改善4Dm2m的CH1-CK异源二聚化及药代动力学,4Dm2m是一种新型强效抗HIV-1的CD4抗体融合蛋白。
Improving the CH1-CK heterodimerization and pharmacokinetics of 4Dm2m, a novel potent CD4-antibody fusion protein against HIV-1.
作者信息
Chen Weizao, Bardhi Ariola, Feng Yang, Wang Yanping, Qi Qianqian, Li Wei, Zhu Zhongyu, Dyba Marzena A, Ying Tianlei, Jiang Shibo, Goldstein Harris, Dimitrov Dimiter S
机构信息
a Protein Interactions Section, Cancer and Inflammation Program, Center for Cancer Research, National Cancer Institute, National Institutes of Health , Frederick , Maryland , USA.
b Departments of Microbiology and Immunology and Pediatrics , Albert Einstein College of Medicine , Bronx , New York , USA.
出版信息
MAbs. 2016 May-Jun;8(4):761-74. doi: 10.1080/19420862.2016.1160180. Epub 2016 Mar 10.
We previously described 4Dm2m, an exceptionally potent broadly neutralizing CD4-antibody fusion protein against HIV-1. It was generated by fusing the engineered single human CD4 domain mD1.22 to both the N and C termini of the human IgG1 heavy chain constant region and the engineered single human antibody domain m36.4, which targets the CD4-induced coreceptor binding site of the viral envelope glycoprotein, to the N terminus of the human antibody kappa light chain constant region via the (G4S)3 polypeptide linkers. However, therapeutic use of 4Dm2m was limited by its short in vivo half-life. Here, we show that a combination of three approaches have successfully increased the persistence of 4Dm2m in mice. First, to stabilize the scaffold, we enhanced heterodimerization between the heavy chain constant domain 1 (CH1) and kappa light chain constant domain (CK) by using structure-guided design and phage-display library technologies. Second, to address the possibility that long polypeptide linkers might render fusion proteins more susceptible to proteolysis, we shortened the (G4S)3 linkers or replaced them with the human IgG1 hinge sequence, which is naturally designed for both flexibility and stability. Third, we introduced two amino acid mutations into the crystallizable fragment (Fc) of the scaffold previously shown to increase antibody binding to the neonatal Fc receptor (FcRn) and prolong half-lives in vivo. Collectively, these approaches markedly increased the serum concentrations of 4Dm2m in mice while not affecting other properties of the fusion protein. The new 4Dm2m variants are promising candidates for clinical development to prevent or treat HIV-1 infection. To our knowledge, this is the first report on stabilized CH1-CK, which is potentially useful as a new heterodimerization scaffold for generation of bispecific and multispecific antibodies or proteins with a more favorable pharmacokinetic profile.
我们之前描述了4Dm2m,一种针对HIV-1的异常强效的广谱中和CD4抗体融合蛋白。它是通过将工程化的单个人CD4结构域mD1.22融合到人IgG1重链恒定区的N端和C端,以及将靶向病毒包膜糖蛋白CD4诱导的共受体结合位点的工程化单个人抗体结构域m36.4,通过(G4S)3多肽接头融合到人抗体κ轻链恒定区的N端而产生的。然而,4Dm2m的治疗用途受到其体内半衰期短的限制。在这里,我们表明三种方法的组合成功地增加了4Dm2m在小鼠体内的持久性。首先,为了稳定支架,我们通过使用结构导向设计和噬菌体展示文库技术增强了重链恒定结构域1(CH1)和κ轻链恒定结构域(CK)之间的异二聚化。其次,为了解决长多肽接头可能使融合蛋白更容易被蛋白酶水解的可能性,我们缩短了(G4S)3接头或用天然设计用于灵活性和稳定性的人IgG1铰链序列替换它们。第三,我们在支架的可结晶片段(Fc)中引入了两个氨基酸突变,之前已证明该突变可增加抗体与新生儿Fc受体(FcRn)的结合并延长体内半衰期。总的来说,这些方法显著提高了小鼠体内4Dm2m的血清浓度,同时不影响融合蛋白的其他特性。新的4Dm2m变体是预防或治疗HIV-1感染临床开发的有前途的候选药物。据我们所知,这是关于稳定化CH1-CK的首次报道,它可能作为一种新的异二聚化支架,用于生成具有更有利药代动力学特征的双特异性和多特异性抗体或蛋白质。
Zotero 插件