Characterization of a <i>Drosophila</i> Proximal‐Sequence‐Element‐Binding Protein Involved in Transcription of Small Nuclear RNA Genes

Su, Yan; Song, Yuru; Wang, Yan; Jessop, Lea; Zhan, Lichun; Stumph, William E.

doi:10.1111/j.1432-1033.1997.t01-1-00231.x

Cited by 26 publications

(45 citation statements)

References 30 publications

(57 reference statements)

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“…Because each of these subunits is required for snRNA transcription by either RNAP II or RNAP III, it seems that the same protein complex functions at both classes of vertebrate snRNA gene promoters. The fact that the PSEA plays a major role in determining RNA polymerase specificity in Drosophila poses the question of whether a similar complex functions at both RNAP II and RNAP III snRNA promoters in insects.Our lab recently reported the partial purification and characterization of the D. melanogaster PSEA-binding protein (DmPBP) (27). Like SNAP c /PTF, DmPBP is a multisubunit…”

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confidence: 99%

Identification and Topological Arrangement of Drosophila Proximal Sequence Element (PSE)-Binding Protein Subunits That Contact the PSEs of U1 and U6 Small Nuclear RNA Genes

Wang

Stumph

1998

Molecular and Cellular Biology

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Most small nuclear RNAs (snRNAs) are synthesized by RNA polymerase II, but U6 and a few others are synthesized by RNA polymerase III. Transcription of snRNA genes by either polymerase is dependent on a proximal sequence element (PSE) located upstream of position ؊40 relative to the transcription start site. In contrast to findings in vertebrates, sea urchins, and plants, the RNA polymerase specificity of Drosophila snRNA genes is intrinsically encoded in the PSE sequence itself. We have investigated the differential interaction of the Drosophila melanogaster PSE-binding protein (DmPBP) with U1 and U6 gene PSEs. By using a site specific protein-DNA photo-cross-linking assay, we identified three polypeptide subunits of DmPBP with apparent molecular masses of 95, 49, and 45 kDa that are in close proximity to the DNA and two additional putative polypeptides of 230 and 52 kDa that may be integral to the complex. The 95-kDa subunit cross-linked at positions spanning the entire length of the PSE, but the 49-and 45-kDa subunits cross-linked only to the 3 half of the PSE. The same polypeptides cross-linked to both the U1 and U6 PSE sequences. However, there were significant differences in the cross-linking patterns of these subunits at a subset of the phosphate positions, depending on whether binding was to a U1 or U6 gene PSE. These data suggest that RNA polymerase specificity is associated with distinct modes of interaction of DmPBP with the DNA at U1 and U6 promoters.In higher eukaryotes, four of the major small nuclear RNAs (snRNAs) found in spliceosomes (U1, U2, U4, and U5) are synthesized by RNA polymerase II (RNAP II), but U6 snRNA is synthesized by RNA polymerase III (RNAP III) (2,3,9,18,22). The U6 gene promoter is representative of an unusual class of RNAP III promoters that contain a TATA box but lack internal promoter elements (5,15,19,30). Promoters of snRNA genes transcribed by either RNAP II or RNAP III contain an essential proximal sequence element (PSE) at a conserved location approximately 40 to 65 bp upstream of the transcription start site that is required for the initiation of snRNA transcription (4,9,18,26,29,30,32,36).In Drosophila melanogaster, the PSE is more specifically named the PSEA to distinguish it from a second, even more proximal conserved element, PSEB, present in the promoters of Drosophila snRNA genes transcribed by RNAP II (36). The PSEB is located at the TATA box position but is a poor TATA box sequence (consensus CATGGAg/aA) (16). PSEB is separated from the upstream PSEA by 8 bp of nonconserved sequence (16,36). Drosophila U6 genes, on the other hand, contain a canonical TATA box rather than a PSEB, and the TATA box is separated by 12 bp from the upstream PSEA (4).In vertebrates and sea urchins, the PSEs of U1 and U2 genes are interchangeable with the PSEs of U6 genes (14,17,23). In these organisms, the PSEs are therefore not responsible for the determination of RNAP specificity. Surprisingly, recent results from our lab revealed that the U1 and U6 PSEAs are not interchangeable in t...

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confidence: 99%

Identification and Topological Arrangement of Drosophila Proximal Sequence Element (PSE)-Binding Protein Subunits That Contact the PSEs of U1 and U6 Small Nuclear RNA Genes

Wang

Stumph

1998

Molecular and Cellular Biology

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“…Previous work had shown that D. melanogaster U1 and U6 snRNA genes can be faithfully transcribed in vitro by using unfractionated SNF prepared from 0 -12-h fruit fly embryos (22)(23)(24)(25). As a control for TRF1-dependent transcription, we also employed a tRNA Arg -maxi gene template (20).…”

Section: Resultsmentioning

confidence: 99%

“…As controls, three U1 snRNA gene loci and three tRNA gene loci were also analyzed. Furthermore, because DmSNAPc is required for transcription of both U1 and U6 snRNA genes (23) but not for the transcription of tRNA genes, we also examined DmSNAPc occupancy by using antibodies against DmSNAP43.…”

Section: Resultsmentioning

confidence: 99%

“…The preparation of the antibodies against D. melanogaster TBP and DmSNAP43 has been described previously (21 In Vitro Transcription Assays-The templates that contained the wild type U1 and U6 promoters have been described previously (22,23). The plasmid pArg-maxi contained a tRNA Arg gene with a 12-bp insertion between the internal promoter elements (19) and was obtained from Deborah Johnson (Department of Molecular Pharmacology and Biochemistry, University of Southern California).…”

Section: Methodsmentioning

confidence: 99%

“…Procedures for in vitro transcription and analysis of the RNA products by primer extension have been previously described in detail (22,23). Transcription reactions (25 l final volume) utilized 15 l of a soluble nuclear fraction (SNF) prepared from D. melanogaster embryos (22,24,25).…”

Section: Methodsmentioning

confidence: 99%

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Differential Utilization of TATA Box-binding Protein (TBP) and TBP-related Factor 1 (TRF1) at Different Classes of RNA Polymerase III Promoters

Verma

Hung

Kang

et al. 2013

Journal of Biological Chemistry

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Background: TATA box-binding protein-related factor 1 (TRF1) was believed to be required for all RNA polymerase III transcription in Drosophila. Results: Chromatin immunoprecipitations and transcription assays indicate TATA box-binding protein (TBP) is utilized at U6 snRNA promoters. Conclusion: Although TRF1 is required for tRNA transcription, TBP is used for U6 transcription. Significance: Different classes of RNA polymerase III promoters differentially utilize TBP and TRF1.

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Transcriptional regulation of snRNAs and its significance for plant development

Ohtani

2016

J Plant Res

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Small nuclear RNA (snRNA) represents a distinct class of non-coding RNA molecules. As these molecules have fundamental roles in RNA metabolism, including pre-mRNA splicing and ribosomal RNA processing, it is essential that their transcription be tightly regulated in eukaryotic cells. The genome of each organism contains hundreds of snRNA genes. Although the structures of these genes are highly diverse among organisms, the trans-acting factors that regulate snRNA transcription are evolutionarily conserved. Recent studies of the Arabidopsis thaliana srd2-1 mutant, which is defective in the snRNA transcription factor, provide insight into the physiological significance of snRNA regulation in plant development. Here, I review the current understanding of the molecular mechanisms underlying snRNA transcription.

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Characterization of a Drosophila Proximal‐Sequence‐Element‐Binding Protein Involved in Transcription of Small Nuclear RNA Genes

Cited by 26 publications

References 30 publications

Identification and Topological Arrangement of Drosophila Proximal Sequence Element (PSE)-Binding Protein Subunits That Contact the PSEs of U1 and U6 Small Nuclear RNA Genes

Identification and Topological Arrangement of Drosophila Proximal Sequence Element (PSE)-Binding Protein Subunits That Contact the PSEs of U1 and U6 Small Nuclear RNA Genes

Differential Utilization of TATA Box-binding Protein (TBP) and TBP-related Factor 1 (TRF1) at Different Classes of RNA Polymerase III Promoters

Transcriptional regulation of snRNAs and its significance for plant development

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