UI - Tesis Membership :: Kembali

UI - Tesis Membership :: Kembali

Pengembangan Metode Analisis Human Insulin secara Indirect ELISA Berbasis Antibodi Poliklonal Dibandingkan dengan KCKT Fase Terbalik = Development of Human Insulin Analysis Method by Indirect ELISA Based on Polyclonal Antibody Compared to Reverse Phase HPLC

Christy Ambarsari; Herman Suryadi, supervisor; Arry Yanuar, supervisor; Ratika Rahmasari, examiner; Taufiq Indra Rukmana, examiner; Abdul Mun`im, examiner (Fakultas Farmasi Universitas Indonesia, 2022)

 Abstrak

Diabetes melitus merupakan kelainan metabolik yang ditandai hiperglikemia dimana landasan terapinya masih menggunakan human insulin. Telah banyak sediaan yang beredar, namun metode analisis yang standar dan valid belum ditetapkan di dalam negeri. Penelitian ini bertujuan untuk mengembangkan dan memvalidasi metode analisis secara indirect ELISA dibandingkan KCKT UV fase terbalik untuk determinasi sediaan. Antibodi poliklonal IgG dihasilkan dari kelinci yang diimunisasi dengan 1 mg/mL antigen human insulin rekombinan, dimurnikan melalui presipitasi dan kromatografi afinitas, dikuantitasi dengan spektrofotometer UV280nm, dikarakterisasi dengan uji Dot blot menggunakan substrat BCIP-NBT, serta dikarakterisasi melalui uji SDS-PAGE dan Western Blot dengan konsentrasi gel 7,5% dan 17,5%. Sedangkan, metode KCKT menggunakan kolom ReliantTM C-18 (4,6 x 150 mm, 5 µm), fase gerak Na2SO4 pH 2,3 : Na2SO4 pH 2,3 dalam asetonitril (55:45,v/v) rasio 38:62 v/v, standar internal etilparaben 10 µg/mL, detektor UV 215 nm, suhu kolom 40°C, laju alir 1 mL/menit, dan volume injek 20 µL. Validasi kedua metode dilakukan terhadap larutan uji yang mengandung m-kresol dan gliserol. Metode ELISA pada rentang 80,11-200,28 µg/mL (r = 0,99) dan KCKT pada 9,735-146,025 µg/ml (r = 0,9997) terbukti linear. Rekoveri pada ELISA dan KCKT adalah 99,11% ± 5,01 dan 100,71% ± 1,11, sedangkan RSD 3,91% dan 0,64%. LOD dan LOQ metode ELISA 22,05 µg/mL dan 73,51 µg/mL, serta KCKT 0,193 µg/ml dan 0,643 µg/ml. Human insulin bersifat stabil pada suhu 2-8°C selama 24 jam (ELISA) dan suhu 23°C selama 48 jam (KCKT). Kesimpulan, hasil validasi kedua metode valid dan mampu mendeterminasi human insulin tanpa berbeda siginifikan (Uji T, a0,05). 

Cannot connect to Ginger Check your internet connection or reload the browser. Disable in this text field Rephrase Rephrase current sentence Edit in Ginger Enable Ginger Cannot connect to Ginger Check your internet connection or reload the browser Disable in this text field phrase. Rephrase current sentence. Edit in Ginger Enable Ginger. Diabetes mellitus is a metabolic disorder characterized by hyperglycemia that is still treated with human insulin. Many preparations on the market, but a standard and valid analytical method has not been established in our country. This study aims to develop and validate an indirect ELISA method for determining human insulin comparative to reverse phase UV HPLC. IgG polyclonal antibodies were produced by immunizing rabbits with 1 mg/mL recombinant human insulin antigen, purified by precipitation and affinity chromatography, quantified by UV spectrophotometer 280nm, characterized by dot blot test using BCIP-NBT substrate, and characterized by SDS-PAGE and Western Blot at 7.5% and 17.5% gel concentrations. The HPLC method was performed using a Reliant TM C-18 column (4.6 x 150 mm, 5 µm), with mobile phase Na2SO4 pH 2.3: Na2SO4 pH 2.3 in acetonitrile (55:45, v/v) ratio 38: 62 (v/v), 10 µg/mL ethylparaben internal standard, UV detector 215 nm, 40°C column temperature, 1 mL/minute flow rate, and 20 µL injection volume. The validation of both methods using test solutions containing m-cresol and glycerol. ELISA method in the range of 80.11-200.28 µg/mL (r = 0.99) and HPLC at 9.735-146.025 µg/ml (r = 0.9997) was resulted to be linear. The recovery yields on ELISA and HPLC were 99.11%±5.01 and 100.71%±1.11. RSD on ELISA and HPLC were 3.91%, and 0.64%, respectively. The LOD and LOQ of the ELISA were 22.05 µg/mL and 73.51 µg/mL, while HPLC were 0.193 µg/ml and 0.643 µg/ml. Human insulin is stable at 2-8°C for 24 hours (ELISA) and 23°C for 48 hours (HPLC). In conclusion, the validation results of both methods are valid and able to determine human insulin with no significant difference (T test, a0.05). Cannot connect to Ginger Check your internet connection or reload the browser Disable in this text field Rephrase Rephrase current sentence Edit in Ginger Enable Ginger Cannot connect to Ginger Check your internet connection or reload the browser Disable in this text field Rephrase Rephrase current sentence Edit in Ginger.

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Jenis Koleksi : UI - Tesis Membership
No. Panggil : T-pdf
Entri utama-Nama orang :
Entri tambahan-Nama orang :
Entri tambahan-Nama badan :
Program Studi :
Subjek :
Penerbitan : Depok: Fakultas Farmasi Universitas Indonesia, 2022
Bahasa : ind
Sumber Pengatalogan : LibUI ind rda
Tipe Konten : text
Tipe Media : computer
Tipe Carrier : online resource
Deskripsi Fisik : xvi, 114 pages : illustration + appendix
Naskah Ringkas :
Lembaga Pemilik : Universitas Indonesia
Lokasi : Perpustakaan UI
  • Ketersediaan
  • Ulasan
  • Sampul
No. Panggil No. Barkod Ketersediaan
T-pdf 15-23-51990910 TERSEDIA
Ulasan:
Tidak ada ulasan pada koleksi ini: 9999920518379
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