Family Report for: YcjY-like

Bacterial proteins. Enzymes of unknown function. YcjY gene involved in uptake and degradation of murein tripeptide under nitrogen starvation in E.Coli. Bacterial cell division gene

Title: Increased expression of genes involved in uptake and degradation of murein tripeptide under nitrogen starvation in Escherichia coli
Choi U, Park YH, Kim YR, Seok YJ, Lee CR
Ref: FEMS Microbiology Letters, 363:, 2016 : PubMed
Abstract


ESTHER: Choi_2016_FEMS.Microbiol.Lett_363_
PubMedSearch: Choi 2016 FEMS.Microbiol.Lett 363
PubMedID: 27231238
Gene_locus related to this paper: ecoli-ycjy

Abstract

Peptidoglycan (also known as murein) is an important envelope component of bacteria, and its turnover usually takes place at considerable levels during normal growth. Amino sugars and murein tripeptide resulting from murein degradation are used for resynthesis of peptidoglycan or as self-generated nutrients or energy sources for cell growth. PgrR (regulator of peptide glycan recycling; formerly YcjZ) was recently identified as a repressor of several genes participating in uptake and degradation of murein tripeptide. In this study, we identified the ycjG gene involved in murein tripeptide degradation as a new direct target of PgrR. The expression of PgrR-regulated genes including ycjY, mppA, mpaA and ycjG was repressed in the presence of a good nitrogen source, but their expression increased under poor nitrogen conditions. Under nitrogen starvation, the pgrR mutant cells exhibited faster growth than wild-type cells, implying that derepression of genes under the control of PgrR may help cells overcome nitrogen limitation. Therefore, these results suggest that nitrogen starvation induces derepression of PgrR-controlled genes involved in uptake and degradation of murein tripeptide, and this may stimulate the utilization of murein tripeptide as a nitrogen source.



        

Title: Harnessing single cell sorting to identify cell division genes and regulators in bacteria
Burke C, Liu M, Britton W, Triccas JA, Thomas T, Smith AL, Allen S, Salomon R, Harry E
Ref: PLoS ONE, 8:e60964, 2013 : PubMed
Abstract


ESTHER: Burke_2013_PLoS.One_8_e60964
PubMedSearch: Burke 2013 PLoS.One 8 e60964
PubMedID: 23565292
Gene_locus related to this paper: ecoli-ycjy

Abstract

Cell division is an essential cellular process that requires an array of known and unknown proteins for its spatial and temporal regulation. Here we develop a novel, high-throughput screening method for the identification of bacterial cell division genes and regulators. The method combines the over-expression of a shotgun genomic expression library to perturb the cell division process with high-throughput flow cytometry sorting to screen many thousands of clones. Using this approach, we recovered clones with a filamentous morphology for the model bacterium, Escherichia coli. Genetic analysis revealed that our screen identified both known cell division genes, and genes that have not previously been identified to be involved in cell division. This novel screening strategy is applicable to a wide range of organisms, including pathogenic bacteria, where cell division genes and regulators are attractive drug targets for antibiotic development.