色谱
色譜
색보
CHINESE JOURNAL OF CHROMATOGRAPHY
2015年
8期
838-842
,共5页
张学亮%罗云敬%姜洁%路勇%冯楠
張學亮%囉雲敬%薑潔%路勇%馮楠
장학량%라운경%강길%로용%풍남
超高效液相色谱-串联质谱%分子印迹固相萃取%β2-受体激动剂%残留%猪肉
超高效液相色譜-串聯質譜%分子印跡固相萃取%β2-受體激動劑%殘留%豬肉
초고효액상색보-천련질보%분자인적고상췌취%β2-수체격동제%잔류%저육
ultra-high performance liquid chromatography-tandem mass spectrometry( UPLC-MS/MS)%molecularly imprinted solid phase extraction%β2-gonists%residues%pork
建立了一种分子印迹固相萃取-超高效液相色谱-串联质谱同时测定猪肉中5种β2-受体激动剂残留的方法。样品经过均质处理后置于乙酸铵/乙酸缓冲液中,加入内标物和β-葡萄糖醛酸酶/芳基硫酸酯酶,于55℃酶解2 h,调节溶液 pH后通过分子印迹固相萃取柱净化,然后采用 BEH C18色谱柱分离,以甲醇-0.1%( v/v)甲酸水溶液为流动相,采用梯度洗脱,在电喷雾正离子多反应监测模式下用内标法定量。检出限( LOD,S/N=3)和定量限( LOQ,S/N=10)分别为0.005~0.009μg/kg和0.015~0.025μg/kg。在0~10μg/kg范围内线性关系良好,相关系数≥0.9933。添加水平为0.25、1、5μg/kg时,回收率为80.4%~92.9%,相对标准偏差为1.2%~6.3%。该方法具有灵敏度高、重复性好、回收率高等优点,适合同时进行多种β2-受体激动剂残留的测定。
建立瞭一種分子印跡固相萃取-超高效液相色譜-串聯質譜同時測定豬肉中5種β2-受體激動劑殘留的方法。樣品經過均質處理後置于乙痠銨/乙痠緩遲液中,加入內標物和β-葡萄糖醛痠酶/芳基硫痠酯酶,于55℃酶解2 h,調節溶液 pH後通過分子印跡固相萃取柱淨化,然後採用 BEH C18色譜柱分離,以甲醇-0.1%( v/v)甲痠水溶液為流動相,採用梯度洗脫,在電噴霧正離子多反應鑑測模式下用內標法定量。檢齣限( LOD,S/N=3)和定量限( LOQ,S/N=10)分彆為0.005~0.009μg/kg和0.015~0.025μg/kg。在0~10μg/kg範圍內線性關繫良好,相關繫數≥0.9933。添加水平為0.25、1、5μg/kg時,迴收率為80.4%~92.9%,相對標準偏差為1.2%~6.3%。該方法具有靈敏度高、重複性好、迴收率高等優點,適閤同時進行多種β2-受體激動劑殘留的測定。
건립료일충분자인적고상췌취-초고효액상색보-천련질보동시측정저육중5충β2-수체격동제잔류적방법。양품경과균질처리후치우을산안/을산완충액중,가입내표물화β-포도당철산매/방기류산지매,우55℃매해2 h,조절용액 pH후통과분자인적고상췌취주정화,연후채용 BEH C18색보주분리,이갑순-0.1%( v/v)갑산수용액위류동상,채용제도세탈,재전분무정리자다반응감측모식하용내표법정량。검출한( LOD,S/N=3)화정량한( LOQ,S/N=10)분별위0.005~0.009μg/kg화0.015~0.025μg/kg。재0~10μg/kg범위내선성관계량호,상관계수≥0.9933。첨가수평위0.25、1、5μg/kg시,회수솔위80.4%~92.9%,상대표준편차위1.2%~6.3%。해방법구유령민도고、중복성호、회수솔고등우점,괄합동시진행다충β2-수체격동제잔류적측정。
An ultra-high performance liquid chromatography-tandem mass spectrometry ( UPLC-MS/MS)method with molecularly imprinted solid phase extraction for the determina-tion of five β2-gonists residues in pork has been developed. After the sample preparation,the ammonium acetate/acetic acid buffer was added,followed by the internal standard and β-glu-curonidase/arylsulfatase enzyme. The solution was incubated at 55 ℃ for 2 h. After adjusting the pH of the solution,it was purified by a molecularly imprinted solid phase extraction col-umn,then analyzed on a BEH C18 column with methanol-0. 1%( v/v ) formic acid aqueous solution as the mobile phases in gradient elution mode. The MS/MS analysis was in positive ion mode and multiple reaction monitoring mode. The analytes were quantified by the internal standard method. The limits of detection( LODs,S/N = 3 ) and the limits of quantification ( LOQs,S/N=10)were 0. 005-0. 009 μg/kg and 0. 015-0. 025 μg/kg,respectively. In the range of 0-10 μg/kg,the correlation coefficients of linear calibration curves were not less than 0. 993 3. At the spiked levels of 0. 25,1. 0 and 5. 0 μg/kg,the recoveries were 80. 4%-92. 9%with the relative standard deviations of 1. 3%-6. 3%. The method is of high sensitivity,good reproducibility,high recovery,and is useful for the simultaneous determination of multiple β2-agonists residues.
