Borner K, Lode H, Elvers A
Antimicrob Agents Chemother. 1982 Dec;22(6):949-53. doi: 10.1128/AAC.22.6.949.
We describe two methods for the quantitative analysis of apalcillin and its metabolites in serum and urine by reverse-phase high-pressure liquid chromatography (HPLC), a fast isocratic method for the parent drug, and a gradient method that allows the simultaneous assay of two metabolites. Serum was deproteinized with acetonitrile, and urine was diluted with buffer solution. The detection limit was about 0.5 micrograms/ml at a detection wavelength of 254 nm and 1.5 micrograms/ml at 310 nm. Within-batch precision (coefficient of variation) varied from 10.2 to 1.1% for concentrations of 7.8 and 185.3 micrograms/ml of serum, respectively. Recovery rates of 95.1 and 97.7% were found in spiked sera. Results obtained by HPLC correlated well with those from a standard microbiological assay (agar diffusion test); the resulting bivariate regression equation for serum was y-bioassay = 2.5 micrograms/ml + 0.992 X xHPLC, and that for urine was ybioassay = 12.0 micrograms/ml + 1.009 X xHPLC. At a detection wavelength of 315 nm, no interferences were observed in 10 healthy volunteers. Healthy subjects who were given 2 g of apalcillin intravenously excreted 18% of the parent drug within 24 h in the urine. Two inactive compounds were furthermore identified in urine as the isomeric forms of the penicilloic acids. Their excretion within 24 h amounted to 6.9 and 11.2% of the dose.
我们描述了两种通过反相高效液相色谱法(HPLC)对血清和尿液中的阿帕西林及其代谢物进行定量分析的方法,一种是针对母体药物的快速等度洗脱方法,另一种是可同时测定两种代谢物的梯度洗脱方法。血清用乙腈进行脱蛋白处理,尿液用缓冲溶液稀释。在检测波长为254nm时,检测限约为0.5微克/毫升,在310nm时为1.5微克/毫升。对于血清浓度为7.8和185.3微克/毫升的情况,批内精密度(变异系数)分别在10.2%至1.1%之间变化。加标血清中的回收率分别为95.1%和97.7%。通过HPLC获得的结果与标准微生物测定法(琼脂扩散试验)的结果相关性良好;血清的双变量回归方程为y - 生物测定法 = 2.5微克/毫升 + 0.992×xHPLC,尿液的双变量回归方程为y - 生物测定法 = 12.0微克/毫升 + 1.009×xHPLC。在检测波长为315nm时,10名健康志愿者未观察到干扰。静脉注射2g阿帕西林的健康受试者在24小时内尿液中排出了18%的母体药物。此外,在尿液中鉴定出两种无活性化合物为青霉酸的异构体形式。它们在24小时内的排泄量分别占给药剂量的6.9%和11.2%。
