The mouse ribosomal gene terminator consists of three functionally separable sequence elements.

Kuhn, Anne; Normann, Andrea; Bartsch, Ingrid; Grummt, Ingrid

doi:10.1002/j.1460-2075.1988.tb02968.x

Cited by 54 publications

(32 citation statements)

References 39 publications

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“…Nsi1 terminated RNA polymerase I transcription, whereas neither Pol II nor Pol III transcription termination was comparably affected in the employed in vitro assay. These results resemble those obtained in experiments investigating mammalian RNA polymerase I transcription termination by the transcription termination factor TTF1 (12,38,46). Hence, at least in such an artificial in vitro system, a specific molecular interplay between Pol I and Nsi1 is required to promote transcription termination.…”

Section: Discussionsupporting

confidence: 81%

“…In mouse, binding of the transcription termination factor TTF1 to a conserved 18-bp DNA element was shown to be sufficient to stop Pol I transcription in vitro (10)(11)(12) and to release the transcripts with the help of Pol I transcript release factor (PTRF) (13,14). The same DNA cis element was able to terminate transcription in vivo (12). Adjacent DNA elements could modulate termination efficiency.…”

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confidence: 99%

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Binding of the Termination Factor Nsi1 to Its Cognate DNA Site Is Sufficient To Terminate RNA Polymerase I Transcription In Vitro and To Induce Termination In Vivo

Merkl

Pérez-Fernández

Pilsl

et al. 2014

Molecular and Cellular Biology

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Different models have been proposed explaining how eukaryotic gene transcription is terminated. Recently, Nsi1, a factor involved in silencing of ribosomal DNA (rDNA), was shown to be required for efficient termination of rDNA transcription by RNA polymerase I (Pol I) in the yeast Saccharomyces cerevisiae. Nsi1 contains Myb-like DNA binding domains and associates in vivo near the 3= end of rRNA genes to rDNA, but information about which and how DNA sequences might influence Nsi1-dependent termination is lacking. Here, we show that binding of Nsi1 to a stretch of 11 nucleotides in the correct orientation was sufficient to pause elongating Pol I shortly upstream of the Nsi1 binding site and to release the transcripts in vitro. The same minimal DNA element triggered Nsi1-dependent termination of pre-rRNA synthesis using an in vivo reporter assay. Termination efficiency in the in vivo system could be enhanced by inclusion of specific DNA sequences downstream of the Nsi1 binding site. These data and the finding that Nsi1 blocks efficiently only Pol I-dependent RNA synthesis in an in vitro transcription system improve our understanding of a unique mechanism of transcription termination. C ellular multisubunit RNA polymerases of all three domains of life share common structural and functional features. After initiation of transcription at their cognate gene promoters, they extend the transcripts until they reach specific DNA cis elements, at which transcription is terminated. Termination occurs when the contacts of the RNA-DNA hybrid within the elongating RNA polymerase are destabilized. Termination finally results in the stopping of RNA synthesis, release of the transcript, and dissociation of the RNA polymerase from the DNA template (reviewed in reference 1). A first step in the termination pathway can be the pausing of the elongating polymerase, which is then followed by the disruption of the elongation complex.Dissociation of the ternary elongation complex formed by RNA polymerase, RNA, and DNA can be caused either by auxiliary protein factors or solely by interactions of DNA and RNA with the transcribing RNA polymerase. Both principles, factordependent and intrinsic termination, have been described for bacterial transcription termination (reviewed in reference 1). In the case of eukaryotic RNA polymerase II (Pol II), either 3=-end processing factors of the mRNA or the yeast RNA-DNA helicase Sen1 (human senataxin) was suggested to disrupt the ternary complex (reviewed in references 2 and 3). This might resemble Rho-dependent termination in bacteria in which the ATP-dependent RNA-DNA helicase Rho destabilizes the elongation complex (4, 5; for a review, see reference 1). RNA polymerase III (Pol III) termination resembles the other bacteria-like termination mechanism, the intrinsic termination, in which the RNA-DNA hybrid is destabilized by a stem-loop in the nascent RNA (6, 7) (8).In contrast to these mechanisms of transcription termination, Pol I requires a termination factor which binds to a specific DNA sequence t...

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Section: Discussionsupporting

confidence: 81%

mentioning

confidence: 99%

Binding of the Termination Factor Nsi1 to Its Cognate DNA Site Is Sufficient To Terminate RNA Polymerase I Transcription In Vitro and To Induce Termination In Vivo

Merkl

Pérez-Fernández

Pilsl

et al. 2014

Molecular and Cellular Biology

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“…Ninety percent of yeast RNAPI terminates at the first terminator (T1), situated upstream of a pause-inducing factor-binding site that is recognized in vitro by Reb1 (Ju et al 1990;Lang and Reeder 1995). In mammals, the major terminator, called the Sal box (Grummt et al 1985;Kuhn et al 1988), is recognized by TTF-I (transcription termination factor for polI) , and like the Reb1-binding site, it must be correctly oriented to cause termination (Grummt et al 1985;Lang and Reeder 1993). The mouse Sal box is an 18-bp element repeated 10 times in the IGS, while humans contain a shorter Sal box (11 bp) that is recognized by the human TTF-I (Bartsch et al 1987;Pfleiderer et al 1990;.…”

Section: Rnapi Terminationmentioning

confidence: 99%

Transcription termination by nuclear RNA polymerases

Richard

Manley²

2009

Genes Dev.

291

326

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Gene transcription in the cell nucleus is a complex and highly regulated process. Transcription in eukaryotes requires three distinct RNA polymerases, each of which employs its own mechanisms for initiation, elongation, and termination. Termination mechanisms vary considerably, ranging from relatively simple to exceptionally complex. In this review, we describe the present state of knowledge on how each of the three RNA polymerases terminates and how mechanisms are conserved, or vary, from yeast to human.

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“…Eucaryotic RNA polymerase I termination (27), although factor dependent, bears little resemblance to p-dependent termination in E. coli but instead resembles aspects of the protein blockage mechanism described by Sellitti et al (50). For polymerase I terminators, it is the DNA to which the factor binds (27), and the signal follows, rather than precedes, the site of termination (27,28).RNA polymerase II appears to incorporate elements of all the above termination mechanisms in its repertoire of strategies. Transcription of the human gastrin gene appears to terminate upstream of the termination signal as for RNA polymerase I (3, 49).…”

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confidence: 99%

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confidence: 99%

Transcription termination at the chicken beta H-globin gene.

Pribýl

Martinson

1988

Mol. Cell. Biol.

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We characterized the transcription termination region of the chicken 3H.-globin gene. First we located the region by nuclear runon transcription in vitro. Then we sequenced and subcloned it into a chloramphenicol acetyltransferase (CAT) expression vector for assay in vivo. The region of PH termination contains two interesting elements located about 1 kilobase downstream of the pH gene poly(A) site. Either element alone can block CAT expression if inserted between the promoter and the poly(A) site of the cat gene in pRSVcat. The first element in the termination region is an unusually large inverted repeat in the DNA (AG = -71 kcal). The second element, 200 base pairs further downstream, is an RNA polymerase II promoter which directs transcription back upstream on the complementary strand. This transcription converges on and collides with that from the 13H gene at or near the inverted repeat where transcription from both directions stops. We propose that the inverted repeat is a strong pause site which positions the converging polymerases for mutual site-specific termination.Transcription termination signals have been identified and studied extensively both in vivo and in vitro for Escherichia coli RNA polymerase and eucaryotic RNA polymerases I and III (4, 26-28, 37, 44). In E. coli, two main types of termination are recognized, factor dependent and factor independent (44). Factor-dependent termination signals precede the actual sites of termination and exhibit considerable sequence flexibility, which makes them difficult to recognize. A protein factor, usually p, interacts with the RNA to assist termination by the polymerase. Factor-independent terminators, in contrast, have well-defined sequence signals and are readily recognizable by their G+C-rich palindrome, which precedes a cluster of dT residues in the nontemplate strand of the DNA at the site of termination. Additional modes of procaryotic transcription termination also occur and may be of physiological significance. These include transcriptional interference of converging (33) or tandem (1) transcription units and transcriptional arrest caused by blockage of the DNA template by a bound factor (50).In eucaryotes, most RNA polymerase III terminators, like the factor-independent terminators in E. coli, possess a dT cluster and exhibit no obligatory requirement for a factor, but they lack a palindrome (37, 44). Eucaryotic RNA polymerase I termination (27), although factor dependent, bears little resemblance to p-dependent termination in E. coli but instead resembles aspects of the protein blockage mechanism described by Sellitti et al. (50). For polymerase I terminators, it is the DNA to which the factor binds (27), and the signal follows, rather than precedes, the site of termination (27,28).RNA polymerase II appears to incorporate elements of all the above termination mechanisms in its repertoire of strategies. Transcription of the human gastrin gene appears to terminate upstream of the termination signal as for RNA polymerase I (3, 49). The terminator for...

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The mouse ribosomal gene terminator consists of three functionally separable sequence elements.

Cited by 54 publications

References 39 publications

Binding of the Termination Factor Nsi1 to Its Cognate DNA Site Is Sufficient To Terminate RNA Polymerase I Transcription In Vitro and To Induce Termination In Vivo

Binding of the Termination Factor Nsi1 to Its Cognate DNA Site Is Sufficient To Terminate RNA Polymerase I Transcription In Vitro and To Induce Termination In Vivo

Transcription termination by nuclear RNA polymerases

Transcription termination at the chicken beta H-globin gene.

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