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Expression and Purification of the Helicase-like Subdomains, H1 and H23, of Reverse Gyrase from A. fulgidus for Heteronuclear NMR studyExpression and Purification of the Helicase-like Subdomains, H1 and H23, of Reverse Gyrase from A. fulgidus for Heteronuclear NMR study
- Other Titles
- Expression and Purification of the Helicase-like Subdomains, H1 and H23, of Reverse Gyrase from A. fulgidus for Heteronuclear NMR study
- Issue Date
- 2015
- Publisher
- 한국자기공명학회
- Keywords
- NMR; reverse gyrase; subdomain; protein purification; helicase-like; hyperthermophile
- Citation
- Journal of the Korean Magnetic Resonance Society, v.19, no.2, pp 95 - 98
- Pages
- 4
- Indexed
- KCI
- Journal Title
- Journal of the Korean Magnetic Resonance Society
- Volume
- 19
- Number
- 2
- Start Page
- 95
- End Page
- 98
- ISSN
- 1226-6531
- Abstract
- Reverse gyrase is a hyperthermophile specific protein which introduces positive supercoils into DNA molecules. Reverse gyrase consists of an N-terminal helicase-like domain and a C-terminal topoisomerase domain. The helicase-like domain shares the three-dimensional structure with two tandem RecA-folds (H1 and H2), in which the subdomain H2 is interrupted by the latch domain (H3). To understand the physical property of the hyperthermophile-specific protein, two subdomains af_H1 and af_H23 have been cloned into E. coli expression vector, pET28a. The 15N-labeled af_H1 and af_H23 proteins were expressed and purified for heteronuclear NMR study. The af_H1 protein exhibits the well-dispersion of amide signals in its 1H/15N-HSQC spectra and thus further NMR study continues to be progressed.
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