Protein purification via consecutive histidine–polyphosphate interaction

氨基三乙酸 组氨酸 聚磷酸盐 化学 串联亲和纯化 蛋白质纯化 亲和层析 生物化学 色谱法 螯合作用 重组DNA 组合化学 标志标签 氨基酸 有机化学 融合蛋白 磷酸盐 基因
作者
Zihao Zhou,Jin Jin,Xu Deng,Zongchao Jia
出处
期刊:Protein Science [Wiley]
卷期号:33 (6) 被引量:5
标识
DOI:10.1002/pro.5021
摘要

While nickel-nitrilotriacetic acid (Ni-NTA) has greatly advanced recombinant protein purification, its limitations, including nonspecific binding and partial purification for certain proteins, highlight the necessity for additional purification such as size exclusion and ion exchange chromatography. However, specialized equipment such as FPLC is typically needed but not often available in many laboratories. Here, we show a novel method utilizing polyphosphate (polyP) for purifying proteins with histidine repeats via non-covalent interactions. Our study demonstrates that immobilized polyP efficiently binds to histidine-tagged proteins across a pH range of 5.5-7.5, maintaining binding efficacy even in the presence of reducing agent DTT and chelating agent EDTA. We carried out experiments of purifying various proteins from cell lysates and fractions post-Ni-NTA. Our results demonstrate that polyP resin is capable of further purification post-Ni-NTA without the need for specialized equipment and without compromising protein activity. This cost-effective and convenient method offers a viable approach as a complementary approach to Ni-NTA.
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