Genetic interference in Trypanosoma brucei by heritable and inducible double-stranded RNA

Shi, Huafang; Djikeng, Appolinaire; Mark, Tomer M.; Wirtz, Elizabeth; Tschudi, Christian; Ullu, Elisabetta

doi:10.1017/s1355838200000297

Cited by 176 publications

(136 citation statements)

References 21 publications

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“…In Vivo Depletion of IF2 by RNAi-Due to the availability of a tightly controlled tetracycline-inducible expression system (29), RNAi has become the method of choice to disrupt gene function in T. brucei (22,23). Thus, to investigate the function of IF2 by RNAi, we prepared a construct that contained a defined sequence of the IF2 gene in the sense, as well as the antisense, direction.…”

Section: Resultsmentioning

confidence: 99%

“…In the presence of tetracycline, the RNA was expressed and formed a stem loop that eventually led to the specific degradation of the IF2 mRNA. There have been two types of stuffer sequences used in stem loop constructs, one of trypanosomal origin as described previously (22) and another one of mouse origin (23). Surprisingly, it was shown that the efficiency of RNAi was generally higher when the mouse sequence was used.…”

Section: Resultsmentioning

confidence: 99%

“…Two versions of the plasmid were prepared. In the first one (TbIF2-Tb), the sense and antisense sequences were separated by a fragment corresponding to 690 nucleotides of the trypanosomal spliced leader sequence (22), whereas in the second one (TbIF2-Mm), a 439-bp fragment, corresponding to positions 341-779 of the mouse Pex11b mRNA, was used as a spacer (23). Using the mouse sequence as a spacer yielded a more efficient down-regulation of the targeted mRNA than if the T. brucei sequence was used.…”

Section: Methodsmentioning

confidence: 99%

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Mitochondrial Initiation Factor 2 of Trypanosoma brucei Binds Imported Formylated Elongator-type tRNAMet

Charrière

Tan

Schneider

2005

Journal of Biological Chemistry

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The mitochondrion of Trypanosoma brucei lacks tRNA genes. Its translation system therefore depends on the import of nucleus-encoded tRNAs. Thus, except for the cytosol-specific initiator tRNA Met , all trypanosomal tRNAs function in both the cytosol and the mitochondrion. The only tRNA Met present in T. brucei mitochondria is therefore the one which, in the cytosol, is involved in translation elongation. Mitochondrial translation initiation depends on an initiator tRNA Met carrying a formylated methionine. This tRNA is then recognized by initiation factor 2, which brings it to the ribosome. To guarantee mitochondrial translation initiation, T. brucei has an unusual methionyl-tRNA formyltransferase that formylates elongator tRNA Met . In the present study, we have identified initiation factor 2 of T. brucei and shown that its carboxyl-terminal domain specifically binds formylated trypanosomal elongator tRNA Met . Furthermore, the protein also recognizes the structurally very different Escherichia coli initiator tRNA Met , suggesting that the main determinant recognized is the formylated methionine. In vivo studies using stable RNA interference cell lines showed that knockdown of initiation factor 2, depending on which construct was used, causes slow growth or even growth arrest. Moreover, concomitantly with ablation of the protein, a loss of oxidative phosphorylation was observed. Finally, although ablation of the methionyltRNA formyltransferase on its own did not impair growth, a complete growth arrest was observed when it was combined with the initiation factor 2 RNA interference cell line showing the slow growth phenotype. Thus, these experiments illustrate the importance of mitochondrial translation initiation for growth of procyclic T. brucei.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Mitochondrial Initiation Factor 2 of Trypanosoma brucei Binds Imported Formylated Elongator-type tRNAMet

Charrière

Tan

Schneider

2005

Journal of Biological Chemistry

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“…The expression of Lsm proteins was silenced by the two approaches. The Lsm8 was silenced by producing dsRNA in the form of a stem-loop structure, as described under "Experimental Procedures" (35,37). For silencing the Lsm3 gene, PCR was used to amplify the gene that was cloned into the pZJM vector carrying the two T7 opposing promoters (35).…”

Section: Fig 4 the Level Of Sl Rna And The Y-structure Intermediatementioning

confidence: 99%

Identification and Functional Characterization of Lsm Proteins in Trypanosoma brucei

Liu¹,

Liang²,

Uliel

et al. 2004

Journal of Biological Chemistry

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RNA interference of Sm proteins inTrypanosoma brucei demonstrated that the stability of the small nuclear RNAs (U1, U2, U4, U5) and the spliced leader RNA, but not U6 RNA, were affected upon Sm depletion (Mandelboim, M., Barth, S., Biton, M., Liang, X. H., and Michaeli, S. (2003) J. Biol. Chem. 278, 51469-51478), suggesting that Lsm proteins that bind and stabilize U6 RNA in other eukaryotes should exist in trypanosomes. In this study, we identified seven Lsm proteins (Lsm2p to Lsm8p) and examined the function of Lsm3p and Lsm8p by RNA interference silencing. Both Lsm proteins were found to be essential for U6 stability and mRNA decay. Silencing was lethal, and cisand trans-splicing were inhibited. Importantly, silencing also affected the level of U4.U6 and the U4.U6/U5 tri-small nuclear ribonucleoprotein complexes. The presence of Lsm proteins in trypanosomes that diverged early in the eukaryotic lineage suggests that these proteins are highly conserved in both structure and function among eukaryotes. Interestingly, however, Lsm1p that is specific to the mRNA decay complex was not identified in the genome data base of any kinetoplastidae, and the Lsm8p that in other eukaryotes exclusively functions in U6 stability was found to function in trypanosomes also in mRNA decay. These data therefore suggest that in trypanosomes only a single Lsm complex may exist.

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“…Regulatable TbMP48 sequences to produce interfering dsRNAi were introduced into both the bloodstream and procyclic stage cell lines, as described (Shi et al 2000;Wang et al 2000). We were unable to produce null mutants of TbMP52 and thus produced mutant BFs in which we introduced a regulatable TbMP52 allele and then deleted both endogenous alleles in BFs as described by Wirtz et al (1999).…”

Section: Functions Of Editing Complex Componentsmentioning

confidence: 99%

Composition of the editing complex ofTrypanosoma brucei

Stuart

Panigrahi

Schnaufer

et al. 2002

Phil. Trans. R. Soc. Lond. B

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The RNA editing that produces most functional mRNAs in trypanosomes is catalysed by a multiprotein complex. This complex catalyses the endoribonucleolytic cleavage, uridylate addition and removal, and RNA ligation steps of the editing process. Enzymatic and in vitro editing analyses reveal that each catalytic step contributes to the speci city of the editing and, together with the interaction between gRNA and the mRNA, results in precisely edited mRNAs. Tandem mass spectrometric analysis was used to identify the genes for several components of biochemically puri ed editing complexes. Their identity and presence in the editing complex were con rmed using immunochemical analyses utilizing mAbs speci c to the editing complex components. The genes for two RNA ligases were identi ed. Genetic studies show that some, but not all, of the components of the complex are essential for editing. The TbMP52 RNA ligase is essential for editing while the TbMP48 RNA ligase is not. Editing was found to be essential in bloodstream form trypanosomes. This is surprising because mutants devoid of genes encoding RNAs that become edited survive as bloodstream forms but encouraging since editing complex components may be targets for chemotherapy.

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Genetic interference in Trypanosoma brucei by heritable and inducible double-stranded RNA

Cited by 176 publications

References 21 publications

Mitochondrial Initiation Factor 2 of Trypanosoma brucei Binds Imported Formylated Elongator-type tRNAMet

Mitochondrial Initiation Factor 2 of Trypanosoma brucei Binds Imported Formylated Elongator-type tRNAMet

Identification and Functional Characterization of Lsm Proteins in Trypanosoma brucei

Composition of the editing complex ofTrypanosoma brucei

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