally. This research aims to purify anti-spike SARS-CoV-2 mAb and compare the best purification results from affinity chromatography with protein G and ion-exchange chromatography methods in order to obtain the most optimal method of purification of anti-spike SARS-CoV-2 mAb. Purification of anti-spike SARS-CoV-2 mAb was carried out using affinity chromatography with protein G and ion exchange chromatography. The purification results from both chromatographic methods were characterized and tested for functionality using SDS-PAGE, measurement of protein concentration, indirect ELISA, and western blot (WB). The results of SDS-PAGE profile showed that mAb purified using protein G in the 19GD and 20GD fractions had a protein band profile with two bands, namely heavy chain ~50 kDa and light chain ~25 kDa with a purity level of 96%. The functionality test with indirect ELISA showed that 19GD and 20GD fractions had OD values ​​of 1.015 and 1.021. Functionality test with WB showed the binding of mAb fraction 19GD to RBD protein at ~38 kDa. The results of characterization and functionality test of purified mAb fraction with ion exchange resin showed a contaminant protein band profile, absorbance values ​​from 0.49—0.82, and no protein band was formed in the WB test. Based on these results, anti-spike SARS-CoV-2 mAb was successfully purified using affinity chromatography with protein G optimally."

"Granulocyte Colony Stimulating Factor (G-CSF) merupakan faktor pertumbuhan hematopoetik yang berfungsi merangsang proliferasi dan diferensiasi neutrofil. Protein G-CSF rekombinan yang dikembangkan dan diproduksi menggunakan sel inang Escherichia coli dan Chinese Hamster Ovary (CHO) masih memiliki kelemahan, sehingga pada penelitian ini dikembangkan suatu produk biosimilar G-CSF rekombinan menggunakan sel inang Pichia pastoris. Fokus penelitian ini adalah memproduksi dan mempurifikasi protein G-CSF rekombinan. Produksi protein rekombinan dilakukan dengan menginduksi kultur menggunakan metanol konsentrasi 0,5% tiap 12 jam dan dilakukan sampling terhadap kultur pada jam ke-0, 12, 24, 36 dan 48. Hasil analisis western blot menunjukkan adanya peningkatan produksi protein rekombinan tiap 12 jam. Protein G-CSF rekombinan dipresipitasi menggunakan amonium sulfat konsentrasi 80%, kemudian didialisis. Konsentrasi protein total diukur dengan spektrofotometer menggunakan metoda Bicinchoninic Acid (BCA). Hasil pengukuran menunjukkan konsentrasi protein total tertinggi adalah sampel protein yang dipresipitasi dengan 80% amonium sulfat. Selanjutnya, purifikasi dilakukan menggunakan teknik kromatografi afinitas dengan resin Ni-NTA. Hasil analisis SDS PAGE menunjukkan protein GCSF rekombinan berukuran 18,5 kDa dan dengan analisis slot blot terdeteksi berwarna ungu.

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Granulocyte Colony Stimulating Factor (G-CSF) is a hematopoietic growth factor that acts to stimulate neutrophilic proliferation and differentiation. Recombinant protein G-CSF developed and produced using cellular host Escherichia coli and Chinese hamster ovary (CHO) still has a weakness, so that in this study we developed a bio similar product of recombinant G-CSF using cellular host Pichia pastoris. The aim of this research was to produce and purify recombinant protein G-CSF. Production of recombinant protein was done by inducing culture with methanol 0.5% every 12 hours and sampling was carried out at 0, 12, 24, 36 and 48 hours. The results of western blot analysis showed an increase the production of recombinant protein every 12 hours. Recombinant protein G-CSF was precipitated using ammonium sulfate 80% of concentration, and then dialyzed. Concentration of total protein was measured by a spectrophotometer using the Bicinchoninic Acid (BCA) method. The measurement results showed the highest concentrations of total protein was present in samples that precipitated with 80% ammonium sulfate. Furthermore, purification performed using affinity chromatography techniques with Ni-NTA resin. The results of SDS PAGE analysis showed the recombinant protein G-CSF sized 18.5 kDa and with a slot blot analysis detected a purple color."