IRIS publication 43335494
Analysis of the Isoprenoid Biosynthesis Pathways in Listeria monocytogenes Reveals a Role for the Alternative 2-C-Methyl-D-Erythritol 4-Phosphate Pathway in Murine Infection
RIS format for Endnote and similar
TY - JOUR - Begley, M,Bron, PA,Heuston, S,Casey, PG,Englert, N,Wiesner, J,Jomaa, H,Gahan, CGM,Hill, C - 2008 - January - Infection and Immunity - Analysis of the Isoprenoid Biosynthesis Pathways in Listeria monocytogenes Reveals a Role for the Alternative 2-C-Methyl-D-Erythritol 4-Phosphate Pathway in Murine Infection - Validated - () - DELTA T-CELLS ESCHERICHIA-COLI PHOSPHATE-PATHWAY BACILLUS-SUBTILIS GENE-EXPRESSION GENOME SEQUENCE IN-VITRO IDENTIFICATION INTEGRATION ACTIVATION - 76 - 5392 - 5401 - Most bacteria synthesize isoprenoids through one of two essential pathways which provide the basic building block, isopentyl diphosphate (IPP): either the classical mevalonate pathway or the alternative non-mevalonate 2-C-methyl-D-erythritol 4-phosphate (MEP) pathway. However, postgenomic analyses of the Listeria monocytogenes genome revealed that this pathogen possesses the genetic capacity to produce the complete set of enzymes involved in both pathways. The nonpathogenic species Listeria innocua naturally lacks the last two genes ( gcpE and lytB) of the MEP pathway, and bioinformatic analyses strongly suggest that the genes have been lost through evolution. In the present study we show that heterologous expression of gcpE and lytB in L. innocua can functionally restore the MEP pathway in this organism and confer on it the ability to induce V gamma 9V delta 2 T cells. We have previously confirmed that both pathways are functional in L. monocytogenes and can provide sufficient IPP for normal growth in laboratory media (M. Begley, C. G. Gahan, A. K. Kollas, M. Hintz, C. Hill, H. Jomaa, and M. Eberl, FEBS Lett. 561: 99-104, 2004). Here we describe a targeted mutagenesis strategy to create a double pathway mutant in L. monocytogenes which cannot grow in the absence of exogenously provided mevalonate, confirming the requirement for at least one intact pathway for growth. In addition, murine studies revealed that mutants lacking the MEP pathway were impaired in virulence relative to the parent strain during intraperitoneal infection, while mutants lacking the classical mevalonate pathway were not impaired in virulence potential. In vivo bioluminescence imaging also confirmed in vivo expression of the gcpE gene ( MEP pathway) during murine infection. - DOI 10.1128/IAI.01376-07 DA - 2008/01 ER -
BIBTeX format for JabRef and similar
@article{V43335494,
= {Begley, M and Bron, PA and Heuston, S and Casey, PG and Englert, N and Wiesner, J and Jomaa, H and Gahan, CGM and Hill, C },
= {2008},
= {January},
= {Infection and Immunity},
= {Analysis of the Isoprenoid Biosynthesis Pathways in Listeria monocytogenes Reveals a Role for the Alternative 2-C-Methyl-D-Erythritol 4-Phosphate Pathway in Murine Infection},
= {Validated},
= {()},
= {DELTA T-CELLS ESCHERICHIA-COLI PHOSPHATE-PATHWAY BACILLUS-SUBTILIS GENE-EXPRESSION GENOME SEQUENCE IN-VITRO IDENTIFICATION INTEGRATION ACTIVATION},
= {76},
pages = {5392--5401},
= {{Most bacteria synthesize isoprenoids through one of two essential pathways which provide the basic building block, isopentyl diphosphate (IPP): either the classical mevalonate pathway or the alternative non-mevalonate 2-C-methyl-D-erythritol 4-phosphate (MEP) pathway. However, postgenomic analyses of the Listeria monocytogenes genome revealed that this pathogen possesses the genetic capacity to produce the complete set of enzymes involved in both pathways. The nonpathogenic species Listeria innocua naturally lacks the last two genes ( gcpE and lytB) of the MEP pathway, and bioinformatic analyses strongly suggest that the genes have been lost through evolution. In the present study we show that heterologous expression of gcpE and lytB in L. innocua can functionally restore the MEP pathway in this organism and confer on it the ability to induce V gamma 9V delta 2 T cells. We have previously confirmed that both pathways are functional in L. monocytogenes and can provide sufficient IPP for normal growth in laboratory media (M. Begley, C. G. Gahan, A. K. Kollas, M. Hintz, C. Hill, H. Jomaa, and M. Eberl, FEBS Lett. 561: 99-104, 2004). Here we describe a targeted mutagenesis strategy to create a double pathway mutant in L. monocytogenes which cannot grow in the absence of exogenously provided mevalonate, confirming the requirement for at least one intact pathway for growth. In addition, murine studies revealed that mutants lacking the MEP pathway were impaired in virulence relative to the parent strain during intraperitoneal infection, while mutants lacking the classical mevalonate pathway were not impaired in virulence potential. In vivo bioluminescence imaging also confirmed in vivo expression of the gcpE gene ( MEP pathway) during murine infection.}},
= {DOI 10.1128/IAI.01376-07},
source = {IRIS}
}Data as stored in IRIS
| AUTHORS | Begley, M,Bron, PA,Heuston, S,Casey, PG,Englert, N,Wiesner, J,Jomaa, H,Gahan, CGM,Hill, C | ||
| YEAR | 2008 | ||
| MONTH | January | ||
| JOURNAL_CODE | Infection and Immunity | ||
| TITLE | Analysis of the Isoprenoid Biosynthesis Pathways in Listeria monocytogenes Reveals a Role for the Alternative 2-C-Methyl-D-Erythritol 4-Phosphate Pathway in Murine Infection | ||
| STATUS | Validated | ||
| TIMES_CITED | () | ||
| SEARCH_KEYWORD | DELTA T-CELLS ESCHERICHIA-COLI PHOSPHATE-PATHWAY BACILLUS-SUBTILIS GENE-EXPRESSION GENOME SEQUENCE IN-VITRO IDENTIFICATION INTEGRATION ACTIVATION | ||
| VOLUME | 76 | ||
| ISSUE | |||
| START_PAGE | 5392 | ||
| END_PAGE | 5401 | ||
| ABSTRACT | Most bacteria synthesize isoprenoids through one of two essential pathways which provide the basic building block, isopentyl diphosphate (IPP): either the classical mevalonate pathway or the alternative non-mevalonate 2-C-methyl-D-erythritol 4-phosphate (MEP) pathway. However, postgenomic analyses of the Listeria monocytogenes genome revealed that this pathogen possesses the genetic capacity to produce the complete set of enzymes involved in both pathways. The nonpathogenic species Listeria innocua naturally lacks the last two genes ( gcpE and lytB) of the MEP pathway, and bioinformatic analyses strongly suggest that the genes have been lost through evolution. In the present study we show that heterologous expression of gcpE and lytB in L. innocua can functionally restore the MEP pathway in this organism and confer on it the ability to induce V gamma 9V delta 2 T cells. We have previously confirmed that both pathways are functional in L. monocytogenes and can provide sufficient IPP for normal growth in laboratory media (M. Begley, C. G. Gahan, A. K. Kollas, M. Hintz, C. Hill, H. Jomaa, and M. Eberl, FEBS Lett. 561: 99-104, 2004). Here we describe a targeted mutagenesis strategy to create a double pathway mutant in L. monocytogenes which cannot grow in the absence of exogenously provided mevalonate, confirming the requirement for at least one intact pathway for growth. In addition, murine studies revealed that mutants lacking the MEP pathway were impaired in virulence relative to the parent strain during intraperitoneal infection, while mutants lacking the classical mevalonate pathway were not impaired in virulence potential. In vivo bioluminescence imaging also confirmed in vivo expression of the gcpE gene ( MEP pathway) during murine infection. | ||
| PUBLISHER_LOCATION | |||
| ISBN_ISSN | |||
| EDITION | |||
| URL | |||
| DOI_LINK | DOI 10.1128/IAI.01376-07 | ||
| FUNDING_BODY | |||
| GRANT_DETAILS |