Chemical inhibition of prometastatic lysyl-tRNA synthetase-laminin receptor interaction

Authors
Kim, Dae GyuLee, Jin YoungKwon, Nam HoonFang, PengfeiZhang, QianWang, JingYoung, Nicolas L.Guo, MinCho, Hye YoungMushtaq, Ameeq UlJeon, Young HoChoi, Jin WooHan, Jung MinKang, Ho WoongJoo, Jae EunHur, YounKang, WonyoungYang, HeekyoungNam, Do-HyunLee, Mi-SookLee, Jung WeonKim, Eun-SookMoon, AreeKim, KibomKim, DoyeunKang, Eun JooMoon, YoungjiRhee, Kyung HeeHan, Byung WooYang, Jee SunHan, GyoonheeYang, Won SukLee, CheoljuWang, Ming-WeiKim, Sunghoon
Issue Date
2014-01
Publisher
NATURE PUBLISHING GROUP
Citation
NATURE CHEMICAL BIOLOGY, v.10, no.1, pp.29 - U57
Abstract
Lysyl-tRNA synthetase (KRS), a protein synthesis enzyme in the cytosol, relocates to the plasma membrane after a laminin signal and stabilizes a 67-kDa laminin receptor (67LR) that is implicated in cancer metastasis; however, its potential as an antimetastatic therapeutic target has not been explored. We found that the small compound BC-K-YH16899, which binds KRS, impinged on the interaction of KRS with 67LR and suppressed metastasis in three different mouse models. The compound inhibited the KRS-67LR interaction in two ways. First, it directly blocked the association between KRS and 67LR. Second, it suppressed the dynamic movement of the N-terminal extension of KRS and reduced membrane localization of KRS. However, it did not affect the catalytic activity of KRS. Our results suggest that specific modulation of a cancer-related KRS-67LR interaction may offer a way to control metastasis while avoiding the toxicities associated with inhibition of the normal functions of KRS.
Keywords
ION-CYCLOTRON RESONANCE; MASS-SPECTROMETRY; SCATTERING SAXS; GENE-EXPRESSION; CELL INVASION; SYSTEM; CANCER; METASTASIS; CARCINOMA; PROTEINS; ION-CYCLOTRON RESONANCE; MASS-SPECTROMETRY; SCATTERING SAXS; GENE-EXPRESSION; CELL INVASION; SYSTEM; CANCER; METASTASIS; CARCINOMA; PROTEINS
ISSN
1552-4450
URI
https://pubs.kist.re.kr/handle/201004/127253
DOI
10.1038/NCHEMBIO.1381
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KIST Article > 2014
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