Progressive lengthening of 3′ untranslated regions of mRNAs by alternative polyadenylation during mouse embryonic development

Ji, Zhe; Lee, Ju Youn; Pan, Zhengxia; Jiang, Bingjun; Tian, Bin

doi:10.1073/pnas.0900028106

Cited by 528 publications

(562 citation statements)

References 35 publications

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“…Other tumor suppressors, such as CSR1 and Cdc73, have also been shown to functionally associate with 3 0 processing factors, such as CPSF3 (Zhu et al, 2009) and CPSF/ CstF (Rozenblatt-Rosen et al, 2009). Recently, it has been shown that the use of alternative mRNA 3 0 cleavage and polyadenylation sites can control the expression of certain genes by eliminating or including several cis-acting elements, such as microRNA target sites and AU-rich elements, in cancer cells and during development (Sandberg et al, 2008;Zlotorynski and Agami, 2008;Ji et al, 2009;Mayr and Bartel, 2009;Singh et al, 2009). Although more work is necessary to determine the functional relevance of the CstF/BARD1/ p53 interaction in the regulation of expression of specific genes involved in DDR, it is possible that the p53-mediated inhibition of mRNA 3 0 processing might also play a role in the selection of different alternative mRNA 3 0 cleavage sites and, consequently, in the regulation of the mRNA levels of genes involved in DDR.…”

Section: Discussionmentioning

confidence: 99%

“…It has been shown that the regulation of mRNA 3 0 end formation can have significant roles in cancer (Kleiman and Manley, 2001;Topalian et al, 2001;Scorilas, 2002;Rozenblatt-Rosen et al, 2009). Most importantly, alternative mRNA cleavage and polyadenylation changes the length of the 3 0 -untranslated region and regulates gene expression of different mRNAs in cancer cells (Mayr and Bartel 2009;Singh et al, 2009) and during cell differentiation (Sandberg et al, 2008;Zlotorynski and Agami, 2008;Ji et al, 2009). Cleavagestimulation factor (CstF) is one of the essential 3 0 processing factors and is most likely active as a dimer of an heterotrimer, consisting of three protein factors called CstF3, CstF2 and CstF1.…”

Section: Introductionmentioning

confidence: 99%

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p53 inhibits mRNA 3′ processing through its interaction with the CstF/BARD1 complex

et al. 2011

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The mechanisms involved in the p53-dependent control of gene expression following DNA damage have not been completely elucidated. Here, we show that the p53 C terminus associates with factors that are required for the ultraviolet (UV)-induced inhibition of the mRNA 3 0 cleavage step of the polyadenylation reaction, such as the tumor suppressor BARD1 and the 3 0 processing factor cleavage-stimulation factor 1 (CstF1). We found that p53 can coexist in complexes with CstF and BARD1 in extracts of UV-treated cells, suggesting a role for p53 in mRNA 3 0 cleavage following DNA damage. Consistent with this, we found that p53 inhibits 3 0 cleavage in vitro and that there is a reverse correlation between the levels of p53 expression and the levels of mRNA 3 0 cleavage under different cellular conditions. Supporting these results, a tumor-associated mutation in p53 not only decreases the interaction with BARD1 and CstF, but also decreases the UV-induced inhibition of 3 0 processing, all of which is restored by wild-type-p53 expression. We also found that p53 expression levels affect the polyadenylation levels of housekeeping genes, but not of p21 and c-fos genes, which are involved in the DNA damage response (DDR). Here, we identify a novel 3 0 RNA processing inhibitory function of p53, adding a new level of complexity to the DDR by linking RNA processing to the p53 network.

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

p53 inhibits mRNA 3′ processing through its interaction with the CstF/BARD1 complex

et al. 2011

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“…Several independent studies have revealed the remarkable fact that either levels of cell proliferation or developmental stage can cause a shift in APA from more distal to more proximal PAS selection Ji et al 2009;Mayr and Bartel 2009). In particular, rapidly dividing cells, as are often found in cancerous tissues, tend to use proximal PAS, while cells in later developmental stages tend to use more distal PAS.…”

Section: Alternative Pas (Apa) Define Different Mrna 39 Utrsmentioning

confidence: 99%

“…In general, cleavage/ poly(A) factors appear to be constitutively expressed, and little evidence exists for the selective use of factors for one PAS versus another. However, it has been observed that some cleavage/poly(A) factors may be present at lower, limiting levels in some cells, such as CstF-64 in pre-B cells (Takagaki and Manley 1998;Ji et al 2009). In this situation, stronger PAS will have a significant kinetic advantage (see below).…”

Section: Alternative Pas (Apa) Define Different Mrna 39 Utrsmentioning

confidence: 99%

Ending the message: poly(A) signals then and now

Proudfoot¹

2011

Genes Dev.

501

477

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Polyadenylation [poly(A)] signals (PAS) are a defining feature of eukaryotic protein-coding genes. The central sequence motif AAUAAA was identified in the mid1970s and subsequently shown to require flanking, auxiliary elements for both 39-end cleavage and polyadenylation of premessenger RNA (pre-mRNA) as well as to promote downstream transcriptional termination. More recent genomic analysis has established the generality of the PAS for eukaryotic mRNA. Evidence for the mechanism of mRNA 39-end formation is outlined, as is the way this RNA processing reaction communicates with RNA polymerase II to terminate transcription. The widespread phenomenon of alternative poly(A) site usage and how this interrelates with pre-mRNA splicing is then reviewed. This shows that gene expression can be drastically affected by how the message is ended. A central theme of this review is that while genomic analysis provides generality for the importance of PAS selection, detailed mechanistic understanding still requires the direct analysis of specific genes by genetic and biochemical approaches.

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“…Large numbers of alternatively spliced exons are coordinately regulated during various processes, including notably cell differentiation and cancer 1,2 , but studies mainy focused on cassette exons. Likewise, alternative polyA sites are widely regulated during several processes, most notably cell proliferation, where shorter forms are preferentially expressed [3][4][5][6][7] , but studies mainly focused on tandem polyA sites, which are located in the same exon. Thus, little is known about the regulation of alternative 3 0 terminal exons, also called alternative last exons (ALEs), which are found in 43,000 human genes and correspond to the alternative use of intronic polyA sites in a splicing-dependent manner [7][8][9] .…”

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confidence: 99%

A recently evolved class of alternative 3′-terminal exons involved in cell cycle regulation by topoisomerase inhibitors

et al. 2014

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Alternative 3 0 -terminal exons, which use intronic polyadenylation sites, are generally less conserved and expressed at lower levels than the last exon of genes. Here we discover a class of human genes, in which the last exon appeared recently during evolution, and the major gene product uses an alternative 3 0 -terminal exon corresponding to the ancestral last exon of the gene. This novel class of alternative 3 0 -terminal exons are downregulated on a large scale by doxorubicin, a cytostatic drug targeting topoisomerase II, and play a role in cell cycle regulation, including centromere-kinetochore assembly. The RNA-binding protein HuR/ ELAVL1 is a major regulator of this specific set of alternative 3 0 -terminal exons. HuR binding to the alternative 3 0 -terminal exon in the pre-messenger RNA promotes its splicing, and is reduced by topoisomerase inhibitors. These findings provide new insights into the evolution, function and molecular regulation of alternative 3 0 -terminal exons.

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Progressive lengthening of 3′ untranslated regions of mRNAs by alternative polyadenylation during mouse embryonic development

Cited by 528 publications

References 35 publications

p53 inhibits mRNA 3′ processing through its interaction with the CstF/BARD1 complex

p53 inhibits mRNA 3′ processing through its interaction with the CstF/BARD1 complex

Ending the message: poly(A) signals then and now

A recently evolved class of alternative 3′-terminal exons involved in cell cycle regulation by topoisomerase inhibitors

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