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对抗体的半胱氨酸封端修饰的机制理解有助于在活的哺乳动物细胞中进行选择性化学工程改造。

Mechanistic understanding of the cysteine capping modifications of antibodies enables selective chemical engineering in live mammalian cells.

作者信息

Zhong Xiaotian, He Tao, Prashad Amar S, Wang Wenge, Cohen Justin, Ferguson Darren, Tam Amy S, Sousa Eric, Lin Laura, Tchistiakova Lioudmila, Gatto Scott, D'Antona Aaron, Luan Yen-Tung, Ma Weijun, Zollner Richard, Zhou Jing, Arve Bo, Somers Will, Kriz Ronald

机构信息

BioMedicine Design, Medicinal Sciences, Pfizer Worldwide R&D, Cambridge, MA 02139, United States.

BioMedicine Design, Medicinal Sciences, Pfizer Worldwide R&D, Cambridge, MA 02139, United States.

出版信息

J Biotechnol. 2017 Apr 20;248:48-58. doi: 10.1016/j.jbiotec.2017.03.006. Epub 2017 Mar 11.

DOI:10.1016/j.jbiotec.2017.03.006
PMID:28300660
Abstract

Protein modifications by intricate cellular machineries often redesign the structure and function of existing proteins to impact biological networks. Disulfide bond formation between cysteine (Cys) pairs is one of the most common modifications found in extracellularly-destined proteins, key to maintaining protein structure. Unpaired surface cysteines on secreted mammalian proteins are also frequently found disulfide-bonded with free Cys or glutathione (GSH) in circulation or culture, the mechanism for which remains unknown. Here we report that these so-called Cys-capping modifications take place outside mammalian cells, not in the endoplasmic reticulum (ER) where oxidoreductase-mediated protein disulfide formation occurs. Unpaired surface cysteines of extracellularly-arrived proteins such as antibodies are uncapped upon secretion before undergoing disulfide exchange with cystine or oxidized GSH in culture medium. This observation has led to a feasible way to selectively modify the nucleophilic thiol side-chain of cell-surface or extracellular proteins in live mammalian cells, by applying electrophiles with a chemical handle directly into culture medium. These findings provide potentially an effective approach for improving therapeutic conjugates and probing biological systems.

摘要

复杂的细胞机制对蛋白质的修饰常常会重新设计现有蛋白质的结构和功能,从而影响生物网络。半胱氨酸(Cys)对之间形成二硫键是细胞外定向蛋白质中最常见的修饰之一,是维持蛋白质结构的关键。分泌的哺乳动物蛋白质上未配对的表面半胱氨酸也经常在循环或培养中与游离半胱氨酸或谷胱甘肽(GSH)形成二硫键,其机制尚不清楚。在这里,我们报告这些所谓的半胱氨酸封端修饰发生在哺乳动物细胞外,而不是在内质网(ER)中,氧化还原酶介导的蛋白质二硫键形成发生在内质网中。诸如抗体等细胞外到达的蛋白质的未配对表面半胱氨酸在分泌时被解封,然后在培养基中与胱氨酸或氧化型谷胱甘肽进行二硫键交换。这一观察结果导致了一种可行的方法,即通过将带有化学手柄的亲电试剂直接应用于培养基中,选择性地修饰活哺乳动物细胞中细胞表面或细胞外蛋白质的亲核硫醇侧链。这些发现可能为改进治疗性偶联物和探索生物系统提供一种有效的方法。

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