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Abstrak :
Terdapat banyak metode untuk mendeteksi kontaminasi melamin dalam makanan atau produk pakan termasuk immunoassay. Dalam penelitian ini, hapten melamin disintesis dengan mereaksikan 2-kloro-4,6-diamino-1,3,5-triazina (CAAT) dengan asam 6-aminokaproat. Karakterisasi hapten dengan spektrometer Fourier Transform Infrared (FTIR) menunjukkan absorpsi ikatan N-H dari gugus amina sekunder alifatik pada frekuensi 3350-3310 cm-1 dan vibrasi ulur ikatan C-N pada daerah sidik jari 1250-1020 cm-1. Karakterisasi dengan 1H-NMR menunjukkan pergeseran kimia pada 4,20 ppm (t, 1H), sedangkan dengan 13C-NMR pada pergeseran kimia 139 ppm. Karakterisasi dengan spektrometer massa menunjukkan M+. m/z 240,4 untuk hapten (C9H16N6O2). Imunogen disintesis dengan cara menkonjugasikan hapten dengan bovine serum albumin (BSA) dengan menggunakan metode ester aktif. Konjugat hapten-BSA menyerap panjang gelombang maksimum UV pada 224 nm. Data menunjukkan bahwa hapten dan imunogen berhasil disintesis. Hapten-BSA kemudian disuntikkan ke kelinci untuk menghasilkan antibodi poliklonal. Setelah tiga minggu imunisasi, serum menunjukkan adanya antibodi melalui Gel Agarose Precipitation Test (AGPT). Dari hasil optimasi awal indirect ELISA diketahui konsentrasi optimum coating antigen hapten-OVA adalah 1 μg/mL dan konjugat HRP-anti rabbit IgG adalah 1:10.000. Dari hasil indirect competitive ELISA diperoleh bahwa pengenceran optimum antibodi yang masih memberikan respon positif berupa absorbansi yang tinggi adalah 1:125 (6 μg/mL). Antiserum yang dihasilkan memiliki sensitivitas yang cukup baik terhadap melamin dengan nilai IC50 sebesar 2,83 ppm dan limit deteksi (IC15) sebesar 0,22 ppm melalui indirect competitive ELISA.

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There are many method to detect the melamine contamination in food or feed product including immunoassay. In this study, hapten of melamine was synthesized by reacting 2-chloro-4,6-diamino-1,3,5-triazine (CAAT) and 6-aminocaproic acid. Characterization of hapten with fourier transform infrared spectroscopy (FTIR) showed secondary N-H stretching vibrational band at 3350-3310 cm-1 and C-N stretching vibrational band at fingerprint region 1250-1020 cm-1. Characterization of hapten with 1H-NMR showed chemical shift at 4,20 ppm (t, 1H), and 139 ppm by 13C-NMR. Hapten also characterized with high-resolution mass spectrometry (HRMS) that showed M+. m/z 240,4 for hapten (C9H16N6O2). The Immunogen was prepared by coupling hapten to bovine serum albumin (BSA) using the active ester method. Hapten-BSA conjugate showed the maximum wavelength of UV absorpstion at 224 nm. The data pointed out that hapten and immunogen was successfully synthesized. Hapten-BSA conjugate then injected into rabbit to produce the polyclonal antibodies. After three weeks immunization, serum showed the presence of antibodies through Agar Gel Precipitation Test (AGPT). The initial optimization of indirect ELISA showed that the optimum concentration of coating antigen hapten-OVA was 1 mg/mL and HRP-conjugated anti-rabbit IgG was 1:10,000. The optimum antibody dilution that still gave a positive response was 1:125 (6 mg/mL) through indirect competitive ELISA. Antiserum produced has a good sensitivity to melamine with IC50 2.83 ppm and a detection limit (IC15) 0.22 ppm using indirect competitive ELISA.

Abstrak :
[ABSTRAK
Antibodi poliklonal anti aflatoksin B1 telah berhasil diproduksi pada hewan uji kelinci betina New Zealand White setelah diimunisasikan hapten aflatoksin B1-CMO yang dikonjugasikan dengan Bovine Serum Albumin (BSA) sebagai antigen. Hapten aflatoksin B1-CMO disintesis menggunakan metode karbodiimida dengan substrat aflatoksin B1 dan carboxymethyl hydroxylamine hemihydrochloride (CMO) sebagai linkernya. Hasil karakterisasi kromatografi lapis tipis dengan nilai Rf rata-rata sebesar 0.395, spektrum UV-Visibel dengan puncak λ maks pada 362, 264, 218 nm, spektrum IR dengan puncak 3448.126 cm-1 (3000-3600 cm-1) : OH, pada 1632.249 cm-1(1540-1725 cm-1) : C=O, dan 1642.451 cm-1 (1640-1690 cm-1) :C=N (Oksim), dan hasil fragmentasi spektrometri massa (MS/MS) pada m/z 386, 368.2, 310 membuktikan hapten aflatoksin B1-CMO berhasil disintesis. Hapten ini kemudian dikonjugasikan dengan BSA membentuk antigen aflatoksin B1-BSA (AFB1-BSA) sebelum diimunisasikan ke kelinci. Spesifitas antigen AFB1-BSA terhadap antibodinya dan uji konjugasi hapten ke BSA menunjukkan hasil positif menggunakan uji Dot Blot Immunoassay dengan konsentrasi BSA di dalam antigennya sebesar 1.74 mg/mL. Serum darah kelinci berdasarkan uji Agar Gel Precipitation Test (AGPT) positif mengandung antibodi poliklonal anti aflatoksin B1 setelah dua pekan (hari ke-11) sejak imunisasi primer antigen AFB1-BSA dilakukan. Dari serum darah bleeding panen, diperoleh konsentrasi antibodinya sebesar sebesar 2.19 mg/mL. Immunokromatogafi strip tes berhasil dibuat dengan nanopartikel iridium oksida (IrO2 NPs) sebagai kandidat label antibodinya dan dapat digunakan untuk mendeteksi sampel H IgG pada rentang 0.1 μg/mL sampai 10 μg/mL. Studi pendahuluan ini menunjukkan bahwa perangkat strip tes ini dapat digunakan untuk aplikasi konjugat sensor antibodi anti aflatoksin B1-nanopartikel iridium oksida untuk deteksi aflatoksin B1.

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ABSTRACT
Polyclonal antibody against aflatoxin B1 have been successfully produced in New Zealand White Rabbit after immunized by hapten of aflatoxin B1-CMO conjugated with Bovine Serum Albumin (BSA) as antigen. Hapten of aflatoxin B1-CMO was synthesized using carbodiimide method with afltoksin B1 as substrate and carboxymethyl hydroxylamine hemihydrochloride (CMO) as its linker. The characterization results of thin layer chromatography with Rf value of 0.395, the spectrum of UV-Visible with λ max peaks at 362, 264, 218 nm, the IR spectrum with peak at 3448.126 cm-1 (3000-3600 cm-1): OH , 1632.249 cm-1(1540-1725 cm-1): C = O, 1642.451 cm-1 (1640-1690 cm-1): C = N (oxime), and the results of mass spectrometry fragmentation (MS / MS) at m/ z of 386, 368.2, 310 proved that hapten of aflatoxin B1 -CMO successfully synthesized. Then, the hapten was conjugated to BSA to form antigen of aflatoxin B1-BSA (AFB1-BSA) before immunized to rabbits. The specificity of antigen of AFB1-BSA to its antibody and the confirmation of hapten-BSA conjugated showed positive results using dot blot immunoassay with BSA concentration in the antigen of 1.74 mg/mL. Based on Agar Gel Precipitation Test (AGPT) shown the rabbit blood serum resulted positive for polyclonal antibody against aflatoxin B1 after two weeks (day 11st) since the primary immunization of its antigen. From blood serum bleeding at harvest obtained the concentration of antibodies was 2.19 mg / mL. An Immunochromatogaphic test strip was successfully fabricated using iridium oxide nanoparticles (IrO2 NPs) as a labeled antibody candidate and can be used to detect the IgG H sample between of 0.1 μg/mL to 10 μg/mL. This preliminary study shown that the device can be used for applications of antibody against aflatoxin B1-nanoparticle iridium oxide conjugate for detection of aflatoxin B1 , Polyclonal antibody against aflatoxin B1 have been successfully produced in New Zealand White Rabbit after immunized by hapten of aflatoxin B1-CMO conjugated with Bovine Serum Albumin (BSA) as antigen. Hapten of aflatoxin B1-CMO was synthesized using carbodiimide method with afltoksin B1 as substrate and carboxymethyl hydroxylamine hemihydrochloride (CMO) as its linker. The characterization results of thin layer chromatography with Rf value of 0.395, the spectrum of UV-Visible with λ max peaks at 362, 264, 218 nm, the IR spectrum with peak at 3448.126 cm-1 (3000-3600 cm-1): OH , 1632.249 cm-1(1540-1725 cm-1): C = O, 1642.451 cm-1 (1640-1690 cm-1): C = N (oxime), and the results of mass spectrometry fragmentation (MS / MS) at m/ z of 386, 368.2, 310 proved that hapten of aflatoxin B1 -CMO successfully synthesized. Then, the hapten was conjugated to BSA to form antigen of aflatoxin B1-BSA (AFB1-BSA) before immunized to rabbits. The specificity of antigen of AFB1-BSA to its antibody and the confirmation of hapten-BSA conjugated showed positive results using dot blot immunoassay with BSA concentration in the antigen of 1.74 mg/mL. Based on Agar Gel Precipitation Test (AGPT) shown the rabbit blood serum resulted positive for polyclonal antibody against aflatoxin B1 after two weeks (day 11st) since the primary immunization of its antigen. From blood serum bleeding at harvest obtained the concentration of antibodies was 2.19 mg / mL. An Immunochromatogaphic test strip was successfully fabricated using iridium oxide nanoparticles (IrO2 NPs) as a labeled antibody candidate and can be used to detect the IgG H sample between of 0.1 μg/mL to 10 μg/mL. This preliminary study shown that the device can be used for applications of antibody against aflatoxin B1-nanoparticle iridium oxide conjugate for detection of aflatoxin B1 ]