用于生产重组蛋白的模块化克隆工具包。

IF 4.1 3区 生物学 Q2 CELL BIOLOGY
Microbial Cell Pub Date : 2024-04-30 eCollection Date: 2024-01-01 DOI:10.15698/mic2024.04.821
Katrin Hieronimus, Tabea Donauer, Jonas Klein, Bastian Hinkel, Julia Vanessa Spänle, Anna Probst, Justus Niemeyer, Salina Kibrom, Anna Maria Kiefer, Luzia Schneider, Britta Husemann, Eileen Bischoff, Sophie Möhring, Nicolas Bayer, Dorothée Klein, Adrian Engels, Benjamin Gustav Ziehmer, Julian Stieβ, Pavlo Moroka, Michael Schroda, Marcel Deponte
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引用次数: 0

摘要

模块化克隆(MoClo)以标准化基因部件库为基础,可通过金门克隆在一锅反应中定向组装成转录单元和多基因构建体。在这里,一个由本科生组成的团队在国际基因工程机器(iGEM)竞赛框架内为原生动物利什曼原虫(Leishmania tarentolae)建立了一个MoClo工具包。我们的模块化工具包基于商业 LEXSY 表达载体的驯化版本,由 34 个基因部分组成,编码各种亲和标签、靶向信号以及荧光和发光蛋白。我们通过在透明梭状芽孢杆菌液体培养物中成功生产出 16 种不同的 SARS-CoV-2 棘蛋白受体结合域 (RBD) 标记版本,证明了我们的试剂盒的实用性。诱导 48 小时后,GST 标记的融合蛋白可获得最高产量的分泌型重组 RBD,而 C 端肽标记往往会被降解,导致分泌型 RBD 的产量降低。将分泌型 RBD 与合成的 O 型糖基化 SP20 模块融合后,其明显的分子质量变化在 10 kDa 左右。在 48 小时的诱导阶段,如果不使用 LEXSY 系统的三种抗生素,RBD 的产量也不会降低。此外,在先导实验中,我们成功地从L. tarentolae液体培养物的上清液中纯化了分泌的RBD。总之,我们建立了一个 MoClo 工具包,并示范了其在透明梭菌重组蛋白生产中的应用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A Modular Cloning Toolkit for the production of recombinant proteins in Leishmania tarentolae.

Modular Cloning (MoClo) is based on libraries of standardized genetic parts that can be directionally assembled via Golden Gate cloning in one-pot reactions into transcription units and multigene constructs. Here, a team of bachelor students established a MoClo toolkit for the protist Leishmania tarentolae in the frame of the international Genetically Engineered Machine (iGEM) competition. Our modular toolkit is based on a domesticated version of a commercial LEXSY expression vector and comprises 34 genetic parts encoding various affinity tags, targeting signals as well as fluorescent and luminescent proteins. We demonstrated the utility of our kit by the successful production of 16 different tagged versions of the receptor binding domain (RBD) of the SARS-CoV-2 spike protein in L. tarentolae liquid cultures. While highest yields of secreted recombinant RBD were obtained for GST-tagged fusion proteins 48 h post induction, C-terminal peptide tags were often degraded and resulted in lower yields of secreted RBD. Fusing secreted RBD to a synthetic O-glycosylation SP20 module resulted in an apparent molecular mass shift around 10 kDa. No disadvantage regarding the production of RBD was detected when the three antibiotics of the LEXSY system were omitted during the 48-h induction phase. Furthermore, the successful purification of secreted RBD from the supernatant of L. tarentolae liquid cultures was demonstrated in pilot experiments. In summary, we established a MoClo toolkit and exemplified its application for the production of recombinant proteins in L. tarentolae.

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来源期刊
Microbial Cell
Microbial Cell Multiple-
CiteScore
6.40
自引率
0.00%
发文量
32
审稿时长
12 weeks
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