Groer Gerhard J, Haslbeck Martin, Gessner André
Mikrobiologisches Institut-Klinische Mikrobiologie, Immunologie und Hygiene, Universitätsklinikum Erlangen, Wasserturmstrasse 3-5, D-91054 Erlangen, Germany.
J Chromatogr B Analyt Technol Biomed Life Sci. 2009 Jun 1;877(16-17):1643-50. doi: 10.1016/j.jchromb.2009.04.007. Epub 2009 Apr 8.
Affinity tags are valuable tools for high-throughput protein isolation in automated screenings or downstream processing approaches and are also widely used in laboratory applications for quick and easy access to many proteins. Here, we describe the preparative purification of soluble extended synaptotagmin 2 (rE-Syt2) at bench scale for basic structural and functional studies. Due to the low protein stability, a classical purification procedure without affinity tag was more powerful than isolation of His((6))-tagged rE-Syt2 and subsequent proteolytic tag-removal. Furthermore, expression analysis of truncated rE-Syt2 variants suggested a concept of interdependent-domain organization in proteins containing multiple C2 domains.
亲和标签是用于自动化筛选或下游处理方法中高通量蛋白质分离的宝贵工具,也广泛应用于实验室应用中,以便快速轻松地获取多种蛋白质。在此,我们描述了在实验室规模下对可溶性延伸突触结合蛋白2(rE-Syt2)进行制备性纯化,用于基础结构和功能研究。由于蛋白质稳定性较低,无亲和标签的经典纯化程序比分离His(6)标记的rE-Syt2并随后进行蛋白酶切去除标签更为有效。此外,截短的rE-Syt2变体的表达分析提出了一种在含有多个C2结构域的蛋白质中相互依赖结构域组织的概念。
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