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BINDING OF A 50-KD PROTEIN TO A U-RICH SEQUENCE IN AN MESSENGER-RNA ENCODING A PROLINE-RICH PROTEIN THAT IS DESTABILIZED BY FUNGAL ELICITOR

被引:37
作者
ZHANG, SQ [1 ]
MEHDY, MC [1 ]
机构
[1] UNIV TEXAS, DEPT BOT, AUSTIN, TX 78713 USA
来源
PLANT CELL | 1994年 / 6卷 / 01期
关键词
D O I
10.1105/tpc.6.1.135
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The mRNA encoding the bean proline-rich protein PvPRP1 has been shown previously to be destabilized in elicitor-treated cells. In this study, we identified a 50-kD protein in cellular extracts that binds specifically to the PvPRP1 mRNA by UV cross-linking assays. Using P-32-labeled RNAs transcribed in vitro from a series of 5' deleted PvPRP1 cDNA clones, we demonstrated that the PvPRP1 mRNA binding protein (PRP-BP) binds to a 27-nucleotide U-rich (similar to 60%) domain in the 3' untranslated region. Poly(U) and, to a lesser extent, poly(A-U) competed for the PRP-BP binding activity. PRP-BP activity is redox regulated in vitro, as shown by the effects of sulfhydryl-modifying reagents on the RNA binding activity. Treatment of cellular extracts with the reducing agents DTT and beta-mercaptoethanol increased binding activity, whereas treatment with the oxidizing agent diamide and the alkylating agent N-ethylmaleimide inhibited binding. In extracts from elicitor-treated cells, PRP-BP activity increased approximately fivefold prior to rapid PvPRP1 mRNA degradation. The increase in PRP-BP activity was apparently due to post-translational regulation because control and elicitor-treated cell extracts supplemented with DTT showed high comparable levels of RNA binding activity. The kinetics of PRP-BP activation after elicitor treatment and its capacity for redox regulation in vitro suggested that PRP-BP may function in the elicitor-induced destabilization of PvPRP1 mRNA.
引用
收藏
页码:135 / 145
页数:11
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