Negative selection of Plasmodium falciparum reveals targeted gene deletion by double crossover recombination
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Duraisingh, MT
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PO Royal Melbourne Hosp, Walter & Eliza Hall Inst Med Res, Melbourne, Vic 3050, AustraliaPO Royal Melbourne Hosp, Walter & Eliza Hall Inst Med Res, Melbourne, Vic 3050, Australia
Duraisingh, MT
[1
]
Triglia, T
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PO Royal Melbourne Hosp, Walter & Eliza Hall Inst Med Res, Melbourne, Vic 3050, AustraliaPO Royal Melbourne Hosp, Walter & Eliza Hall Inst Med Res, Melbourne, Vic 3050, Australia
Triglia, T
[1
]
Cowman, AF
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PO Royal Melbourne Hosp, Walter & Eliza Hall Inst Med Res, Melbourne, Vic 3050, AustraliaPO Royal Melbourne Hosp, Walter & Eliza Hall Inst Med Res, Melbourne, Vic 3050, Australia
Cowman, AF
[1
]
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[1] PO Royal Melbourne Hosp, Walter & Eliza Hall Inst Med Res, Melbourne, Vic 3050, Australia
The genome sequence of Plasmodium falciparum, the causative agent of the most severe form of malaria in humans, rapidly approaches completion, but our ability to genetically manipulate this organism remains limited. Chromosomal integration has only been achieved following the prolonged maintenance of circularised episomal plasmids which selects for single crossover recombinants. It has not been possible to construct genetic deletions via double crossover recombination, presumably due to the low frequency of this event. We have used the Herpes simplex virus thymidine kinase gene and the Escherichia coli cytosine deaminase. gene for negative selection of P. falciparium. Parasites were transformed with plasmids expressing the thymidine kinase and cytosine deaminase genes by positive selection for the human dihydrofolate reductase gene. Parasites expressing thymidine kinase are susceptible to the pro-drug ganciclovir while those expressing cytosine deaminase are sensitive to 5-fluorocytosine. Parental parasites were inherently resistant to these drugs. A significant 'bystander effect' was evident in cultures with either ganciclovir or 5-fluorocytosine. Positive and negative selection of the thymidine kinase transformants with both ganciclovir and WR99210 resulted in the selection of parasites containing a genetic deletion of the Pfrh3 gene, the first targeted double crossover deletions in P. falciparum. The use of negative selection for gene disruptions via double crossover recombination will dramatically improve our ability to analyse protein function and opens the possibility of using this strategy for a variety of gene deletion and modification experiments in the analysis of this important infectious agent. (C) 2002 Australian Society for Parasitology Inc. Published by Elsevier Science Ltd. All rights reserved.
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DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756
BZIK, DJ
LI, WB
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DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756
LI, WB
HORII, T
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DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756
HORII, T
INSELBURG, J
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DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
HIRSCHOWITZ, EA
OHWADA, A
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
OHWADA, A
PASCAL, WR
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
PASCAL, WR
RUSSI, TJ
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
RUSSI, TJ
CRYSTAL, RG
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
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DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756
BZIK, DJ
LI, WB
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DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756
LI, WB
HORII, T
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DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756
HORII, T
INSELBURG, J
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DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756DARTMOUTH COLL,HITCHCOCK MED CTR,DARTMOUTH MED SCH,DEPT MICROBIOL,HANOVER,NH 03756
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
HIRSCHOWITZ, EA
OHWADA, A
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
OHWADA, A
PASCAL, WR
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
PASCAL, WR
RUSSI, TJ
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA
RUSSI, TJ
CRYSTAL, RG
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CORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USACORNELL UNIV, MED CTR, NEW YORK HOSP, DIV INTENSE PULSED NEUTRON SOURCE, NEW YORK, NY 10021 USA