T7 RNA聚合酶
RNA聚合酶
分子生物学
化学
溶解
重组DNA
聚合酶
大肠杆菌
核糖核酸
RNA依赖性RNA聚合酶
生物化学
噬菌体
抄写(语言学)
DNA
生物
基因
哲学
语言学
出处
期刊:CSH Protocols
[Cold Spring Harbor Laboratory Press]
日期:2013-11-01
卷期号:2013 (11): pdb.prot078527-pdb.prot078527
被引量:48
标识
DOI:10.1101/pdb.prot078527
摘要
For large-scale transcription reactions or for cost savings, a laboratory may want to prepare its own recombinant T7-, SP6-, or T3-phage RNA polymerases. It is convenient to perform this preparation every 2-3 years and have a consistent and reliable source of phage RNA polymerase for many in vitro transcription reactions. In the protocol presented here, the recombinant plasmid expressing T7 RNA polymerase (RNAP) as a his6-tagged molecule is under an isopropyl β-d-1-thio-galactopyranoside (IPTG)-inducible promoter. The bacteria are lysed by sonication, the his6-tagged protein in the bacterial lysate is purified by binding to Ni-NTA agarose, and the resin is then extensively washed and eluted with imidazole. The purified enzyme is dialyzed against a glycerol-containing storage buffer and can then be stored for months or years at -20°C.
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