Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilis

Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilis

The Gram-positive model bacterium Bacillus subtilis contains two glutamate dehydrogenase-encoding genes, rocG and gudB. While the rocG gene encodes the functional GDH, the gudB gene is cryptic (gudBCR) in the laboratory strain 168 due to a perfect 18 bp-long direct repeat that renders the GudB enzym...

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Main Authors: Lorena eStannek, Katrin eGunka, Rachel eCare, Ulf eGerth, Fabian Moritz Commichau
Format: Article
Language:English
Published: Frontiers Media S.A. 2015-01-01
Series:Frontiers in Microbiology
Subjects:
Glutamate Dehydrogenase
Protein Folding
Proteolysis
Protein modification
arginine phosphorylation
Online Access:http://journal.frontiersin.org/Journal/10.3389/fmicb.2014.00758/full
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spelling doaj-ee3e6f6821354b97b8289e93dddd07b52020-11-24T23:58:11ZengFrontiers Media S.A.Frontiers in Microbiology1664-302X2015-01-01510.3389/fmicb.2014.00758127667Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilisLorena eStannek0Katrin eGunka1Rachel eCare2Ulf eGerth3Fabian Moritz Commichau4University of GöttingenUniversity of GöttingenUniversity of GöttingenUniversity of GreifswaldUniversity of GöttingenThe Gram-positive model bacterium Bacillus subtilis contains two glutamate dehydrogenase-encoding genes, rocG and gudB. While the rocG gene encodes the functional GDH, the gudB gene is cryptic (gudBCR) in the laboratory strain 168 due to a perfect 18 bp-long direct repeat that renders the GudB enzyme inactive and unstable. Although constitutively expressed the GudBCR protein can hardly be detected in B. subtilis as it is rapidly degraded within stationary growth phase. Its high instability qualifies GudBCR as a model substrate for studying protein turnover in B. subtilis. Recently, we have developed a visual screen to monitor the GudBCR stability in the cell using a GFP-GudBCR fusion. Using fluorescent microscopy we found that the GFP protein is simultaneously degraded together with GudBCR. This allows us to analyze the stability of GudBCR in living cells. By combining the visual screen with a transposon mutagenesis approach we looked for mutants that show an increased fluorescence signal compared to the wild type indicating a stabilized GFP-GudBCR fusion. We observed, that disruption of the arginine kinase encoding gene mcsB upon transposon insertion leads to increased amounts of the GFP-GudBCR fusion in this mutant. Deletion of the cognate arginine phosphatase YwlE in contrast results in reduced levels of the GFP-GudBCR fusion. Recently, it was shown that the kinase McsB is involved in phosphorylation of GudBCR on arginine residues. Here we show that selected arginine-lysine point mutations of GudBCR exhibit no influence on degradation. The activity of McsB and YwlE, however, are crucial for the activation and inhibition, respectively, of a proteolytic machinery that efficiently degrades the unstable GudBCR protein in B. subtilis.http://journal.frontiersin.org/Journal/10.3389/fmicb.2014.00758/fullGlutamate DehydrogenaseProtein FoldingProteolysisProtein modificationarginine phosphorylation
collection DOAJ
language English
format Article
sources DOAJ
author Lorena eStannek
Katrin eGunka
Rachel eCare
Ulf eGerth
Fabian Moritz Commichau
spellingShingle Lorena eStannek
Katrin eGunka
Rachel eCare
Ulf eGerth
Fabian Moritz Commichau
Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilis
Frontiers in Microbiology
Glutamate Dehydrogenase
Protein Folding
Proteolysis
Protein modification
arginine phosphorylation
author_facet Lorena eStannek
Katrin eGunka
Rachel eCare
Ulf eGerth
Fabian Moritz Commichau
author_sort Lorena eStannek
title Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilis
title_short Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilis
title_full Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilis
title_fullStr Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilis
title_full_unstemmed Factors that mediate and prevent degradation of the inactive and unstable GudB protein in Bacillus subtilis
title_sort factors that mediate and prevent degradation of the inactive and unstable gudb protein in bacillus subtilis
publisher Frontiers Media S.A.
series Frontiers in Microbiology
issn 1664-302X
publishDate 2015-01-01
description The Gram-positive model bacterium Bacillus subtilis contains two glutamate dehydrogenase-encoding genes, rocG and gudB. While the rocG gene encodes the functional GDH, the gudB gene is cryptic (gudBCR) in the laboratory strain 168 due to a perfect 18 bp-long direct repeat that renders the GudB enzyme inactive and unstable. Although constitutively expressed the GudBCR protein can hardly be detected in B. subtilis as it is rapidly degraded within stationary growth phase. Its high instability qualifies GudBCR as a model substrate for studying protein turnover in B. subtilis. Recently, we have developed a visual screen to monitor the GudBCR stability in the cell using a GFP-GudBCR fusion. Using fluorescent microscopy we found that the GFP protein is simultaneously degraded together with GudBCR. This allows us to analyze the stability of GudBCR in living cells. By combining the visual screen with a transposon mutagenesis approach we looked for mutants that show an increased fluorescence signal compared to the wild type indicating a stabilized GFP-GudBCR fusion. We observed, that disruption of the arginine kinase encoding gene mcsB upon transposon insertion leads to increased amounts of the GFP-GudBCR fusion in this mutant. Deletion of the cognate arginine phosphatase YwlE in contrast results in reduced levels of the GFP-GudBCR fusion. Recently, it was shown that the kinase McsB is involved in phosphorylation of GudBCR on arginine residues. Here we show that selected arginine-lysine point mutations of GudBCR exhibit no influence on degradation. The activity of McsB and YwlE, however, are crucial for the activation and inhibition, respectively, of a proteolytic machinery that efficiently degrades the unstable GudBCR protein in B. subtilis.
topic Glutamate Dehydrogenase
Protein Folding
Proteolysis
Protein modification
arginine phosphorylation
url http://journal.frontiersin.org/Journal/10.3389/fmicb.2014.00758/full
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