Probing the structure of mouse Ehrlich ascites cell 5.8S, 18S and 28S ribosomal RNA<i>in situ</i>

Holmberg, Lovisa; Melander, Yvette; Nygård, Odd

doi:10.1093/nar/22.8.1374

Cited by 38 publications

(63 citation statements)

References 43 publications

(22 reference statements)

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“…Similar observations were made with mouse 28S rRNA, in which the U's corresponding to the U's involved in apoptotic D8 cleavage (Fig. 7C) were highly accessible to chemical modification (20). In addition, the 3Ј bulge loop that is cleaved in D8 has been found to be prone to RNase T 2 digestion in studies done with in vitro-transcribed human D8b regions (30).…”

Section: Discussionsupporting

confidence: 77%

“…Neither such extracts nor selected added RNases could reproduce the apoptosis-specific cuts in D2, both of which occur in regions recently shown to be inaccessible to chemical modification in the isolated ribosome (18,20). These findings indicate the existence of apoptosisassociated changes of ribosome conformation.…”

mentioning

confidence: 79%

“…The discrete nature of the observed cleavages argues against generally increased RNase activity or random polynucleotide degradation as the explanation for apoptotic rRNA fragmentation. Another argument is that the regions cleaved in the D2 subdomain are known to be inaccessible to chemical modification in the intact ribosome (18,20), suggesting that the ribosome conformation is changed during apoptosis in such a way as to expose these D2c regions to RNase. We believe that 28S rRNA fragmentation is an example of the limited, selective, and controlled macromolecular degradation characteristic of apoptotic cells before secondary necrosis occurs (23,24,36).…”

Section: Discussionmentioning

confidence: 99%

“…In addition, the 3Ј bulge loop that is cleaved in D8 has been found to be prone to RNase T 2 digestion in studies done with in vitro-transcribed human D8b regions (30). Apparently, in the D8b tertiary structure this bulge loop is accessible to RNases (30), and the D8 region itself is exposed on the ribosomal surface (18,20). When the apoptotic D8 cleavage sites are compared, the consensus sequence is GCGGU ê U(U)CCC.…”

Section: Discussionmentioning

confidence: 99%

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Fine Mapping of 28S rRNA Sites Specifically Cleaved in Cells Undergoing Apoptosis

Houge

Robaye

Eikhom

et al. 1995

Molecular and Cellular Biology

115

135

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Bona fide apoptosis in rat and human leukemia cells, rat thymocytes, and bovine endothelial cells was accompanied by limited and specific cleavage of polysome-associated and monosome-associated 28S rRNA, with 18S rRNA being spared. Specific 28S rRNA cleavage was observed in all instances of apoptotic death accompanied by internucleosomal DNA fragmentation, with cleavage of 28S rRNA and of DNA being linked temporally. This indicates that 28S rRNA fragmentation may be as general a feature of apoptosis as internucleosomal DNA fragmentation and that concerted specific cleavage of intra-and extranuclear polynucleotides occurs in apoptosis. Apoptosis-associated cleavage sites were mapped to the 28S rRNA divergent domains D2, D6 (endothelial cells), and D8. The D2 cuts occurred in hairpin loop junctions considered to be buried in the intact ribosome, suggesting that this rRNA region becomes a target for RNase attack in apoptotic cells. D8 was cleaved in two exposed UU(U) sequences in bulge loops. Treatment with agents causing necrotic cell death or aging of cell lysates failed to produce any detectable limited D2 cleavage but did produce a more generalized cleavage in the D8 region. Of potential functional interest was the finding that the primary cuts in D2 exactly flanked a 0.3-kb hypervariable subdomain (D2c), allowing excision of the latter. The implication of hypervariable rRNA domains in apoptosis represents the first association of any functional process with these enigmatic parts of the ribosomes.

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Section: Discussionsupporting

confidence: 77%

mentioning

confidence: 79%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

See 2 more Smart Citations

Fine Mapping of 28S rRNA Sites Specifically Cleaved in Cells Undergoing Apoptosis

Houge

Robaye

Eikhom

et al. 1995

Molecular and Cellular Biology

115

135

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“…Oligo 4 is targeted to a region of the large highly variable expansion sequence D2 (Gerbi, 1996), where insertion of a marker sequence in Tetrahymena is known to be viable (Sweeney et al, 1996). Oligo 5 is targeted to a region in the expansion sequence D12 that is known to be available for chemical modification in mouse ribosomes, indicating that this region may be uncovered near the surface of the ribosome (Holmberg et al, 1994a). Also, an insert at this site is viable in Tetrahymena (Sweeney et al, 1996).…”

Section: Resultsmentioning

confidence: 99%

Diffusion-based Transport of Nascent Ribosomes in the Nucleus

Politz

Tuft

Pederson

2003

MBoC

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Although the complex process of ribosome assembly in the nucleolus is beginning to be understood, little is known about how the ribosomal subunits move from the nucleolus to the nuclear membrane for transport to the cytoplasm. We show here that large ribosomal subunits move out from the nucleolus and into the nucleoplasm in all directions, with no evidence of concentrated movement along directed paths. Mobility was slowed compared with that expected in aqueous solution in a manner consistent with anomalous diffusion. Once nucleoplasmic, the subunits moved in the same random manner and also sometimes visited another nucleolus before leaving the nucleus. INTRODUCTIONIn eukaryotes, rRNA transcription and ribosome assembly take place in the nucleolus. Nascent ribosomes then exit the nucleolus and move into the cytoplasm. Multiple ribosomal proteins assemble with rRNA in the nucleolus and may facilitate proper processing of the pre-rRNA primary transcript (Fatica and Tollervey, 2002). Additionally, a significant number of nonribosomal proteins bind to these formative ribosomes in the nucleolus and also in the nucleoplasm after the nascent ribosomal subunits leave the nucleolus Kuersten et al., 2001;Nissan et al., 2002). The binding of particular proteins in a prescribed order is probably necessary for nucleocytoplasmic transport of the processed ribosomal subunits (e.g., Milkereit et al., 2001). The nuclear export of both the large and small ribosomal subunits has been shown to be dependent, at least indirectly, on the Ran-GTPase cycle and the exportin CRM1, and it is likely that CRM1-mediated export of 60S subunits requires the adaptor protein NMD3 (Moy and Silver, 1999;Ho et al., 2000;Gadal et al., 2001;Thomas and Kutay, 2003;Trotta et al., 2003). In situ hybridization experiments in fission yeast have indicated that rRNA may accumulate along short tracks when near the nuclear pores but nonetheless appears to exit from all the pores, not just those near the nucleolus (Léger-Silvestre et al., 1999). In situ hybridization studies in mammalian cells have primarily addressed the distribution of rRNA within the nucleolus (Huang, 2002) rather than the routes of extranucleolar rRNA traffic, because although high signal representing rRNA is routinely detected in both the nucleolus and the cytoplasm, nucleoplasmic signal which might represent ribosomes moving to the nuclear periphery is not easily detectable by in situ hybridization (PuvionDutilleul et al., 1991;Lazdins et al., 1997; J.C.R. Politz, unpublished observations). Therefore, very little is known about the spatial pattern or mechanism of rRNA movement from the nucleolus into the nucleoplasm and then to the nuclear pores for export (Cullen, 2000;Kuersten et al., 2001;Lei and Silver, 2002), although all three classes of eukaryotic RNAs, rRNA, mRNA, and pol III transcripts have been shown to exit from all the nuclear pores (Dworetzky and Feldherr, 1988;Pante et al., 1997;Mattaj and Englmeier, 1998).In previous studies in live cells (Politz et al., 1998, we investigat...

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Depurination of A4256 in 28 S rRNA by the Ribosome-inactivating Proteins from Barley and Ricin Results in Different Ribosome Conformations

Holmberg

Nygård

1996

Journal of Molecular Biology

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Probing the structure of mouse Ehrlich ascites cell 5.8S, 18S and 28S ribosomal RNAin situ

Cited by 38 publications

References 43 publications

Fine Mapping of 28S rRNA Sites Specifically Cleaved in Cells Undergoing Apoptosis

Fine Mapping of 28S rRNA Sites Specifically Cleaved in Cells Undergoing Apoptosis

Diffusion-based Transport of Nascent Ribosomes in the Nucleus

Depurination of A4256 in 28 S rRNA by the Ribosome-inactivating Proteins from Barley and Ricin Results in Different Ribosome Conformations

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