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Engineering of an elastic scaffolding polyprotein based on an SH3-binding intrinsically disordered titin PEVK module

机译:基于SH3结合本质无序三角型钉素PEVK模块的弹性脚手架聚丙烯的工程

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摘要

Titin is a large elastic protein found in muscle that maintains the elasticity and structural integrity of the sarcomere. The PEVK region of titin is intrinsically disordered, highly elastic and serves as a hub to bind signaling proteins. Systematic investigation of the structure and affinity profile of the PEVK region will provide important information about the functions of titin. Since PEVK is highly heterogeneous due to extensive differential splicing from more than one hundred exons, we engineered and expressed polyproteins that consist of a defined number of identical single exon modules. These customized polyproteins reduce heterogeneity, amplify interactions of less dominant modules, and most importantly, provide tags for atomic force microscopy and allow more readily interpretable data from single-molecule techniques.Expression and purification of recombinant polyprotein with repeat regions presented many technical challenges: recombination events in tandem repeats of identical DNA sequences exacerbated by high GC content, toxicity of polymer plasmid and expressed protein to the bacteria; early truncation of proteins expressed with different numbers of modules; and extreme sensitivity to proteolysis. We have investigated a number of in vitro and in vivo bacterial and yeast expression systems, as well as baculoviral systems as potential solutions to these problems. We successfully expressed and purified in gram quantities a polyprotein derived from human titin exon 172 using Pichia pastoris yeast. This study provides valuable insights into the technical challenges regarding the engineering and purification of a tandem repeat sequence of an intrinsically disordered biopolymer.
机译:Titin是一种在肌肉中发现的大型弹性蛋白,可维持肌节的弹性和结构完整性。 titin的PEVK区本质上是无序的,具有高弹性,并充当结合信号蛋白的枢纽。对PEVK区域的结构和亲和力概况的系统研究将提供有关titin功能的重要信息。由于PEVK由于来自一百多个外显子的广泛差异剪接而高度异质,因此我们设计并表达了由确定数量的相同单外显子模块组成的多蛋白。这些定制的多蛋白可减少异质性,扩大主要模块之间的相互作用,最重要的是为原子力显微镜提供标签,并允许更容易地解释单分子技术的数据。具有重复区域的重组多蛋白的表达和纯化面临许多技术挑战:重组高GC含量,聚合物质粒的毒性和表达的蛋白对细菌的影响加剧了相同DNA序列串联重复的事件;早期截短不同数量模块表达的蛋白质;对蛋白水解反应极其敏感。我们已经研究了许多体外和体内细菌和酵母表达系统以及杆状病毒系统,作为解决这些问题的潜在方法。我们成功地表达和纯化了使用巴斯德毕赤酵母酵母从人纤溶酶外显子172衍生的多蛋白克。这项研究提供了宝贵的见解,涉及有关固有无序生物聚合物串联重复序列的工程设计和纯化的技术挑战。

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