Method for rapidly detecting beta receptor agonist in pork
A β-receptor and agonist technology, applied in the field of analysis and detection, can solve the problems of cumbersome process, large loss of repeated extraction, unsuitable for the detection of large batches of samples, etc., and achieve the effect of simple operation and shortened enzymatic hydrolysis time
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Embodiment 1
[0022] 1) Weigh 2g of pork sample, add 8g of 0.2mol / L ammonium acetate buffer solution with a pH value of 5.0 to the pork sample, homogenize at 5000r / min for 1min, add 5000U of β-glucose hydrochloride to the homogenized pork sample Aldosidase and arylsulfatase, 35°C, enzymatic hydrolysis for 3 hours, add 20g of a mixture of isopropanol and ethyl acetate with a volume ratio of 7:5, vortex for 10 minutes, and centrifuge at 8000rpm for 5 minutes to obtain the supernatant, which is set aside ;
[0023] 2) Equilibrate the MCX solid-phase extraction column with 10ml of methanol, 10ml of deionized water, and 10ml of 0.1mol / L hydrochloric acid solution in sequence. After pretreatment of the MCX solid-phase extraction column, load the supernatant from step 1) onto the MCX The solid-phase extraction column was rinsed with deionized water and vacuum-drained the MCX solid-phase extraction column, and the MCX solid-phase extraction column was eluted with a mixture of ammonia and methanol a...
Embodiment 2
[0027] 1) Weigh 2g of pork sample, add 8g of 0.2mol / L ammonium acetate buffer solution with a pH value of 5.0 to the pork sample, homogenize at 5000r / min for 1min, add 5500U of β-glucose hydrochloride to the homogenized pork sample Alsidase and arylsulfatase, 37°C, enzymatic hydrolysis for 4 hours, add 20g of a mixture of isopropanol and ethyl acetate with a volume ratio of 7:5, vortex for 13 minutes, and centrifuge at 8000rpm for 7 minutes to obtain the supernatant, which is set aside ;
[0028] 2) Equilibrate the MCX solid-phase extraction column with 10ml of methanol, 10ml of deionized water, and 10ml of 0.1mol / L hydrochloric acid solution in sequence. After pretreatment of the MCX solid-phase extraction column, load the supernatant from step 1) onto the MCX The solid-phase extraction column was rinsed with deionized water and vacuum-drained the MCX solid-phase extraction column, and the MCX solid-phase extraction column was eluted with a mixture of ammonia and methanol at ...
Embodiment 3
[0032] 1) Weigh 2g of pork sample, add 8g of 0.2mol / L ammonium acetate buffer solution with a pH value of 5.0 to the pork sample, homogenize at 5000r / min for 1min, add 6000U of β-glucose hydrochloride to the homogenized pork sample Aldosidase and arylsulfatase, 39°C, enzymatic hydrolysis for 5h, add 20g of a mixture of isopropanol and ethyl acetate with a volume ratio of 7:5, vortex for 15min, and centrifuge at 8000rpm for 10min to obtain the supernatant, which is set aside ;
[0033] 2) Equilibrate the MCX solid-phase extraction column with 10ml of methanol, 10ml of deionized water, and 10ml of 0.1mol / L hydrochloric acid solution in sequence. After pretreatment of the MCX solid-phase extraction column, load the supernatant from step 1) onto the MCX The solid-phase extraction column was rinsed with deionized water and vacuum-drained the MCX solid-phase extraction column, and the MCX solid-phase extraction column was eluted with a mixture of ammonia and methanol at a volume rat...
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