Nuclear Medicine Department, Cannizzaro Hospital, Via Messina 829, 95126 Catania, Italy.
FORA S.p.A., Via Alfred Bernhard Nobel 11/a, 43122 Parma, Italy.
Bioconjug Chem. 2024 Mar 20;35(3):324-332. doi: 10.1021/acs.bioconjchem.3c00519. Epub 2024 Feb 17.
Immunoconjugates exploit the high affinity of monoclonal antibodies for a recognized antigen to selectively deliver a cytotoxic payload, such as drugs or radioactive nuclides, at the site of disease. Despite numerous techniques have been recently developed for site-selective bioconjugations of protein structures, reaction of ε-amine group of lysine residues with electrophilic reactants, such as activated esters (NHS), is the main method reported in the literature as it maintains proteins in their native conformation. Since antibodies hold a high number of lysine residues, a heterogeneous mixture of conjugates will be generated, which can result in decreased target affinity. Here, we report an intradomain regioselective bioconjugation between the monoclonal antibody Trastuzumab and the -hydroxysuccinimide ester of the chelator 2,2',2″,2‴-(1,4,7,10-tetraazacyclododecane-1,4,7,10-tetrayl)tetraacetic acid (DOTA) by a kinetically controlled reaction adding substoichiometric quantities of the activated ester to the mAb working at slightly basic pH. Liquid chromatography-mass spectrometry (LC-MS) analyses were carried out to assess the chelator-antibody ratio (CAR) and the number of chelating moieties linked to the mAb chains. Proteolysis experiments showed four lysine residues mainly involved in bioconjugation (K188 for the light chain and K30, K293, and K417 for the heavy chain), each of which was located in a different domain. Since the displayed intradomain regioselectivity, a domain mapping MS-workflow, based on a selective domain denaturation, was developed to quantify the percentage of chelator linked to each mAb domain. The resulting immunoconjugate mixture showed an average CAR of 0.9. About a third of the heavy chains were found as monoconjugated, whereas conjugation of the chelator in the light chain was negligible. Domain mapping showed the CH3 domain bearing 13% of conjugated DOTA, followed by CH2 and VH respectively bearing 12.5 and 11% of bonded chelator. Bioconjugation was not found in the CH1 domain, whereas for the light chain, only the CL domain was conjugated (6%). Data analysis based on LC-MS quantification of different analytical levels (intact, reduced chains, and domains) provided the immunoconjugate formulation. A mixture of immunoconjugates restricted to 15 species was obtained, and the percentage of each one within the mixture was calculated. In particular, species bearing 1 DOTA with a relative abundance ranging from 4 to 20-fold, in comparison to species bearing 2DOTA, were observed. Pairing of bioconjugation under kinetic control with the developed domain mapping MS-workflow could raise the standard of chemical quality for immunoconjugates obtained with commercially available reactants.
免疫偶联物利用单克隆抗体对识别抗原的高亲和力,选择性地将细胞毒性有效载荷(如药物或放射性核素)递送到疾病部位。尽管最近已经开发了许多用于蛋白质结构的位点选择性生物偶联的技术,但赖氨酸残基的 ε-胺与亲电试剂(如活化酯(NHS))的反应是文献中报道的主要方法,因为它使蛋白质保持其天然构象。由于抗体含有大量的赖氨酸残基,因此会产生异质的缀合物混合物,这可能导致靶标亲和力降低。在这里,我们报告了单克隆抗体曲妥珠单抗与螯合剂 2,2',2″,2‴-(1,4,7,10-四氮杂环十二烷-1,4,7,10-四乙酸)四乙酸(DOTA)的 - 羟基琥珀酰亚胺酯之间的域内区域选择性生物偶联,通过动力学控制反应将亚化学计量的活化酯添加到在略碱性 pH 下工作的 mAb 中。进行液相色谱-质谱 (LC-MS) 分析以评估螯合剂-抗体比 (CAR) 和与 mAb 链连接的螯合部分的数量。蛋白水解实验表明,四个赖氨酸残基主要参与生物偶联(轻链的 K188 和重链的 K30、K293 和 K417),每个残基都位于不同的结构域中。由于显示出的域内区域选择性,开发了一种基于选择性域变性的域映射 MS 工作流程,以定量与每个 mAb 域连接的螯合剂的百分比。所得免疫偶联物混合物的平均 CAR 为 0.9。大约三分之一的重链被发现为单缀合,而轻链中的缀合则可以忽略不计。域映射显示 CH3 结构域带有 13%的结合 DOTA,其次是 CH2 和 VH,分别带有 12.5%和 11%的结合螯合剂。在 CH1 结构域中未发现生物偶联,而对于轻链,仅 CL 结构域被缀合(6%)。基于 LC-MS 对不同分析水平(完整、还原链和结构域)的定量分析提供了免疫偶联物配方。获得了限制在 15 种物质的免疫偶联物混合物,并且计算了混合物中每种物质的百分比。特别是,观察到带有 1 个 DOTA 的物质的相对丰度范围为 4 到 20 倍,与带有 2 个 DOTA 的物质相比。动力学控制下的生物偶联与开发的域映射 MS 工作流程的结合可以提高使用市售试剂获得的免疫偶联物的化学质量标准。
