Amari J V, Mazsaroff I
Genetics Institute, Andover, MA 01810, USA.
J Chromatogr A. 1996 Apr 5;729(1-2):113-24. doi: 10.1016/0021-9673(95)01242-7.
A two-dimensional size-exclusion-reversed-phase high-performance liquid chromatographic assay has been developed for the quantitation of recombinant human interleukin-11 fusion protein (rhIL-11 FP) expressed in E. coli cells. The sample preparation procedure included the optimization of lysis buffer components to achieve maximum rhIL-11 FP recovery through the disruption of associations between rhIL-11 FP and E. coli components. The E. coli cells were dialyzed into lysis buffer and lysed by a French Press prior to two-dimensional chromatographic analysis. A size-exclusion column was used first to remove high- and low-molecular-mass E. coli components. Then reversed-phase chromatography was used to separate and quantify the rhIL-11 FP. The assay was linear over the range of 0.0294 to 0.235 mg/ml. The limit of quantitation, 0.0294 mg/ml, was based on % normalized residuals and precision criteria not exceeding 10%. The reproducibility of the assay for lysate samples was good on a daily (% R.S.D. = 1.0; n = 5) and a day-to-day reproducibility was good (% R.S.D. = 2.2; n = 9). Selectivity and chromatographic peak identification were based upon gel electrophoresis and N-terminal sequencing of the rhIL-11 FP peak collected from the reversed-phase column.
已开发出一种二维尺寸排阻反相高效液相色谱法,用于定量在大肠杆菌细胞中表达的重组人白细胞介素-11融合蛋白(rhIL-11 FP)。样品制备程序包括优化裂解缓冲液成分,以通过破坏rhIL-11 FP与大肠杆菌成分之间的结合来实现rhIL-11 FP的最大回收率。在进行二维色谱分析之前,将大肠杆菌细胞透析到裂解缓冲液中,并用法国压榨机裂解。首先使用尺寸排阻柱去除高分子量和低分子量的大肠杆菌成分。然后使用反相色谱法分离和定量rhIL-11 FP。该测定法在0.0294至0.235 mg/ml范围内呈线性。定量限为0.0294 mg/ml,基于归一化残差百分比和不超过10%的精密度标准。裂解物样品测定法的日内重现性良好(%R.S.D.=1.0;n=5),日间重现性也良好(%R.S.D.=2.2;n=9)。选择性和色谱峰鉴定基于从反相柱收集的rhIL-11 FP峰的凝胶电泳和N端测序。
