首页> 外文期刊>Journal of Analytical Methods in Chemistry >Implementation and Validation of an Analytical Method for Lincomycin Determination in Feathers and Edible Tissues of Broiler Chickens by Liquid Chromatography Tandem Mass Spectrometry
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Implementation and Validation of an Analytical Method for Lincomycin Determination in Feathers and Edible Tissues of Broiler Chickens by Liquid Chromatography Tandem Mass Spectrometry

机译:通过液相色谱法串联质谱法实施和验证肉鸡羽毛的分析方法和肉鸡鸡的可食用组织

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Recent studies have detected different antimicrobial residues in broiler chicken feathers, where they persisted for longer periods of time and at greater concentrations than in edible tissues. However, until today, lincomycin behaviour in this nonedible tissue has not been assessed yet. Considering this, an analytical methodology to detect and quantify this antibiotic concentration in feathers, muscle, and liver tissues from broiler chickens was implemented and in-house validated. The methodology will allow the determination of the bioaccumulation of this highly persistent antibiotic in feathers of treated birds. For this purpose, 98% lincomycin and 95% lincomycin D3 standards were used. Methanol was selected as the extraction solvent, and Chromabond? Florisil? cartridges were used for the clean-up stage. The separation of analytes was performed through the analytical column SunFire C18 with a running time of 4?minutes, and the instrumental analysis was performed through an LC-MS/MS, with a liquid chromatograph Agilent? 1290 Infinity, coupled to an AB SCIEX? API 5500 mass spectrometer. An internal protocol for an in-house validation was designed based on recommendations from Commission Decision 2002/657/EC and the Guidance document on the estimation of limit of detection and limit of quantification for measurements in the field of contaminants in feed and food. The average retention time for lincomycin was 2.255?min (for quantifier ion, 126.0). The calibration curves showed a coefficient of determination (r2) greater than 0.99 for all matrices, while recovery levels ranged between 98% and 101%. The limit of detection (LOD) calculated was of 19, 22, and 10?μg·kg?1, and the limit of quantification (LOQ) was of 62, 73, and 34?μg·kg?1 in feathers, muscle, and liver, respectively. This method detects lincomycin in the studied matrices, confidently and accurately, as it is required for designing analytical studies of drug residues in edible and nonedible tissues, such as feathers.
机译:最近的研究发现了肉鸡鸡羽中不同的抗微生物残留物,在那里它们持续时间更长的时间和比食用组织更大的浓度。然而,直到今天,尚未评估该非可用组织中的林霉素行为。考虑到这一点,实施了从肉鸡,肌肉和肉鸡中的抗生素组织中检测和量化这种抗生素浓度的分析方法,并在内部验证。该方法将允许在经处理的鸟类的羽毛中测定这种高度持久的抗生素的生物累积。为此目的,使用98%的Lincomcin和95%的Lincomcycin D3标准。选择甲醇作为萃取溶剂,和Compabond? Florisil?墨盒用于清理阶段。通过分析塔SunFire C18进行分析物的分离,运行时间为4?分钟,通过LC-MS / MS进行仪器分析,液相色谱仪安静? 1290无限,耦合到AB SCIEX? API 5500质谱仪。根据委员会决定2002/657 / EC的建议和关于估算饲料和食品领域的污染物领域的测量限制的估算和定量限制的指导文件,设计了内部验证的内部协议。 LiNcomcin的平均保留时间为2.255?min(用于量子离子,126.0)。校准曲线显示所有矩阵大于0.99的测定系数(R2),而恢复水平范围为98%至101%。计算的检测极限(LOD)为19,22和10?μg·kg?1,并且量化限度(LOQ)为62,73和34?μg·kg?1在羽毛,肌肉,和肝脏分别。该方法可自信地和准确地检测所研究的矩阵中的林核霉素,因为它需要设计可食用和非可用组织中的药物残留物的分析研究,例如羽毛。

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