Xiong Cheng-Yi, Natarajan Arutselvan, Shi Xu-Bao, Denardo Gerald L, Denardo Sally J
Department of Internal Medicine, Division of Hematology/Oncology, Section of Radiodiagnosis and Therapy, University of California Davis Cancer Center 1508 Alhambra Boulevard, Sacramento, CA 95816, USA.
Protein Eng Des Sel. 2006 Aug;19(8):359-67. doi: 10.1093/protein/gzl020. Epub 2006 Jun 7.
MUC1 mucin expressed in epithelial cancer, such as prostate and breast, is aberrantly glycosylated providing unique targets for imaging and therapy. In order to create a broadly applicable construct to target these unique epitopes on metastatic cancer, we selected an antibody fragment (scFv) that binds both synthetic MUC1 core peptide and epithelial cancer cell-expressed MUC1, and developed a recombinant bivalent molecule (di-scFv). Genetically engineered modifications of the di-scFv were constructed to create five molecular versions, each having a free cysteine (di-scFv-c) at different locations for site-specific conjugation. The effects of the engineered cysteine in the varied sites were studied relative to tumor binding and polyethylene glycol-maleimide (PEG-Mal) conjugation (PEGylation). Escherichia coli production as well as binding to MUC1 core peptide, human tumor cell lines and human tumor biopsies, were comparable. However, the location of the engineered cysteine in these di-scFv-c did influence PEGylation efficiency of this free thiol; higher PEGylation efficiency occurred with this cysteine in the inter-scFv linkage. Di-scFv-c PEG, with the cysteine engineered after the fifth amino acid in the linker, was used as an example to demonstrate comparable antigen-binding to non-PEGylated di-scFv-c. In summary, novel anti-MUC1 di-scFv-c molecules can be efficiently produced, purified and conjugated by site-specific PEGylation without loss of immunoreactivity, thus providing flexible multidentate constructs for cancer-targeted imaging and therapy.
在上皮癌(如前列腺癌和乳腺癌)中表达的MUC1粘蛋白发生了异常糖基化,为成像和治疗提供了独特的靶点。为了构建一种广泛适用的构建体来靶向转移性癌症上的这些独特表位,我们选择了一种能同时结合合成MUC1核心肽和上皮癌细胞表达的MUC1的抗体片段(单链抗体片段),并开发了一种重组二价分子(双单链抗体片段)。对双单链抗体片段进行基因工程修饰,构建了五个分子版本,每个版本在不同位置都有一个游离半胱氨酸(双单链抗体片段-c),用于位点特异性偶联。研究了不同位点上工程化半胱氨酸相对于肿瘤结合和聚乙二醇-马来酰亚胺(PEG-Mal)偶联(聚乙二醇化)的影响。大肠杆菌生产以及与MUC1核心肽、人肿瘤细胞系和人肿瘤活检组织的结合情况相当。然而,这些双单链抗体片段-c中工程化半胱氨酸的位置确实影响了这种游离巯基的聚乙二醇化效率;在双单链抗体片段间连接区的这种半胱氨酸具有更高的聚乙二醇化效率。以连接子中第五个氨基酸后工程化半胱氨酸的双单链抗体片段-c聚乙二醇为例,证明其与非聚乙二醇化双单链抗体片段-c具有相当的抗原结合能力。总之,新型抗MUC1双单链抗体片段-c分子可以通过位点特异性聚乙二醇化高效生产、纯化和偶联,而不会丧失免疫反应性,从而为癌症靶向成像和治疗提供灵活的多齿构建体。