Cleavage specificity of chloroplast and nuclear tRNA 3'-processing nucleases.

Oommen, Abraham; Li, Xin-Qiang; Gegenheimer, Peter

doi:10.1128/mcb.12.2.865

Cited by 39 publications

(29 citation statements)

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“…9, 39, 44, and 45 and M. Mayer and A.M., unpublished results), mitochondrion (ref. 4 and this work), and chloroplast (36,40,44), all three enzymes possibly encoded by very similar or even a single nuclear gene(s) and routed to the different organelles after translation in the cytoplasm. It will thus be very interesting to identify the respective nuclear gene(s) in plants and to analyze the sorting of each of the encoded proteins.…”

Section: Discussionmentioning

confidence: 67%

“…Because in mammalian and yeast mitochondria, 3Ј processing is also performed in a single-step reaction (5,7,43), these organelles most likely lost their prokaryotic 3Ј processing activity and adapted the nuclear host-derived enzyme. A similar process has probably occurred in chloroplast evolution, because these plant organelles also use a eukaryotic-like 3Ј processing pathway (36,40,44). Plant cells appear to contain similar RNase Z activities in each compartment: nucleus (refs.…”

Section: Discussionmentioning

confidence: 95%

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5′ end maturation and RNA editing have to precede tRNA 3′ processing in plant mitochondria

Kunzmann

Brennicke

Marchfelder

1998

Proc. Natl. Acad. Sci. U.S.A.

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We report the characterization and partial purification of potato mitochondrial RNase Z, an endonuclease that generates mature tRNA 3 ends. The enzyme consists of one (or more) protein(s) without RNA subunits. Products of the processing reaction are tRNA molecules with 3 terminal hydroxyl groups and 3 trailers with 5 terminal phosphates. The main processing sites are located immediately 3 to the discriminator and one nucleotide further downstream. This endonucleolytic processing at and close to the tRNA 3 end in potato mitochondria suggests a higher similarity to the eukaryotic than to the prokaryotic tRNA 3 processing pathway. Partial purification and separation of RNase Z from the 5 processing activity RNase P allowed us to determine biochemical characteristics of the enzyme. The activity is stable over broad pH and temperature ranges, with peak activity at pH 8 and 30°C. Optimal concentrations for MgCl 2 and KCl are 5 mM and 30 mM, respectively. The potato mitochondrial RNase Z accepts only tRNA precursors with mature 5 ends. The precursor for tRNA Phe requires RNA editing for efficient processing by RNase Z.In all genetic systems, mature functional tRNAs are generated by several processing reactions that include the removal of cotranscribed 5Ј and 3Ј extensions. Processing at the tRNA 5Ј end is catalyzed by the ubiquitous endoribonuclease RNase P (1, 2) well characterized in prokaryotes (3). Although the reaction at the tRNA 5Ј end is alike in bacteria, archaeas, and eukaryotes (nuclei and organelles), tRNA 3Ј end maturation seems to be more variable.In Escherichia coli an endonucleolytic cleavage several nucleotides downstream of the tRNA is followed by exonucleolytic removal of some of the residual nucleotides. Only after RNase P has then matured the 5Ј terminus of the tRNA are the remaining extra 3Ј residues removed. This step yields the mature tRNA molecule because the terminal CCA OH sequence is genomically encoded in E. coli (for review, see ref. 4).The majority of nuclear and chloroplast 3Ј processing enzymes have been found to be endonucleases cleaving at the tRNA 3Ј end (5-10), although prokaryotic-like 3Ј maturation with exonucleases being involved has also been observed (11)(12)(13)(14). At present the general consensus appears to attribute a multistep processing pathway to prokaryotes, whereas in eukaryotes single-step reactions predominate.Mitochondria may have retained a prokaryotic-like processing system because they are thought to be of prokaryotic origin according to the endosymbiont theory (15). On the other hand, they may have adapted the host nuclear enzymes for processing, precedence having been found with tRNA modifying enzymes in yeast mitochondria (16) and plant mitochondria (17). To clarify the nature and origin of the plant mitochondrial tRNA processing machinery, the enzymes involved have to be investigated and characterized in detail.A special feature of mitochondrial tRNA maturation in plant cells is the involvement of RNA editing (18)(19)(20)). Herein we demonstrate that...

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Section: Discussionmentioning

confidence: 67%

Section: Discussionmentioning

confidence: 95%

5′ end maturation and RNA editing have to precede tRNA 3′ processing in plant mitochondria

Kunzmann

Brennicke

Marchfelder

1998

Proc. Natl. Acad. Sci. U.S.A.

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“…Endonucleolytic activities that are responsible for eukaryotic tRNA 3Ј processing (3Ј tRNase or RNase Z) have been described in various organisms (Castano et al 1985;Oommen et al 1992;Nashimoto 1997;Kunzmann et al 1998;Levinger et al 1998). Recently, such activities were purified and cloned from plant and archaea, and are shown to be members of the ELAC1/2 family of proteins (Schiffer et al 2002).…”

Section: Introductionmentioning

confidence: 99%

Co-evolution of tRNA 3′ trailer sequences with 3′ processing enzymes in bacteria

Gong²,

Joshi³

et al. 2005

RNA

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Maturation of the tRNA 3 terminus is a complicated process in bacteria. Usually, it is initiated by an endonucleolytic cleavage carried out by RNase E and Z in different bacteria. In Escherichia coli, RNase E cleaves AU-rich sequences downstream of tRNA, producing processing intermediates with a few extra residues at the 3 end; these are then removed by exoribonuclease trimming to generate the mature 3 end. Here we show that essentially all E. coli tRNA precursors contain a potential RNase E cleavage site, the AU-rich sequence element (AUE), in the 3 trailer. This suggests that RNase E cleavage and exonucleolytic trimming is a general pathway for tRNA maturation in this organism. Remarkably, the AUE immediately downstream of each tRNA is selectively conserved in bacteria having RNase E and tRNA-specific exoribonucleases, suggesting that this pathway for tRNA processing is also commonly used in these bacteria. Two types of RNase E-like proteins are identified in actinobacteria and the ␣-subdivision of proteobacteria. The tRNA 3 proximal AUE is conserved in bacteria with only one type of E-like protein.Selective conservation of the AUE is usually not observed in bacteria without RNase E. These results demonstrate a novel example of co-evolution of RNA sequences with processing activities.

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“…However, CCA-less precursors in Bacillus subtilis are processed endonucleolytically by tRNase Z (Pellegrini et al 2003;Wen et al 2005). Conversely, the major pathway for eukaryotic tRNA 3 ′ -end processing is endonucleolytic, while trimming by exonucleases serves as an alternative (Garber and Gage 1979;Hagenbuchle et al 1979;Castaño et al 1985;Engelke et al 1985;Frendewey et al 1985;Manam and Van Tuyle 1987;Stange and Beier 1987;Furter et al 1992;Oommen et al 1992;Papadimitriou and Gross 1996;Han and Kang 1997;Nashimoto 1997;Mayer et al 2000;Schiffer et al 2002).…”

Section: Introductionmentioning

confidence: 99%

tRNA 3′ processing in yeast involves tRNase Z, Rex1, and Rrp6

Skowronek

Grzechnik

Späth

et al. 2013

RNA

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Mature tRNA 3 ′ ends in the yeast Saccharomyces cerevisiae are generated by two pathways: endonucleolytic and exonucleolytic. Although two exonucleases, Rex1 and Rrp6, have been shown to be responsible for the exonucleolytic trimming, the identity of the endonuclease has been inferred from other systems but not confirmed in vivo. Here, we show that the yeast tRNA 3 ′ endonuclease tRNase Z, Trz1, is catalyzing endonucleolytic tRNA 3 ′ processing. The majority of analyzed tRNAs utilize both pathways, with a preference for the endonucleolytic one. However, 3′ -end processing of precursors with long 3 ′ trailers depends to a greater extent on Trz1. In addition to its function in the nucleus, Trz1 processes the 3 ′ ends of mitochondrial tRNAs, contributing to the general RNA metabolism in this organelle.

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Cleavage specificity of chloroplast and nuclear tRNA 3'-processing nucleases.

Cited by 39 publications

References 45 publications

5′ end maturation and RNA editing have to precede tRNA 3′ processing in plant mitochondria

5′ end maturation and RNA editing have to precede tRNA 3′ processing in plant mitochondria

Co-evolution of tRNA 3′ trailer sequences with 3′ processing enzymes in bacteria

tRNA 3′ processing in yeast involves tRNase Z, Rex1, and Rrp6

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