Sequence determinants and evolution of constitutive and alternative splicing in yeast species

RNA splicing is a key process in eukaryotic gene expression. Most Intron-containing genes are constitutively spliced, hence efficient splicing of an intron is crucial for efficient gene expression. Here we use a large synthetic oligo library of ~20,000 variants to explore how different intronic sequence features affect splicing efficiency and mRNA expression levels in S. cerevisiae. Using a combinatorial design of synthetic introns we demonstrate how non-consensus splice site sequences affect splicing efficiency in each of the three splice sites. We then show that S. cerevisiae splicing machinery tends to select alternative 3' splice sites downstream of the original site, and we suggest that this tendency created a selective pressure, leading to the avoidance of cryptic splice site motifs near introns' 3' ends. We further use natural intronic sequences from other yeast species, whose splicing machineries have diverged to various extents, to show how intron architectures in the various species have been adapted to the organism's splicing machinery. We suggest that the observed tendency for cryptic splicing is a result of a loss of a specific splicing factor, U2AF1. Lastly, we show that synthetic sequences containing two introns give rise to alternative RNA isoforms in S. cerevisiae, exposing intronic features that control and facilitate alternative splicing. Our study reveals novel mechanisms by which introns are shaped in evolution to allow cells to regulate their transcriptome.

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A broad analysis of splicing regulation in yeast using a large library of synthetic introns

PLoS Genetics ◽

10.1371/journal.pgen.1009805 ◽

2021 ◽

Vol 17 (9) ◽

pp. e1009805

Author(s):

Dvir Schirman ◽

Zohar Yakhini ◽

Yitzhak Pilpel ◽

Orna Dahan

Keyword(s):

Gene Expression ◽

Alternative Splicing ◽

Splice Site ◽

Donor Site ◽

Regulation Of Gene Expression ◽

Combinatorial Design ◽

Acceptor Site ◽

Functional Sites ◽

Splicing Efficiency ◽

Splicing Machinery

RNA splicing is a key process in eukaryotic gene expression, in which an intron is spliced out of a pre-mRNA molecule to eventually produce a mature mRNA. Most intron-containing genes are constitutively spliced, hence efficient splicing of an intron is crucial for efficient regulation of gene expression. Here we use a large synthetic oligo library of ~20,000 variants to explore how different intronic sequence features affect splicing efficiency and mRNA expression levels in S. cerevisiae. Introns are defined by three functional sites, the 5’ donor site, the branch site, and the 3’ acceptor site. Using a combinatorial design of synthetic introns, we demonstrate how non-consensus splice site sequences in each of these sites affect splicing efficiency. We then show that S. cerevisiae splicing machinery tends to select alternative 3’ splice sites downstream of the original site, and we suggest that this tendency created a selective pressure, leading to the avoidance of cryptic splice site motifs near introns’ 3’ ends. We further use natural intronic sequences from other yeast species, whose splicing machineries have diverged to various extents, to show how intron architectures in the various species have been adapted to the organism’s splicing machinery. We suggest that the observed tendency for cryptic splicing is a result of a loss of a specific splicing factor, U2AF1. Lastly, we show that synthetic sequences containing two introns give rise to alternative RNA isoforms in S. cerevisiae, demonstrating that merely a synthetic fusion of two introns might be suffice to facilitate alternative splicing in yeast. Our study reveals novel mechanisms by which introns are shaped in evolution to allow cells to regulate their transcriptome. In addition, it provides a valuable resource to study the regulation of constitutive and alternative splicing in a model organism.

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hnRNP A1 Regulates Alternative Splicing of Tau Exon 10 by Targeting 3′ Splice Sites

Cells ◽

10.3390/cells9040936 ◽

2020 ◽

Vol 9 (4) ◽

pp. 936 ◽

Cited By ~ 1

Author(s):

Yongchao Liu ◽

Donggun Kim ◽

Namjeong Choi ◽

Jagyeong Oh ◽

Jiyeon Ha ◽

...

Keyword(s):

Gene Expression ◽

Gene Ontology ◽

Alternative Splicing ◽

Splice Site ◽

Hnrnp A1 ◽

Gene Ontology Analysis ◽

Splice Sites ◽

Neuronal Function ◽

Brain Functions ◽

Exon 10

The ratio control of 4R-Tau/3R-Tau by alternative splicing of Tau exon 10 is important for maintaining brain functions. In this study, we show that hnRNP A1 knockdown induces inclusion of endogenous Tau exon 10, conversely, overexpression of hnRNP A1 promotes exon 10 skipping of Tau. In addition, hnRNP A1 inhibits splicing of intron 9, but not intron 10. Furthermore, hnRNP A1 directly interacts with the 3′ splice site of exon 10 to regulate its functions in alternative splicing. Finally, gene ontology analysis demonstrates that hnRNP A1-induced splicing and gene expression targets a subset of genes with neuronal function.

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A moveable 5' splice site in adenine phosphoribosyltransferase genes of Drosophila species.

Molecular and Cellular Biology ◽

10.1128/mcb.9.5.2220 ◽

1989 ◽

Vol 9 (5) ◽

pp. 2220-2223 ◽

Cited By ~ 6

Author(s):

D Johnson ◽

S Henikoff

Keyword(s):

Gene Expression ◽

Alternative Splicing ◽

Splice Site ◽

Gene Evolution ◽

Drosophila Species ◽

Splice Sites ◽

Adenine Phosphoribosyltransferase ◽

Splice Junctions ◽

Encoding Genes ◽

Normal Feature

In two distantly related Drosophila species, the use of alternate 5' splice sites to process an intron in pre-mRNA from homologous adenine phosphoribosyltransferase (APRT)-encoding genes led to RNAs encoding nonfunctional peptides in addition to APRT. The production of aberrantly spliced transcripts as a normal feature of gene expression supports a general model of eucaryotic gene evolution through alternative splicing and moveable splice junctions.

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A moveable 5' splice site in adenine phosphoribosyltransferase genes of Drosophila species

Molecular and Cellular Biology ◽

10.1128/mcb.9.5.2220-2223.1989 ◽

1989 ◽

Vol 9 (5) ◽

pp. 2220-2223

Author(s):

D Johnson ◽

S Henikoff

Keyword(s):

Gene Expression ◽

Alternative Splicing ◽

Splice Site ◽

Gene Evolution ◽

Drosophila Species ◽

Splice Sites ◽

Adenine Phosphoribosyltransferase ◽

Splice Junctions ◽

Encoding Genes ◽

Normal Feature

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Discovery of driver non-coding splice-site-creating mutations in cancer

Nature Communications ◽

10.1038/s41467-020-19307-6 ◽

2020 ◽

Vol 11 (1) ◽

Author(s):

Song Cao ◽

Daniel Cui Zhou ◽

Clara Oh ◽

Reyka G. Jayasinghe ◽

Yanyan Zhao ◽

...

Keyword(s):

Gene Expression ◽

Splice Site ◽

Rna Splicing ◽

Large Scale ◽

Intron Size ◽

Splice Sites ◽

Genome Wide ◽

Clinical Consequences

Abstract Non-coding mutations can create splice sites, however the true extent of how such somatic non-coding mutations affect RNA splicing are largely unexplored. Here we use the MiSplice pipeline to analyze 783 cancer cases with WGS data and 9494 cases with WES data, discovering 562 non-coding mutations that lead to splicing alterations. Notably, most of these mutations create new exons. Introns associated with new exon creation are significantly larger than the genome-wide average intron size. We find that some mutation-induced splicing alterations are located in genes important in tumorigenesis (ATRX, BCOR, CDKN2B, MAP3K1, MAP3K4, MDM2, SMAD4, STK11, TP53 etc.), often leading to truncated proteins and affecting gene expression. The pattern emerging from these exon-creating mutations suggests that splice sites created by non-coding mutations interact with pre-existing potential splice sites that originally lacked a suitable splicing pair to induce new exon formation. Our study suggests the importance of investigating biological and clinical consequences of noncoding splice-inducing mutations that were previously neglected by conventional annotation pipelines. MiSplice will be useful for automatically annotating the splicing impact of coding and non-coding mutations in future large-scale analyses.

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Role of small nuclear RNAs in eukaryotic gene expression

Essays in Biochemistry ◽

10.1042/bse0540079 ◽

2013 ◽

Vol 54 ◽

pp. 79-90 ◽

Cited By ~ 34

Author(s):

Saba Valadkhan ◽

Lalith S. Gunawardane

Keyword(s):

Gene Expression ◽

Protein Interactions ◽

Rna Stability ◽

Splice Sites ◽

Branch Site ◽

Small Nuclear Rnas ◽

Eukaryotic Gene Expression ◽

Eukaryotic Gene ◽

Rna Biogenesis

Eukaryotic cells contain small, highly abundant, nuclear-localized non-coding RNAs [snRNAs (small nuclear RNAs)] which play important roles in splicing of introns from primary genomic transcripts. Through a combination of RNA–RNA and RNA–protein interactions, two of the snRNPs, U1 and U2, recognize the splice sites and the branch site of introns. A complex remodelling of RNA–RNA and protein-based interactions follows, resulting in the assembly of catalytically competent spliceosomes, in which the snRNAs and their bound proteins play central roles. This process involves formation of extensive base-pairing interactions between U2 and U6, U6 and the 5′ splice site, and U5 and the exonic sequences immediately adjacent to the 5′ and 3′ splice sites. Thus RNA–RNA interactions involving U2, U5 and U6 help position the reacting groups of the first and second steps of splicing. In addition, U6 is also thought to participate in formation of the spliceosomal active site. Furthermore, emerging evidence suggests additional roles for snRNAs in regulation of various aspects of RNA biogenesis, from transcription to polyadenylation and RNA stability. These snRNP-mediated regulatory roles probably serve to ensure the co-ordination of the different processes involved in biogenesis of RNAs and point to the central importance of snRNAs in eukaryotic gene expression.

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Control of adenovirus E1B mRNA synthesis by a shift in the activities of RNA splice sites

Molecular and Cellular Biology ◽

10.1128/mcb.4.5.966-972.1984 ◽

1984 ◽

Vol 4 (5) ◽

pp. 966-972

Author(s):

C Montell ◽

E F Fisher ◽

M H Caruthers ◽

A J Berk

Keyword(s):

Splice Site ◽

Rna Splicing ◽

Early Phase ◽

Late Phase ◽

Productive Infection ◽

Splice Sites ◽

Mrna Synthesis ◽

Adenovirus E1b ◽

Cryptic Splice Sites ◽

Rna Splice Sites

The primary transcript from adenovirus 2 early region 1B (E1B) is processed by differential RNA splicing into two overlapping mRNAs, 13S and 22S. The 22S mRNA is the major E1B mRNA during the early phase of infection, whereas the 13S mRNA predominates during the late phase. In previous work, it has been shown that this shift in proportions of the E1B mRNAs is influenced by increased cytoplasmic stability of the 13S mRNA at late times in infection. Two observations presented here demonstrate that the increase in proportion of the 13S mRNA at late times is also regulated by a change in the specificity of RNA splicing. First, the relative concentrations of the 13S to 22S nuclear RNAs were not constant throughout infection but increased at late times. Secondly, studies with the mutant, adenovirus 2 pm2250 , provided evidence that there was an increased propensity to utilize a 5' splice in the region of the 13S 5' splice site at late times in infection. Adenovirus 2 pm2250 has a G----C transversion in the first base of E1B 13S mRNA intron preventing splicing of the 13S mRNA but not of the 22S mRNA. During the early phase of a pm2250 infection, the E1B primary transcripts were processed into the 22S mRNA only. However, during the late phase, when the 13S mRNA normally predominates, E1B primary transcripts were also processed by RNA splicing at two formerly unused or cryptic 5' splice sites. Both cryptic splice sites were located much closer to the disrupted 13S 5' splice site than to the 22S 5' splice site. Thus, the temporal increase in proportion of the 13S mRNA to the 22S mRNA is regulated by two processes, an increase in cytoplasmic stability of the 13S mRNA and an increased propensity to utilize the 13S 5' splice site during the late phase of infection. Adenovirus 2 pm2250 was not defective for productive infection of HeLa cells or for transformation of rat cells.

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ALG-1 Influences Accurate mRNA Splicing Patterns in the Caenorhabditis elegans Intestine and Body Muscle Tissues by Modulating Splicing Factor Activities

Genetics ◽

10.1534/genetics.119.302223 ◽

2019 ◽

Vol 212 (3) ◽

pp. 931-951 ◽

Cited By ~ 3

Author(s):

Kasuen Kotagama ◽

Anna L. Schorr ◽

Hannah S. Steber ◽

Marco Mangone

Keyword(s):

Gene Expression ◽

Alternative Splicing ◽

Rna Splicing ◽

Specific Gene ◽

Splicing Factors ◽

Tissue Specific ◽

Link Type ◽

Body Muscle ◽

Mirna Targets ◽

Mirna Pathway

MicroRNAs (miRNAs) are known to modulate gene expression, but their activity at the tissue-specific level remains largely uncharacterized. To study their contribution to tissue-specific gene expression, we developed novel tools to profile putative miRNA targets in the Caenorhabditis elegans intestine and body muscle. We validated many previously described interactions and identified ∼3500 novel targets. Many of the candidate miRNA targets curated are known to modulate the functions of their respective tissues. Within our data sets we observed a disparity in the use of miRNA-based gene regulation between the intestine and body muscle. The intestine contained significantly more putative miRNA targets than the body muscle highlighting its transcriptional complexity. We detected an unexpected enrichment of RNA-binding proteins targeted by miRNA in both tissues, with a notable abundance of RNA splicing factors. We developed in vivo genetic tools to validate and further study three RNA splicing factors identified as putative miRNA targets in our study (asd-2, hrp-2, and smu-2), and show that these factors indeed contain functional miRNA regulatory elements in their 3′UTRs that are able to repress their expression in the intestine. In addition, the alternative splicing pattern of their respective downstream targets (unc-60, unc-52, lin-10, and ret-1) is dysregulated when the miRNA pathway is disrupted. A reannotation of the transcriptome data in C. elegans strains that are deficient in the miRNA pathway from past studies supports and expands on our results. This study highlights an unexpected role for miRNAs in modulating tissue-specific gene isoforms, where post-transcriptional regulation of RNA splicing factors associates with tissue-specific alternative splicing.

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In vivo recognition of a vertebrate mini-exon as an exon-intron-exon unit.

Molecular and Cellular Biology ◽

10.1128/mcb.13.5.2677 ◽

1993 ◽

Vol 13 (5) ◽

pp. 2677-2687 ◽

Cited By ~ 40

Author(s):

D A Sterner ◽

S M Berget

Keyword(s):

Splice Site ◽

Rna Splicing ◽

Troponin I ◽

Exon Skipping ◽

Splice Sites ◽

Small Vertebrate ◽

Upstream Exon ◽

I Gene

Very small vertebrate exons are problematic for RNA splicing because of the proximity of their 3' and 5' splice sites. In this study, we investigated the recognition of a constitutive 7-nucleotide mini-exon from the troponin I gene that resides quite close to the adjacent upstream exon. The mini-exon failed to be included in spliced RNA when placed in a heterologous gene unless accompanied by the upstream exon. The requirement for the upstream exon disappeared when the mini-exon was internally expanded, suggesting that the splice sites bordering the mini-exon are compatible with those of other constitutive vertebrate exons and that the small size of the exon impaired inclusion. Mutation of the 5' splice site of the natural upstream exon did not result in either exon skipping or activation of a cryptic 5' splice site, the normal vertebrate phenotypes for such mutants. Instead, a spliced RNA accumulated that still contained the upstream intron. In vitro, the mini-exon failed to assemble into spliceosome complexes unless either internally expanded or accompanied by the upstream exon. Thus, impaired usage of the mini-exon in vivo was accompanied by impaired recognition in vitro, and recognition of the mini-exon was facilitated by the presence of the upstream exon in vivo and in vitro. Cumulatively, the atypical in vivo and in vitro properties of the troponin exons suggest a mechanism for the recognition of this mini-exon in which initial recognition of an exon-intron-exon unit is followed by subsequent recognition of the intron.

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An Intronic Splicing Enhancer Binds U1 snRNPs To Enhance Splicing and Select 5′ Splice Sites

Molecular and Cellular Biology ◽

10.1128/mcb.20.24.9225-9235.2000 ◽

2000 ◽

Vol 20 (24) ◽

pp. 9225-9235 ◽

Cited By ~ 50

Author(s):

Andrew J. McCullough ◽

Susan M. Berget

Keyword(s):

Splice Site ◽

Maximal Activity ◽

Splice Sites ◽

Base Pairing ◽

Rich Region ◽

U1 Snrnp ◽

Splicing Efficiency ◽

Site Recognition ◽

Splicing Enhancer

ABSTRACT Intronic G triplets are frequently located adjacent to 5′ splice sites in vertebrate pre-mRNAs and have been correlated with splicing efficiency and specificity via a mechanism that activates upstream 5′ splice sites in exons containing duplicated sites (26). Using an intron dependent upon G triplets for maximal activity and 5′ splice site specificity, we determined that these elements bind U1 snRNPs via base pairing with U1 RNA. This interaction is novel in that it uses nucleotides 8 to 10 of U1 RNA and is independent of nucleotides 1 to 7. In vivo functionality of base pairing was documented by restoring activity and specificity to mutated G triplets through compensating U1 RNA mutations. We suggest that the G-rich region near vertebrate 5′ splice sites promotes accurate splice site recognition by recruiting the U1 snRNP.

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