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用于预防重组单克隆抗体HER2中甲硫氨酸氧化的抗氧化剂

Antioxidants for prevention of methionine oxidation in recombinant monoclonal antibody HER2.

作者信息

Lam X M, Yang J Y, Cleland J L

机构信息

Department of Pharmaceutical Research and Development, Genentech, Inc., San Francisco, CA 94080, USA.

出版信息

J Pharm Sci. 1997 Nov;86(11):1250-5. doi: 10.1021/js970143s.

Abstract

Recombinant humanized monoclonal antibody HER2, rhuMAb HER2, in liquid formulations undergoes oxidation when exposed to intense light and elevated temperatures (30 & 40 degrees C). Met-255 in the heavy chain of the Fc region of the antibody is the primary site of oxidation. Met-431 of the Fc fragment can also be oxidized under extreme conditions. The amount of oxidation was determined by cleaving the Fab and Fc fragments by papain digestion, and the oxidized Fc fragment was detected by hydrophobic interaction chromatography. Oxidation of rhuMAb HER2 was also formulation dependent. The presence of NaCl in the rhuMAb HER2 formulation caused an increase in oxidation at higher temperatures after contact with stainless steel containers or stainless steel components in the filling process. The corrosion of stainless steel by chloride ions at the low pH of the formulation buffer generated iron ions that catalyzed methionine oxidation in rhuMAb HER2. Temperature-induced oxidation of rhuMAb HER2 occurred by the formation of free radicals, and light-induced oxidation of rhuMAb HER2 occurred via single oxygen pathway. Antioxidants, such as methionine, sodium thiosulfate, catalase, or platinum, prevented Met oxidation in rhuMAb HER2, presumably as free radicals or oxygen scavengers. The minimum effective levels (molar ratios of protein to antioxidant) required to inhibit temperature-induced oxidation were 1:5 and 1:25 for methionine and thiosulfate, respectively. A thiosulfate adduct of rhuMAb HER2 was observed by cation-exchange chromatography. These studies demonstrate that stoichiometric amounts of methionine and thiosulfate are sufficient to eliminate temperature-induced oxidation of rhuMAb HER2 caused by free radicals that were generated by the presence of metal ion and peroxide impurities in the formulation.

摘要

重组人源化单克隆抗体HER2(rhuMAb HER2)的液体制剂在强光和高温(30℃和40℃)下会发生氧化。抗体Fc区域重链中的Met-255是氧化的主要位点。在极端条件下,Fc片段的Met-431也会被氧化。通过木瓜蛋白酶消化裂解Fab和Fc片段来测定氧化量,并通过疏水相互作用色谱法检测氧化的Fc片段。rhuMAb HER2的氧化也取决于制剂。rhuMAb HER2制剂中NaCl的存在会导致在灌装过程中与不锈钢容器或不锈钢部件接触后,在较高温度下氧化增加。制剂缓冲液低pH值下氯离子对不锈钢的腐蚀产生了铁离子,催化了rhuMAb HER2中的甲硫氨酸氧化。rhuMAb HER2的温度诱导氧化是通过自由基的形成发生的,而光诱导氧化是通过单线态氧途径发生的。抗氧化剂,如甲硫氨酸、硫代硫酸钠、过氧化氢酶或铂,可防止rhuMAb HER2中的Met氧化,推测是作为自由基或氧清除剂。抑制温度诱导氧化所需的最低有效水平(蛋白质与抗氧化剂的摩尔比),甲硫氨酸和硫代硫酸盐分别为1:5和1:25。通过阳离子交换色谱法观察到了rhuMAb HER2的硫代硫酸盐加合物。这些研究表明,化学计量的甲硫氨酸和硫代硫酸盐足以消除制剂中金属离子和过氧化物杂质产生的自由基引起的rhuMAb HER2的温度诱导氧化。

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