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机构地区:[1]昆明市食品药品检验所,昆明650032 [2]中国食品药品检定研究院,北京100050
出 处:《药物分析杂志》2014年第7期1251-1255,共5页Chinese Journal of Pharmaceutical Analysis
摘 要:目的:建立固相萃取高效液相色谱(SPE-HPLC)法测定马破伤风免疫球蛋白F(ab’)2中灭活剂Triton X-100的残留量。方法:采用Oasis固相萃取小柱对样品进行预处理,以水和5%甲醇为淋洗剂,以甲醇为洗脱剂,收集甲醇洗脱物用于HPLC分析。采用ZORBAX Extend-C18色谱柱(4.6 mm×150 mm,5μm),流动相为甲醇-水(80∶20),流速1.0 mL·min-1,检测波长230 nm,柱温30℃,进样量10μL。结果:Triton X-100浓度在0.56~55.34μg·mL-1范围内,与峰面积线性关系良好(r=0.9998);检测限(S/N=3)为2.03 ng,定量限(S/N=10)为4.06 ng;提取回收率为91.8%。结论:本方法操作简便、准确、重复性好,可用于Triton X-100的残留量测定。Objective: To establish a SPE- HPLC method for the determination of Triton X- 100 residues in equine antitetanus immunoglobulin F( ab')2. Methods: Samples were pre- treated on Oasis HLB SPE column,then cleaned- up by water and 5% methanol,and finally extracted by methanol. The analysis of extracts was performed on a ZORBAX Extend- C18column( 4. 6 mm × 150 mm,5 μm) with a mobile phase consisting of methanol- water( 80∶20,v/v) at a flow rate of 1.0 mL·min- 1. The column temperature was set at 30 ℃ and the injection volume was 10 μL. Triton X- 100 was detected at the wavelength of 230 nm with a DAD detection. Results: The established HPLC method resulted in sharp and symmetric peaks of Triton X- 100,whereas the calibration curve of Triton X- 100 displayed a good linearity within the concentration of 0. 56- 55. 34 μg·mL- 1( r =0. 9998). The LOD and LOQ were 2. 03 ng and 4. 06 ng,respectively. Specificity,precision,accuracy,stability and robustness were acceptable. The extraction recovery was 91. 8%. Conclusion: The results indicate that the established method is convenient,accurate and reproducible,which can be used in the analysis of Triton X- 100 residues in equine antitetanus immunoglobulin F( ab')2.
关 键 词:马破伤风免疫球蛋白F(ab’)2 TRITON X-100 灭活剂 裂解剂 辛基苯氧基聚2-乙氧基乙醇 杂质残留检测 固相萃取 高效液相色谱法
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