4.7 Article

In-tube solid phase microextraction and determination of ractopamine in pork muscle samples using amide group modified polysaccharide-silica hybrid monolith as sorbent prior to HPLC analysis

期刊

FOOD CHEMISTRY
卷 355, 期 -, 页码 -

出版社

ELSEVIER SCI LTD
DOI: 10.1016/j.foodchem.2021.129662

关键词

Agarose-silica hybrid monolith; In-tube solid-phase microextraction; Enrichment; Ractopamine; Pork samples

资金

  1. National Natural Science Foundation of China [41701358]
  2. Scientific Research and Develop Project of Henan Province [1223041346]
  3. Industry Academic Research Collaboration Program [152107000090]
  4. 111 Project [D17007]
  5. Henan Center for Outstanding Overseas Scientists [GZS2018003]
  6. Education Key Projects of Henan Provincial Department [19A150002]

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A facile in-tube solid phase microextraction procedure was developed to enrich ractopamine before HPLC-UV analysis, using an amide groups modified polysaccharide-silica hybrid monolith as an efficient sorbent. The method showed ideal selectivity for ractopamine, with enrichment factors ranging from 50.5 to 1.8 and recoveries from 85.2% to 108.1%.
A facile in-tube solid phase microextraction (in-tube SPME) procedure was developed to enrich ractopamine before HPLC-UV analysis. This was achieved by employing amide groups modified polysaccharide-silica hybrid monolith as an efficient sorbent. The monolith was synthesized by a simple reaction with agarose oxide and tetramethoxylisane, followed by the modification of amide groups via subsequent ring opening, ?thiol?ene? click and dehydration reactions. Under the optimized extraction conditions, the enrichment factors for ractopamine, dopamine, clenbuterol, para-methylphenol and phenol were determined to be 50.5, 32.2, 4.8, 2.1 and 1.8, respectively. The monolithic column has ideal selectivity for ractopamine. Coupled with HPLC-UV, this method demonstrated a linearity within 2.0?800 ng/g for ractopamine with spiking in pork muscles (R2 = 0.9958). The LOD was 0.64 ng/g (S/N = 3) and recoveries ranged from 85.2 to 108.1% (n = 3). This approach provides a feasible way for analysis of trace ractopamine in biological samples.

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