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Cited 2 time in webofscience Cited 2 time in scopus
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An Easy Way for the Rapid Purification of Recombinant Proteins from Helicobacter pylori Using a Newly Designed Expression Vector

Authors
Kang, Hyung-LyunJo, Jin-SungKwon, Soon-UckSong, Jae-YoungSeo, Ji-HyunCho, Myung-JeBaik, Seung-ChulYoun, Hee-ShangRhee, Kwang-HoLee, Woo-Kon
Issue Date
Jul-2014
Publisher
MICROBIOLOGICAL SOCIETY KOREA
Keywords
Helicobacter pylori; pBKHGC; vector
Citation
JOURNAL OF MICROBIOLOGY, v.52, no.7, pp 604 - 608
Pages
5
Indexed
SCIE
SCOPUS
KCI
Journal Title
JOURNAL OF MICROBIOLOGY
Volume
52
Number
7
Start Page
604
End Page
608
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/18924
DOI
10.1007/s12275-014-3679-y
ISSN
1225-8873
1976-3794
Abstract
We constructed a H. pylori expression vector which consisted of both a His-tag and a GST tag as purification tools for recombinant protein and a chloramphenicol resistant cat gene as a reporter. The backbone of the vector pBK contained an ColEI origin of replication and a kanamycin resistant gene. A set of oligos for the His-tag and the PCR product of gst (glutathione S-transferase) gene were inserted sequentially in frame in the multi-cloning site of pBK. The orf of cat was inserted downstream of the gst to generate pBKHGC. The 3' part of H. pylori clpB and flaA were cloned into the vector which was introduced into H. pylori. Recombinant proteins were purified by GSH affinity column, digested with thrombin and were analyzed by western blotting. The final recombinant proteins were successfully purified.
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의과대학 (의학과)
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