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RF1 衰减可实现高效的非天然氨基酸掺入,用于生产均一的抗体药物偶联物。

RF1 attenuation enables efficient non-natural amino acid incorporation for production of homogeneous antibody drug conjugates.

机构信息

Sutro Biopharma Inc, South San Francisco, CA, 94080, USA.

出版信息

Sci Rep. 2017 Jun 8;7(1):3026. doi: 10.1038/s41598-017-03192-z.

Abstract

Amber codon suppression for the insertion of non-natural amino acids (nnAAs) is limited by competition with release factor 1 (RF1). Here we describe the genome engineering of a RF1 mutant strain that enhances suppression efficiency during cell-free protein synthesis, without significantly impacting cell growth during biomass production. Specifically, an out membrane protease (OmpT) cleavage site was engineered into the switch loop of RF1, which enables its conditional inactivation during cell lysis. This facilitates extract production without additional processing steps, resulting in a scaleable extract production process. The RF1 mutant extract allows nnAA incorporation at previously intractable sites of an IgG1 and at multiple sites in the same polypeptide chain. Conjugation of cytotoxic agents to these nnAAs, yields homogeneous antibody drug conjugates (ADCs) that can be optimized for conjugation site, drug to antibody ratio (DAR) and linker-warheads designed for efficient tumor killing. This platform provides the means to generate therapeutic ADCs inaccessible by other methods that are efficient in their cytotoxin delivery to tumor with reduced dose-limiting toxicities and thus have the potential for better clinical impact.

摘要

琥珀密码子抑制用于插入非天然氨基酸(nnAAs)受到释放因子 1(RF1)的竞争限制。在这里,我们描述了一种 RF1 突变菌株的基因组工程改造,该菌株在无细胞蛋白质合成过程中提高了抑制效率,而在生物量生产过程中对细胞生长的影响不大。具体来说,在 RF1 的开关环中设计了一个外膜蛋白酶(OmpT)切割位点,使其在细胞裂解时能够条件性失活。这便于提取产物的生产,而无需额外的处理步骤,从而实现了可扩展的提取产物生产工艺。RF1 突变体提取物允许 nnAA 在 IgG1 的以前难以处理的部位以及同一多肽链中的多个部位掺入。将细胞毒性剂缀合到这些 nnAAs 上,得到均一的抗体药物偶联物(ADC),可以针对缀合部位、药物与抗体的比率(DAR)以及为有效杀伤肿瘤而设计的连接子弹头进行优化。该平台提供了一种方法,可以生成其他方法无法获得的治疗性 ADC,这些 ADC 能够有效递送至肿瘤的细胞毒素,从而减少剂量限制毒性,因此具有更好的临床效果的潜力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c207/5465077/e50fec5b361b/41598_2017_3192_Fig1_HTML.jpg

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