Dynamic association and localization of human H/ACA RNP proteins

Kittur, Nupur; Darzacq, Xavier; Roy, Suheeta; Singer, Robert H.; Meier, U. Thomas

doi:10.1261/rna.249306

Cited by 28 publications

(24 citation statements)

References 41 publications

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“…Together, the structures of the U65hp/S14 complex and the archaeal H/ACA RNP illustrate how this could occur. The H/ACA RNA is believed to remain stably associated with the snoRNP for multiple rounds of pseudouridylation (24), although a very recent study indicates that only Cbf5 is irreversibly associated with the H/ACA RNA (41).…”

Section: Discussionmentioning

confidence: 99%

H/ACA small nucleolar RNA pseudouridylation pockets bind substrate RNA to form three-way junctions that position the target U for modification

Feigon

2007

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

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), the authors note that in Fig. 1A, the sequence of the 5Ј side of the 5Ј pseudouridylation pocket of the U65 H/ACA snoRNA, as well as a portion of the lower stem of the 3Ј hairpin, were drawn incorrectly. Additionally, in the Fig. 1 legend and elsewhere in the text, the numbering of the substrate RNA, which was based on Bortolin et al. [Bortolin M-L, Ganot P, Kiss T (1999) EMBO J 18:457-469], differs by one nucleotide from that found in the genomic sequence (refer to the snoRNA database, snoRNA-LMBE-db, at www-snorna.biotoul.fr). The correct numbers for the pseudouridylation sites are 4427 and 4373 for the 5Ј and 3Ј pseudouridylation pockets, respectively. The corrected figure and legend appear below. These errors do not affect the conclusions of the article. (U65hp), the substrate rRNA (S14), and the U65hp/S14 complex. S14 contains the sequence of human 28S rRNA (4422-4434), including U4427 (underlined), which is targeted for pseudouridylation, and an extra U (lowercase) at the 5Ј end.

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Section: Discussionmentioning

confidence: 99%

H/ACA small nucleolar RNA pseudouridylation pockets bind substrate RNA to form three-way junctions that position the target U for modification

Feigon

2007

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

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“…Therefore, it may depend on those of other proteins, such as the multiple nuclear localization signals of NAP57 (Meier and Blobel 1994;Heiss et al 1999;Youssoufian et al 1999). Third, SHQ1 has to act before cotranscriptional association of NAP57 with H/ACA RNA and other core proteins because SHQ1 only binds NAP57 alone and because, once assembled with the core trimer, H/ACA RNAs will no longer exchange (Wang and Meier 2004;Kittur et al 2006). Therefore, SHQ1 may function as a NAP57 chaperone and/or licensing factor marking it ready for RNP assembly.…”

Section: Discussionmentioning

confidence: 99%

“…siRNAs were as previously described ) except for siSHQ1, which was a combination of siSHQ1.1, GCU ACGAAAAUUUGUCAAUTT; siSHQ1.2, GGAAGUAGUUGACG AUGAATT; and siSHQ1.3, GGACAGCAAAACCACUUGUTT (Ambion). Cells were maintained, treated, and transfected as we previously described Kittur et al 2006). Similarly, the inducible H/ACA RNA cell line and related analyses ) and the cell line containing integrated Lac operator arrays (Janicki et al 2004) have been described.…”

Section: Dna/rna Constructs Transfections and Translationsmentioning

confidence: 99%

SHQ1 is required prior to NAF1 for assembly of H/ACA small nucleolar and telomerase RNPs

Grozdanov

Roy

Kittur

et al. 2009

RNA

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128

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Assembly of H/ACA RNPs in yeast is aided by at least two accessory factors, Naf1p and Shq1p. Although the function of Naf1p and its human ortholog NAF1 has been delineated in detail, that of Shq1p and its putative human ortholog SHQ1 remains obscure. We demonstrate that SHQ1 indeed functions in the biogenesis of human H/ACA RNPs and we dissect its mechanism of action. Like NAF1, SHQ1 binds the major H/ACA core protein and pseudouridine synthase NAP57 (aka dyskerin) but precedes the assembly role of NAF1 at nascent H/ACA RNAs because the interaction of SHQ1 with NAP57 in vivo and in vitro precludes that of NAF1 and of the other H/ACA core proteins that are present at the sites of H/ACA RNA transcription. The N-terminal heat shock protein 20-like CS domain of SHQ1 is dispensable for NAP57 binding. Consistent with its role as an assembly factor, SHQ1 localizes to the nucleoplasm and is excluded from nucleoli and Cajal bodies, the sites of mature H/ACA RNPs. In an in vitro assembly system of functional H/ACA RNPs that is dependent on NAF1, excess recombinant SHQ1 interferes with assembly. Importantly, knockdown of cellular SHQ1 prevents accumulation of a newly synthesized H/ACA reporter RNA and generally reduces the levels of endogenous H/ACA RNAs including telomerase RNA. In summary, the sequential action of SHQ1 and NAF1 is required for functional assembly of H/ACA RNPs in vivo and in vitro. This step-wise process could serve as an efficient means of quality control during H/ACA RNP assembly.

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“…It has recently been shown that overexpressed human Naf1 delocalises to the cytoplasm. 42 This might be due to a concentration effect, shifting the equilibrium between monomeric and dimeric forms of human Naf1. Naf1 most likely assembles along with Cbf5, Nop10 and Nhp2, early during H/ACA snoRNA transcription.…”

Section: Discussionmentioning

confidence: 99%

The Box H/ACA RNP Assembly Factor Naf1p Contains a Domain Homologous to Gar1p Mediating its Interaction with Cbf5p

Leulliot

Godin

Hoareau-Aveilla

et al. 2007

Journal of Molecular Biology

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Dynamic association and localization of human H/ACA RNP proteins

Cited by 28 publications

References 41 publications

H/ACA small nucleolar RNA pseudouridylation pockets bind substrate RNA to form three-way junctions that position the target U for modification

H/ACA small nucleolar RNA pseudouridylation pockets bind substrate RNA to form three-way junctions that position the target U for modification

SHQ1 is required prior to NAF1 for assembly of H/ACA small nucleolar and telomerase RNPs

The Box H/ACA RNP Assembly Factor Naf1p Contains a Domain Homologous to Gar1p Mediating its Interaction with Cbf5p

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