RraA a Protein Inhibitor of RNase E Activity that Globally Modulates RNA Abundance in E. coli
نویسندگان
چکیده
Ribonuclease E (RNase E) has a key role in mRNA degradation and the processing of catalytic and structural RNAs in E. coli. We report the discovery of an evolutionarily conserved 17.4 kDa protein, here named RraA (regulator of ribonuclease activity A) that binds to RNase E and inhibits RNase E endonucleolytic cleavages without altering cleavage site specificity or interacting detectably with substrate RNAs. Overexpression of RraA circumvents the effects of an autoregulatory mechanism that normally maintains the RNase E cellular level within a narrow range, resulting in the genome-wide accumulation of RNase E-targeted transcripts. While not required for RraA action, the C-terminal RNase E region that serves as a scaffold for formation of a multiprotein degradosome complex modulates the inhibition of RNase E catalytic activity by RraA. Our results reveal a possible mechanism for the dynamic regulation of RNA decay and processing by inhibitory RNase binding proteins.
منابع مشابه
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The recently discovered RraA protein acts as an inhibitor of the essential endoribonuclease RNase E, and we demonstrated that ectopic expression of RraA affects the abundance of more than 700 transcripts in Escherichia coli (K. Lee, X. Zhan, J. Gao, J. Qiu, Y. Feng, R. Meganathan, S. N. Cohen, and G. Georgiou, Cell 114:623-634, 2003). We show that rraA is expressed from its own promoter, P(rraA...
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Dedication To my parents. Ellington, who allowed me to use his lab for RNase protection assay and growth rate experiment. I acknowledge Drs. sharing strains and antibodies. Many thanks to all the former and current Georgiou group members for their friendship and help. In particular, I thank Meng Zhao for doing the RraA and RraB co-precipitation experiment, Xiaoming Zhan for helping with the RPA...
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ورودعنوان ژورنال:
- Cell
دوره 114 شماره
صفحات -
تاریخ انتشار 2003