Statements in which the resource exists as a subject.
PredicateObject
rdf:type
lifeskim:mentions
pubmed:issue
15
pubmed:dateCreated
2008-7-18
pubmed:abstractText
Listeria monocytogenes is able to efficiently utilize glycerol as a carbon source. In a defined minimal medium, the growth rate (during balanced growth) in the presence of glycerol is similar to that in the presence of glucose or cellobiose. Comparative transcriptome analyses of L. monocytogenes showed high-level transcriptional upregulation of the genes known to be involved in glycerol uptake and metabolism (glpFK and glpD) in the presence of glycerol (compared to that in the presence of glucose and/or cellobiose). Levels of expression of the genes encoding a second putative glycerol uptake facilitator (GlpF(2)) and a second putative glycerol kinase (GlpK(2)) were less enhanced under these conditions. GlpK(1) but not GlpK(2) was essential for glycerol catabolism in L. monocytogenes under extracellular conditions, while the loss of GlpK(1) affected replication in Caco-2 cells less than did the loss of GlpK(2) and GlpD. Additional genes whose transcription levels were higher in the presence of glycerol than in the presence of glucose and cellobiose included those for two dihydroxyacetone (Dha) kinases and many genes that are under carbon catabolite repression control. Transcriptional downregulation in the presence of glycerol (compared to those in the presence glucose and cellobiose) was observed for several genes and operons that are positively regulated by glucose, including genes involved in glycolysis, N metabolism, and the biosynthesis of branched-chain amino acids. The highest level of transcriptional upregulation was observed for all PrfA-dependent genes during early and late logarithmic growth in glycerol. Under these conditions, a low level of HPr-Ser-P and a high level of HPr-His-P were present in the cells, suggesting that all enzyme IIA (EIIA) (or EIIB) components of the phosphotransferase system (PTS) permeases expressed will be phosphorylated. These and other data suggest that the phosphorylation state of PTS permeases correlates with PrfA activity.
pubmed:commentsCorrections
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pubmed:language
eng
pubmed:journal
pubmed:citationSubset
IM
pubmed:chemical
pubmed:status
MEDLINE
pubmed:month
Aug
pubmed:issn
1098-5530
pubmed:author
pubmed:issnType
Electronic
pubmed:volume
190
pubmed:owner
NLM
pubmed:authorsComplete
Y
pubmed:pagination
5412-30
pubmed:dateRevised
2009-11-19
pubmed:meshHeading
pubmed-meshheading:18502850-Humans, pubmed-meshheading:18502850-Animals, pubmed-meshheading:18502850-Mice, pubmed-meshheading:18502850-Glucose, pubmed-meshheading:18502850-Glycerol, pubmed-meshheading:18502850-Phosphorylation, pubmed-meshheading:18502850-Epithelial Cells, pubmed-meshheading:18502850-Listeria monocytogenes, pubmed-meshheading:18502850-Macrophages, pubmed-meshheading:18502850-Bacterial Proteins, pubmed-meshheading:18502850-Membrane Transport Proteins, pubmed-meshheading:18502850-Cell Line, pubmed-meshheading:18502850-Genetic Complementation Test, pubmed-meshheading:18502850-Peptide Termination Factors, pubmed-meshheading:18502850-Down-Regulation, pubmed-meshheading:18502850-Cellobiose, pubmed-meshheading:18502850-Gene Deletion, pubmed-meshheading:18502850-Gene Expression Profiling
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