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Sphingosine Kinase Assay System with Fluorescent Detection in High Performance Liquid Chromatography
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  • Sphingosine Kinase Assay System with Fluorescent Detection in High Performance Liquid Chromatography
  • Sphingosine Kinase Assay System with Fluorescent Detection in High Performance Liquid Chromatography
저자명
Jin. You-Xun,Yoo. Hwan-Soo,Kihara. Akio,Choi. Chang-Hwan,Oh. Seik-Wan,Moon. Dong-Cheul,Igarashi. Yasuyuki,Lee. Yong-Moon
간행물명
Archives of pharmacal research : a publication of the Pharmaceutical Society of Korea
권/호정보
2006년|29권 11호|pp.1049-1054 (6 pages)
발행정보
대한약학회
파일정보
정기간행물|ENG|
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기타
이 논문은 한국과학기술정보연구원과 논문 연계를 통해 무료로 제공되는 원문입니다.
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기타언어초록

Activation of Sphingosine kinase (Sphk) increases a bioactive lipid, sphingosine 1-phosphate (S1P) and has been observed in a variety of cancer cells. Therefore, inhibition of Sphk activity was an important target for the development of anticancer drugs. As a searching tool for Sphk inhibitor, we developed fluorescent Sphk activity assay combined with high performance liquid chromatography (HPLC). Previously we established murine teraticarcinoma mutant F9-12 cells which lack S1P lyase and stably express Sphk1. By using F9-12 cells, optimal assay conditions were established as follows; $100;{mu}M;of;C_{17}-Sph;and;30;{mu}g$ protein of F9-12 cells lysate in 20 min. Sphingosine analog $C_{17}-Sph$ was efficiently phosphorylated by Sphk activity ($K_{m}:67.08;{mu}M,;V_{max};:1507.5;pmol/min/mg$). New product $C_{17}-S1P$ was separated from S1P in reversed-phase HPLC. In optimized conditions, 300 nM of phorbol 12-myristate 13-acetate (PMA) increased Sphk activity approximately twice while $20;{mu}M$ of N,N-dimethylsphingosine (DMS) reduced 70% of Sphk activity in F9-12 cells lysate. In conclusion, we established non-radioactive but convenient Sphk assay system by using HPLC and F9-12 cells.