Aptamer AFB1-20 of aflatoxin B1 and application thereof
An aflatoxin and nucleic acid aptamer technology, applied in the field of nucleic acids, can solve the problems of limited application scope and rapid development of immunological detection methods, short reagent life, difficult preservation, and difficulty in antibody preparation. Modification marks, promising effects
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Embodiment 1
[0047] Example 1 Target AFB 1 Synthesis and characterization of -beads
[0048] Using agarose microbeads as the solid phase carrier of target molecules is beneficial to the separation of unbound or weakly bound and non-specific binding sequences, and is suitable for flow cytometry detection. will AFB 1 The synthetic route coupled to agarose microbeads is as follows:
[0049]
[0050] Take 7.6mg AFB 1 Dissolve in 4mL pyridine, add 35mg carboxymethylhydroxylamine hydrochloride, reflux at 80°C overnight, concentrate in vacuo and silica gel column chromatography (chloroform / methanol=10:1), isolate AFB 1 -oxime was dissolved in 3 mL of anhydrous dichloromethane, 5.4 mg of NHS, 9.6 mg of dicyclohexylcarbodiimide and 5 mg of dimethylaminopyridine were added, stirred overnight with a magnetic rotor, filtered and concentrated by evaporation to obtain AFB 1 -oxime activated ester (11.Chu, F.S.; Hsia, M.T.; Sun, P.S.: Preparation and characterization of aflatox-n B1-1-(O-carboxyme...
Embodiment 2
[0051] Embodiment 2 Aflatoxin B 1 Screening of specific aptamers
[0052](1) Design and synthesis of random oligonucleotide library
[0053] Design and synthesize a random oligonucleotide library with a fixed region of 18 nucleotides at both ends and a random region of 45 nucleotides in the middle as follows: 5'-ATA CCA GCT TAT TCA ATT-N45-AGA TAG TAA GTG CAA TCT -3', storage capacity in 10 15 . The primer sequences used were forward primer (FP): 5'-ATA CCA GCT TAT TCA ATT-3', reverse primer (RP): 5'-AGA TTG CAC TTA CTA TCT-3', fluorescent labeling primer (FFP ): 5'-FAM-ATA CCA GCT TAT TCA ATT-3', biotin-labeled primer (BRP): 5'-Bio-AGA TTG CAC TTA CTA TCT-3' (12.Shangguan, D.; Li, Y .;Tang,Z.;Cao,Z.C.;Chen,H.W.;Mallikaracchy,P.;Sefah,K.;Yang,C.J.;Tan,W.Aptamers evolved from live cells as effective molecular probes for cancer study.Proc Natl Acad Sci USA2006, 103, 11838-11843).
[0054] (2) Screening of nucleic acid aptamers
[0055] AFB 1 -beads are used as target mol...
Embodiment 3
[0057] Example 3 Fluorescence Polarization and Fluorescence Spectrum Research on Nucleic Acid Aptamer and Aflatoxin B 1 interaction between
[0058] Binding buffer (20mM Tris-HCl, pH8.0, 100mM NaCl, 5mM KCl, 2mM MgCl 2 , 1mM CaCl 2 ) Prepare a 2 μM unlabeled nucleic acid aptamer solution, conduct heat denaturation treatment, 95°C for 5 minutes, ice bath for 5 minutes, and place at room temperature for 30 minutes. Then add aflatoxin B to it 1 Make the final concentration 0.2μM, and incubate at room temperature for 30min. The blank group is aflatoxin B alone under the same conditions 1 Solution, the control group is random sequence Random. Determine the fluorescence anisotropy value of each group of solution systems (Ex: 365nm; Em: 442nm); scan the fluorescence spectrum of each group of solution systems (Ex: 365nm; Em: 380-650nm) (see Figure 5 and 6 ).
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