Feedback regulation of small RNA processing by the cleavage product.

RNA Biol

a Department of Microbiology, Immunobiology and Genetics, Max F. Perutz Laboratories (MFPL) , University of Vienna, Vienna Biocenter (VBC), Vienna , Austria.

Published: August 2019

Many bacterial small RNAs (sRNAs) are processed resulting in variants with roles potentially distinct from the primary sRNAs. In sRNA GlmZ activates expression of by base-pairing when the levels of glucosamine-6-phosphate (GlcN6P) are low. GlmS synthesizes GlcN6P, which is required for cell envelope biosynthesis. When dispensable, GlmZ is cleaved by RNase E in the base-pairing sequence. Processing requires protein RapZ, which binds GlmZ and recruits RNase E by interaction. Cleavage is counteracted by the homologous sRNA GlmY, which accumulates upon GlcN6P scarcity and sequesters RapZ. Here, we report a novel role for a processed sRNA. We observed that processing of GlmZ is never complete . Even upon RapZ overproduction, a fraction of GlmZ remains full-length, while the 5' cleavage product (GlmZ*) accumulates. GlmZ* retains all elements required for RapZ binding. Accordingly, GlmZ* can displace full-length GlmZ from RapZ and counteract processing . To mimic GlmZ* , sRNA chimeras were employed consisting of foreign 3' ends including a terminator fused to the 3' end of GlmZ*. , these chimeras perform indistinguishable from GlmZ*. Expression of the chimeras inhibited processing of endogenous GlmZ, causing moderate upregulation of GlmS synthesis. Hence, accumulation of GlmZ* prevents complete GlmZ turnover. This mechanism may serve to adjust a robust basal expression level that is buffered against fluctuations in RapZ availability.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC6602413PMC
http://dx.doi.org/10.1080/15476286.2019.1612693DOI Listing

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