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The Pentatricopeptide Repeat Protein OTP87 Is Essential for RNA Editing of nad7 and atp1 Transcripts in Arabidopsis Mitochondria Kamel Hammani‡§, Catherine.

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Presentation on theme: "The Pentatricopeptide Repeat Protein OTP87 Is Essential for RNA Editing of nad7 and atp1 Transcripts in Arabidopsis Mitochondria Kamel Hammani‡§, Catherine."— Presentation transcript:

1 The Pentatricopeptide Repeat Protein OTP87 Is Essential for RNA Editing of nad7 and atp1 Transcripts in Arabidopsis Mitochondria Kamel Hammani‡§, Catherine Colas des Francs-Small‡, Mizuki Takenaka¶, Sandra K. Tanz‡, Kenji Okuda ‖, Toshiharu Shikanai ‖, Axel Brennicke¶ and Ian Small‡ From the: ‡ Australian Research Council Centre of Excellence in Plant Energy Biology, University of Western Australia, Crawley 6009 Western Australia, Australia, ; § Institut de Biologie Moléculaire des Plantes du CNRS, Université de Strasbourg, 12 rue du Général Zimmer, 67084 Strasbourg Cedex, France, ; ¶ Molekulare Botanik, Universität Ulm, 89069 Ulm, Germany, and ; ‖ Department of Botany, Graduate School of Science, Kyoto University, Kyoto 606-8502, Japan Ian Small, U. of Western Australia

2 Background: Arabidopsis and PPR proteins Arabidopsis thaliana – most favored model for plant biology because of its genetics  A small dicot in the mustard family  Short life cycle (seed-to-seed in 6 wks)  Well-developed genetics  Smallest genome of angiosperms (low in repetitive DNA)  Genome has been completely sequenced (transcriptomics and proteomics also well developed) Elliot Meyerowitz, Calif. Institute of Technology

3 Pentatricopeptide Repeat (PPR) Proteins Contain tandem arrays of pentatricopeptide repeats (PPRs) Found in many eukaryotes, but so many more in angiosperms!  e.g., > 400 in Arabidopsis Most are targeted to organelles (M & C) There are several subgroups Based on those whose functions are known, they mediate aspects of RNA processing, especially RNA editing. From Lurin et al. 2004

4 Molecular characterization and phenotypic analysis of the Arabidopsis otp87 mutant. Has a T-DNA insertion that knock-outs the PPR protein, OTP87. Mutant can be complemented with wild-type OTP87 gene.

5 C. RFP fused to the presequence of cytochrome oxidase IV (mito. marker) D. RFP fused to the rbcS protein (plastid marker) A,B. Amino acids 1-100 of OTP87 fused to GFP. OTP87 is Dual- targeted to Mitochondria and Chloroplasts

6 Chloroplasts appear normal in the otp87 null mutant.

7 Two editing sites in mitochondria are affected in the OTP87 KO mutant; 1 each in the atp1 and nad7 mRNAs. Only the former changes an amino acid, however. ©2011 by American Society for Biochemistry and Molecular Biology

8 ATP synthase complex assembly is defective in the otp87 KO.

9 Pollen structure of WT and otp87 plants is normal. Hammani K et al. J. Biol. Chem. 2011;286:21361-21371 ©2011 by American Society for Biochemistry and Molecular Biology

10 Homology between the cis-elements surrounding the two affected editing sites (nad7-C24 and atp1-C1178). Hammani K et al. J. Biol. Chem. 2011;286:21361-21371 ©2011 by American Society for Biochemistry and Molecular Biology

11 Electrophoretic mobility shift assays using recombinant OTP87 protein. Conclusion: OTP87 binds specifically to small RNAs with the editing sites for nad7 and atp1.

12 Conclusions Arabidopsis OTP87 is dual-targeted to chloroplasts and mitochondria, but may function only in the latter. OTP87 is required for 2 editing sites in the mitochondria, one each in nad7 and atp1. The loss of atp1 editing leaves a non-conserved amino acid, which appears to inhibit stable assembly of the atp synthase complex. This could account for the phenotype of the OTP87 insertional mutant. Recombinant OTP87 binds to the 2 editing sites specifically, in an in vitro shift assay. OTP87 may recruit the editing enzyme to those sites.

13 Assessing Strengths & Weaknesses of a Paper Usually consider the following:  Originality (specifically discussed at end of Introduction & beginning of Discussion sections)  Significance (discussed in Abstract and Discussion sections)  Quality of data?  Are conclusions supported by the data?  Is the paper clear and well written? Methods well described? Is the data presentation clear? How could the paper be improved?

14 Strengths and weaknesses Strengths  Novelty: new protein, and a rare KO mutant in a PPR protein that gives a clear phenotype  Significance: the first protein from Arabidopsis shown to bind to 2 different editing sites in vitro. Will enable further biochemical studies of how it binds RNA, specifically.  Quality of the data was generally high, and supported the conclusions. Weaknesses  Some of the writing, e.g. the figure legends, was not very clear even if the reader was an expert.  Work still provided no clues about what the editing enzyme(s) are.


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