TY - JOUR
T1 - Molecular mechanism of transcription inhibition by phage T7 gp2 protein
AU - Mekler, Vladimir
AU - Minakhin, Leonid
AU - Sheppard, Carol
AU - Wigneshweraraj, Sivaramesh
AU - Severinov, Konstantin
N1 - Funding Information:
This work was supported by the National Institutes of Health grants GM59295 and GM64530 and the Russian Academy of Sciences Presidium Molecular and Cellular Biology Program grant to K.S. S.W. is the recipient of a Biotechnology and Biological Sciences Research Council David Phillips Fellowship ( BB/E023703 ), and C.S. is the recipient of a Biotechnology and Biological Sciences Research Council Doctoral Training Grant studentship.
PY - 2011/11/11
Y1 - 2011/11/11
N2 - Escherichia coli T7 bacteriophage gp2 protein is a potent inhibitor of host RNA polymerase (RNAP). gp2 inhibits formation of open promoter complex by binding to the β′ jaw, an RNAP domain that interacts with downstream promoter DNA. Here, we used an engineered promoter with an optimized sequence to obtain and characterize a specific promoter complex containing RNAP and gp2. In this complex, localized melting of promoter DNA is initiated but does not propagate to include the point of the transcription start. As a result, the complex is transcriptionally inactive. Using a highly sensitive RNAP beacon assay, we performed quantitative real-time measurements of specific binding of the RNAP-gp2 complex to promoter DNA and various promoter fragments. In this way, the effect of gp2 on RNAP interaction with promoters was dissected. As expected, gp2 greatly decreased RNAP affinity to downstream promoter duplex. However, gp2 also inhibited RNAP binding to promoter fragments that lacked downstream promoter DNA that interacts with the β′ jaw. The inhibition was caused by gp2-mediated decrease of the RNAP binding affinity to template and non-template strand segments of the transcription bubble downstream of the - 10 promoter element. The inhibition of RNAP interactions with single-stranded segments of the transcription bubble by gp2 is a novel effect, which may occur via allosteric mechanism that is set in motion by the gp2 binding to the β′ jaw.
AB - Escherichia coli T7 bacteriophage gp2 protein is a potent inhibitor of host RNA polymerase (RNAP). gp2 inhibits formation of open promoter complex by binding to the β′ jaw, an RNAP domain that interacts with downstream promoter DNA. Here, we used an engineered promoter with an optimized sequence to obtain and characterize a specific promoter complex containing RNAP and gp2. In this complex, localized melting of promoter DNA is initiated but does not propagate to include the point of the transcription start. As a result, the complex is transcriptionally inactive. Using a highly sensitive RNAP beacon assay, we performed quantitative real-time measurements of specific binding of the RNAP-gp2 complex to promoter DNA and various promoter fragments. In this way, the effect of gp2 on RNAP interaction with promoters was dissected. As expected, gp2 greatly decreased RNAP affinity to downstream promoter duplex. However, gp2 also inhibited RNAP binding to promoter fragments that lacked downstream promoter DNA that interacts with the β′ jaw. The inhibition was caused by gp2-mediated decrease of the RNAP binding affinity to template and non-template strand segments of the transcription bubble downstream of the - 10 promoter element. The inhibition of RNAP interactions with single-stranded segments of the transcription bubble by gp2 is a novel effect, which may occur via allosteric mechanism that is set in motion by the gp2 binding to the β′ jaw.
KW - RNA polymerase
KW - T7 bacteriophage
KW - open promoter complex
KW - protein beacon assay
KW - transcription inhibition
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U2 - 10.1016/j.jmb.2011.09.029
DO - 10.1016/j.jmb.2011.09.029
M3 - Article
C2 - 21963987
AN - SCOPUS:80855133551
SN - 0022-2836
VL - 413
SP - 1016
EP - 1027
JO - Journal of molecular biology
JF - Journal of molecular biology
IS - 5
ER -