T7Max transcription system

被引:13
作者
Deich, Christopher [1 ]
Cash, Brock [1 ]
Sato, Wakana [1 ]
Sharon, Judee [1 ]
Aufdembrink, Lauren [1 ]
Gaut, Nathaniel J. [1 ]
Heili, Joseph [1 ]
Stokes, Kaitlin [1 ]
Engelhart, Aaron E. [1 ]
Adamala, Katarzyna P. [1 ]
机构
[1] Univ Minnesota, Dept Genet Cell Biol & Dev, Minneapolis, MN 55455 USA
基金
美国国家卫生研究院; 美国国家航空航天局; 美国国家科学基金会;
关键词
in vitro transcription; in vitro translation; synthetic cells; cell-free protein expression; IN-VITRO; RNA-POLYMERASE; PROTEIN; EXPRESSION; STABILITY; VIVO; GENE; DNA;
D O I
10.1186/s13036-023-00323-1
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
BackgroundEfficient cell-free protein expression from linear DNA templates has remained a challenge primarily due to template degradation. In addition, the yields of transcription in cell-free systems lag behind transcriptional efficiency of live cells. Most commonly used in vitro translation systems utilize T7 RNA polymerase, which is also the enzyme included in many commercial kits.ResultsHere we present characterization of a variant of T7 RNA polymerase promoter that acts to significantly increase the yields of gene expression within in vitro systems. We have demonstrated that T7Max increases the yield of translation in many types of commonly used in vitro protein expression systems. We also demonstrated increased protein expression yields from linear templates, allowing the use of T7Max driven expression from linear templates.ConclusionsThe modified promoter, termed T7Max, recruits standard T7 RNA polymerase, so no protein engineering is needed to take advantage of this method. This technique could be used with any T7 RNA polymerase- based in vitro protein expression system.
引用
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页数:14
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