Systematic Production of Inactivating and Non-inactivating Suppressor Mutations at the RelA Locus That Compensate the Detrimental Effects of Complete Spot Loss and Affect Glycogen Content in Escherichia Coli

Overview

Journal PLoS One

Specialties General Medicine
Science

Date 2014 Sep 5

PMID 25188023

Citations 10

Authors

Manuel Montero

Mehdi Rahimpour

Alejandro M Viale

Goizeder Almagro

Gustavo Eydallin

Angel Sevilla

Manuel Canovas

Cristina Bernal

Ana Belen Lozano

Francisco Jose Munoz

Edurne Baroja-Fernandez

Abdellatif Bahaji

Hirotada Mori

Francisco M Codoner

Javier Pozueta-Romero

Affiliations

Soon will be listed here.

Abstract

In Escherichia coli, ppGpp is a major determinant of growth and glycogen accumulation. Levels of this signaling nucleotide are controlled by the balanced activities of the ppGpp RelA synthetase and the dual-function hydrolase/synthetase SpoT. Here we report the construction of spoT null (ΔspoT) mutants obtained by transducing a ΔspoT allele from ΔrelAΔspoT double mutants into relA+ cells. Iodine staining of randomly selected transductants cultured on a rich complex medium revealed differences in glycogen content among them. Sequence and biochemical analyses of 8 ΔspoT clones displaying glycogen-deficient phenotypes revealed different inactivating mutations in relA and no detectable ppGpp when cells were cultured on a rich complex medium. Remarkably, although the co-existence of ΔspoT with relA proficient alleles has generally been considered synthetically lethal, we found that 11 ΔspoT clones displaying high glycogen phenotypes possessed relA mutant alleles with non-inactivating mutations that encoded stable RelA proteins and ppGpp contents reaching 45-85% of those of wild type cells. None of the ΔspoT clones, however, could grow on M9-glucose minimal medium. Both Sanger sequencing of specific genes and high-throughput genome sequencing of the ΔspoT clones revealed that suppressor mutations were restricted to the relA locus. The overall results (a) defined in around 4 nmoles ppGpp/g dry weight the threshold cellular levels that suffice to trigger net glycogen accumulation, (b) showed that mutations in relA, but not necessarily inactivating mutations, can be selected to compensate total SpoT function(s) loss, and (c) provided useful tools for studies of the in vivo regulation of E. coli RelA ppGpp synthetase.

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