Your search keyword '"ICLIP"' showing total 14 results

1. Improved library preparation with the new iCLIP2 protocol

Author

Andreas Buchbender, F. X. Reymond Sutandy, Heike Hänel, Nadine Körtel, Holger Mutter, Stefanie Ebersberger, Anke Busch, and Julian König

Subjects

0303 health sciences, Binding Sites, DNA, Complementary, Ultraviolet Rays, Computer science, Library preparation, 030302 biochemistry & molecular biology, RNA-Binding Proteins, Computational biology, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Cross-Linking Reagents, Adapter (genetics), Humans, Immunoprecipitation, Molecular Biology, ICLIP, Gene Library, 030304 developmental biology

Abstract

Individual-nucleotide resolution UV crosslinking and immunoprecipitation (iCLIP) is a state-of-the-art technology to map the RNA interaction sites of an RNA-binding protein (RBP) across the transcriptome. Here, we present the new iCLIP2 protocol that allows to obtain high-quality iCLIP libraries in a fast and efficient manner. The new protocol comprises separate adapter ligations, two cDNA amplification steps and bead-based size selection. The full procedure can be completed within four days. Our advances significantly increase the complexity of the iCLIP2 libraries, resulting in a more comprehensive representation of RBP binding sites. Overall, the methodological advances in iCLIP2 allow efficient library generation and thereby promote the versatile and flexible application of this important technology.

Published

2020

2. CLIP and RNA interactome studies to unravel genome-wide RNA-protein interactions in vivo in Arabidopsis thaliana

Author

Marlene Reichel, Tino Köster, and Dorothee Staiger

Subjects

0303 health sciences, biology, 030302 biochemistry & molecular biology, Arabidopsis, High-Throughput Nucleotide Sequencing, RNA-Binding Proteins, food and beverages, RNA, RNA-binding protein, Computational biology, biology.organism_classification, Interactome, General Biochemistry, Genetics and Molecular Biology, Transcriptome, 03 medical and health sciences, Immunoprecipitation, Arabidopsis thaliana, Molecular Biology, Post-transcriptional regulation, ICLIP, Genome, Plant, 030304 developmental biology

Abstract

Post-transcriptional regulation makes an important contribution to adjusting the transcriptome to environmental changes in plants. RNA-binding proteins are key players that interact specifically with mRNAs to co-ordinate their fate. While the regulatory interactions between proteins and RNA are well understood in animals, until recently little information was available on the global binding landscape of RNA-binding proteins in higher plants. This is not least due to technical challenges in plants. In turn, while numerous RNA-binding proteins have been identified through mutant analysis and homology-based searches in plants, only recently a full compendium of proteins with RNA-binding activity has been experimentally determined for the reference plant Arabidopsis thaliana. State-of-the-art techniques to determine RNA-protein interactions genome-wide in animals are based on the covalent fixation of RNA and protein in vivo by UV light. This has only recently been successfully applied to plants. Here, we present practical considerations on the application of UV irradiation based methods to comprehensively determine in vivo RNA-protein interactions in Arabidopsis thaliana, focussing on individual nucleotide resolution crosslinking immunoprecipitation (iCLIP) and mRNA interactome capture. Copyright © 2019 Elsevier Inc. All rights reserved.

Published

2020

3. RNA inhibits dMi-2/CHD4 Chromatin Binding and Nucleosome Remodelling

Author

Lea Albert, Thorsten Stiewe, Joel P. Mackay, Jonathan Lenz, Mara John, Roland K. Hartmann, Ho-Ryung Chung, Yichen Zhong, Clemens Thölken, Olalla Vázquez, Oliver Roßbach, Markus Gößringer, Andrea Nist, Alexander Brehm, and Ikram Ullah

Subjects

History, Polymers and Plastics, RNase P, Chemistry, Chromatin binding, RNA, Industrial and Manufacturing Engineering, Cell biology, Chromatin, Nucleosome mobilization, Transcription (biology), Nucleosome, Business and International Management, human activities, ICLIP

Abstract

The ATP-dependent nucleosome remodeller Mi-2/CHD4 broadly modulates epigenetic landscapes to repress transcription and to maintain genome integrity. Here we use individual nucleotide resolution crosslinking and immunoprecipitation (iCLIP) to show that Drosophila Mi-2 associates with thousands of mRNA molecules in vivo. Biochemical data reveal that recombinant dMi-2 preferentially binds to G-rich RNA molecules using two intrinsically disordered regions of previously undefined function. Pharmacological inhibition of transcription and RNase digestion approaches establish that RNA inhibits the association of dMi-2 with chromatin. We also show that RNA inhibits dMi-2-mediated nucleosome mobilization by competing with the nucleosome substrate. Importantly, this activity is shared by CHD4, the human homolog of dMi-2, strongly suggesting that RNA-mediated regulation of remodeller activity is an evolutionary conserved mechanism. Our data support a model in which RNA serves to protect actively transcribed regions of the genome from dMi-2/CHD4mediated establishment of repressive chromatin structures.

Published

2021

4. SARS-CoV-2 nucleocapsid protein binds host mRNAs and attenuates stress granules to impair host stress response

Author

Syed Nabeel-Shah, Hyunmin Lee, Nujhat Ahmed, Giovanni L. Burke, Shaghayegh Farhangmehr, Kanwal Ashraf, Shuye Pu, Ulrich Braunschweig, Guoqing Zhong, Hong Wei, Hua Tang, Jianyi Yang, Edyta Marcon, Benjamin J. Blencowe, Zhaolei Zhang, and Jack F. Greenblatt

Subjects

G3BP1, mRNA-binding, Proteomics, G3BP2, Cell biology, 0303 health sciences, Multidisciplinary, SARS-CoV-2, Molecular biology, iCLIP, viruses, Science, COVID-19, Article, N protein, Gene regulation, 3. Good health, 03 medical and health sciences, 0302 clinical medicine, Stress granules, Virology, Nucleocapsid, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) nucleocapsid (N) protein is essential for viral replication, making it a promising target for antiviral drug and vaccine development. SARS-CoV-2 infected patients exhibit an uncoordinated immune response; however, the underlying mechanistic details of this imbalance remain obscure. Here, starting from a functional proteomics workflow, we catalogued the protein-protein interactions of SARS-CoV-2 proteins, including an evolutionarily conserved specific interaction of N with the stress granule resident proteins G3BP1 and G3BP2. N localizes to stress granules and sequesters G3BPs away from their typical interaction partners, thus attenuating stress granule formation. We found that N binds directly to host mRNAs in cells, with a preference for 3´ UTRs, and modulates target mRNA stability. We show that the N protein rewires the G3BP1 mRNA-binding profile and suppresses the physiological stress response of host cells, which may explain the imbalanced immune response observed in SARS-CoV-2 infected patients., Graphical Abstract

Published

2022

5. Co-transcriptional Loading of RNA Export Factors Shapes the Human Transcriptome

Author

Stuart A. Wilson, Nicolas Viphakone, Catherine G. Heath, Llywelyn Griffith, David Sims, and Ian Sudbery

Subjects

Nucleocytoplasmic Transport Proteins, Polyadenylation, TREX, Transcription, Genetic, Active Transport, Cell Nucleus, Biology, Article, RNA Transport, NXF1, DEAD-box RNA Helicases, 03 medical and health sciences, 0302 clinical medicine, Humans, RNA, Messenger, Molecular Biology, co-transcriptional splicing, 030304 developmental biology, 0303 health sciences, Messenger RNA, Cap binding complex, Binding Sites, alternative polyadenylation, RNA, Nuclear Proteins, RNA-Binding Proteins, Cell Biology, Exons, 3. Good health, Cell biology, EJC, Gene Expression Regulation, RNA splicing, Eukaryotic Initiation Factor-4A, Exon junction complex, nucleo-cytoplasmic transport, Transcriptome, ICLIP, 030217 neurology & neurosurgery, Transcription Factors

Abstract

Summary During gene expression, RNA export factors are mainly known for driving nucleo-cytoplasmic transport. While early studies suggested that the exon junction complex (EJC) provides a binding platform for them, subsequent work proposed that they are only recruited by the cap binding complex to the 5′ end of RNAs, as part of TREX. Using iCLIP, we show that the export receptor Nxf1 and two TREX subunits, Alyref and Chtop, are recruited to the whole mRNA co-transcriptionally via splicing but before 3′ end processing. Consequently, Alyref alters splicing decisions and Chtop regulates alternative polyadenylation. Alyref is recruited to the 5′ end of RNAs by CBC, and our data reveal subsequent binding to RNAs near EJCs. We demonstrate that eIF4A3 stimulates Alyref deposition not only on spliced RNAs close to EJC sites but also on single-exon transcripts. Our study reveals mechanistic insights into the co-transcriptional recruitment of mRNA export factors and how this shapes the human transcriptome., Graphical Abstract, Highlights • 5′ cap binding complex CBC acts as a transient landing pad for Alyref • Alyref is deposited upstream of the exon-exon junction next to the EJC • Alyref can be deposited on introns and regulate splicing • Chtop is mainly deposited on 3′ UTRs and influences poly(A) site choices, TREX plays a pivotal role in RNA export, though the mechanisms governing its deposition on RNA are obscure. Viphakone et al. show that the cap binding and exon junction complexes drive the ordered deposition of TREX throughout the body of RNA. In doing so, TREX regulates processing of the RNA.

Published

2019

6. Global analysis of CPSF2-mediated alternative splicing: Integration of global iCLIP and transcriptome profiling data

Author

Michael R. Green, Lihua Julie Zhu, Ashish Misra, and Jianhong Ou

Subjects

lcsh:QH426-470, iCLIP, RNA-Seq, Cleavage and polyadenylation specificity factor, Biology, Biochemistry, SYMPK, 03 medical and health sciences, RNA interference, Data in Brief, Genetics, 030304 developmental biology, 0303 health sciences, Gene knockdown, 030302 biochemistry & molecular biology, Alternative splicing, lcsh:Genetics, RNA splicing, Proteome, Molecular Medicine, CPSF, RNA-seq, ICLIP, Biotechnology

Abstract

Alternative splicing is a key mechanism for generating proteome diversity, however the mechanisms regulating alternative splicing are poorly understood. Using a genome-wide RNA interference screening strategy, we identified cleavage and polyadenylation specificity factor (CPSF) and symplekin (SYMPK) as cofactors of the well-known splicing regulator RBFOX2. To determine the role of CPSF in alternative splicing on a genome-wide level, we performed paired-end RNA sequencing (RNA-seq) to compare splicing events in control cells and RBFOX2 or CPSF2 knockdown cells. We also performed individual-nucleotide resolution UV cross-linking and immunoprecipitation (iCLIP) to identify direct binding targets of RBFOX2 and CPSF2. Here, we describe the experimental design, and the quality control and data analyses that were performed on the dataset. The raw sequencing data have been deposited in NCBI's Gene Expression Omnibus and are accessible through GEO Series accession number GSE60392.

Published

2015

7. Aubergine iCLIP Reveals piRNA-Dependent Decay of mRNAs Involved in Germ Cell Development in the Early Embryo

Author

Martine Simonelig, Tomaz Curk, Stéphanie Pierson, Jean-Pierre Desvignes, Fillip Port, Thomas Grentzinger, Jeremy Dufourt, Catherine Papin, Claudia Armenise, Grégory Baronian, Bridlin Barckmann, Séverine Chambeyron, Institut de génétique humaine (IGH), Université de Montpellier (UM)-Centre National de la Recherche Scientifique (CNRS), Division of Cell Biology, Medical Research Council Laboratory of Molecular Biology, Cambridge CB2 0QH, UK, Institut de Génomique Fonctionnelle - Montpellier GenomiX (IGF MGX), Institut de Génomique Fonctionnelle (IGF), Université de Montpellier (UM)-Université Montpellier 1 (UM1)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Montpellier 2 - Sciences et Techniques (UM2)-Centre National de la Recherche Scientifique (CNRS)-Université de Montpellier (UM)-Université Montpellier 1 (UM1)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Montpellier 2 - Sciences et Techniques (UM2)-Centre National de la Recherche Scientifique (CNRS), and Faculty of Computer and Information Science, University of Ljubljana, 1000 Ljubljana, Slovenia

Subjects

Resource, endocrine system, RNA Stability, Piwi-interacting RNA, Biology, General Biochemistry, Genetics and Molecular Biology, Germline, 03 medical and health sciences, 0302 clinical medicine, Peptide Initiation Factors, medicine, Animals, Drosophila Proteins, RNA, Messenger, RNA Processing, Post-Transcriptional, RNA, Small Interfering, lcsh:QH301-705.5, 030304 developmental biology, Regulation of gene expression, Genetics, AU-rich element, [SDV.GEN]Life Sciences [q-bio]/Genetics, 0303 health sciences, urogenital system, MRNA cleavage, Gene Expression Regulation, Developmental, RNA, 3. Good health, Germ Cells, medicine.anatomical_structure, lcsh:Biology (General), Drosophila, ICLIP, 030217 neurology & neurosurgery, Germ cell

Abstract

Summary The Piwi-interacting RNA (piRNA) pathway plays an essential role in the repression of transposons in the germline. Other functions of piRNAs such as post-transcriptional regulation of mRNAs are now emerging. Here, we perform iCLIP with the PIWI protein Aubergine (Aub) and identify hundreds of maternal mRNAs interacting with Aub in the early Drosophila embryo. Gene expression profiling reveals that a proportion of these mRNAs undergo Aub-dependent destabilization during the maternal-to-zygotic transition. Strikingly, Aub-dependent unstable mRNAs encode germ cell determinants. iCLIP with an Aub mutant that is unable to bind piRNAs confirms piRNA-dependent binding of Aub to mRNAs. Base pairing between piRNAs and mRNAs can induce mRNA cleavage and decay that are essential for embryonic development. These results suggest general regulation of maternal mRNAs by Aub and piRNAs, which plays a key developmental role in the embryo through decay and localization of mRNAs encoding germ cell determinants., Graphical Abstract, Highlights • Aub binds to maternal mRNAs in early Drosophila embryos • Interaction between Aub and maternal mRNAs depends on piRNAs • aub mutants are defective in mRNA decay during the MZT • Aub-dependent unstable mRNAs encode germ cell determinants, Using iCLIP, Barckmann et al. identify several hundred maternal mRNAs that interact with Aub in early embryos. A number of these mRNAs undergo Aub-dependent destabilization in the soma during the maternal-to-zygotic transition and encode germ cell determinants.

Published

2015

8. MOV10 and FMRP Regulate AGO2 Association with MicroRNA Recognition Elements

Author

Kenneth S. Kosik, Hongjun Zhou, Stephanie Ceman, Radhika S. Khetani, Geena Skariah, Phillip J. Kenny, Miri Kim, Mary Luz Arcila, and Jenny Drnevich

Subjects

congenital, hereditary, and neonatal diseases and abnormalities, Knockout, Medical Physiology, Biology, General Biochemistry, Genetics and Molecular Biology, Article, Fragile X Mental Retardation Protein, Mice, microRNA, Translational regulation, Animals, Humans, Binding site, lcsh:QH301-705.5, 3' Untranslated Regions, Genetics, Mice, Knockout, Binding Sites, Mechanism (biology), Brain, Translation (biology), RNA Helicase A, Cell biology, GC Rich Sequence, nervous system diseases, MicroRNAs, HEK293 Cells, lcsh:Biology (General), Argonaute Proteins, RNA Interference, Biochemistry and Cell Biology, Transcriptome, ICLIP, Function (biology), RNA Helicases, Protein Binding

Abstract

© 2014 The Authors. The fragile X mental retardation protein FMRP regulates translation of its bound mRNAs through incompletely defined mechanisms. FMRP has been linked to the microRNA pathway, and we show here that it associates with the RNA helicase MOV10, also associated with the microRNA pathway. FMRP associates with MOV10 directly and in an RNA-dependent manner and facilitates MOV10's association with RNAs in brain and cells, suggesting a cooperative interaction. We identified the RNAs recognized by MOV10 using RNA immunoprecipitation and iCLIP. Examination of the fate of MOV10 on RNAs revealed a dual function for MOV10 in regulating translation: it facilitates microRNA-mediated translation of some RNAs, but it also increases expression of other RNAs by preventing AGO2 function. The latter subset was also bound by FMRP in close proximity to the MOV10 binding site, suggesting that FMRP prevents MOV10-mediated microRNA suppression. We have identified a mechanism for FMRP-mediated translational regulation through its association with MOV10. Kenny etal. show that FMRP recruits the helicase MOV10 to mRNAs for translation regulation. MOV10 and FMRP modulate AGO association with RNAs, and all three proteins bind near microRNA recognition elements. MOV10 usually facilitates microRNA-mediated regulation; however, proximal binding of FMRP blocks AGO association to allow translation.

Published

2014

9. Endogenous miRNA and Target Concentrations Determine Susceptibility to Potential ceRNA Competition

Author

Phillip A. Sharp, Andrew D. Bosson, Jesse R. Zamudio, Massachusetts Institute of Technology. Department of Biology, Koch Institute for Integrative Cancer Research at MIT, Bosson, Andrew David, Zamudio, Jesse Ray, and Sharp, Phillip A.

Subjects

Gene regulatory network, Computational biology, Biology, Article, Cell Line, Mice, Single-cell analysis, RNA interference, microRNA, Animals, Immunoprecipitation, Gene Regulatory Networks, 3' Untranslated Regions, Molecular Biology, Embryonic Stem Cells, Genetics, Competing endogenous RNA, Mesenchymal Stem Cells, Cell Biology, Argonaute, Non-coding RNA, MicroRNAs, Argonaute Proteins, RNA Interference, Single-Cell Analysis, ICLIP, Protein Binding

Abstract

Target competition (ceRNA crosstalk) within miRNA-regulated gene networks has been proposed to influence biological systems. To assess target competition, we characterize and quantitate miRNA networks in two cell types. Argonaute iCLIP reveals that hierarchical binding of high- to low-affinity miRNA targets is a key characteristic of in vivo activity. Quantification of cellular miRNA and mRNA/ncRNA target pool levels indicates that miRNA:target pool ratios and an affinity partitioned target pool accurately predict in vivo Ago binding profiles and miRNA susceptibility to target competition. Using single-cell reporters, we directly test predictions and estimate that ∼3,000 additional high-affinity target sites can affect active miRNA families with low endogenous miRNA:target ratios, such as miR-92/25. In contrast, the highly expressed miR-294 and let-7 families are not susceptible to increases of nearly 10,000 sites. These results show differential susceptibility based on endogenous miRNA:target pool ratios and provide a physiological context for ceRNA competition in vivo., National Institutes of Health (U.S.) (Grants RO1-GM34277 and R01-CA133404), National Cancer Institute (U.S.) (Grants PO1-CA42063 and F32CA139902), National Cancer Institute (U.S.) (Cancer Center Support Core Grant P30-CA14051)

Published

2014

10. Rbfox2-Coordinated Alternative Splicing of Mef2d and Rock2 Controls Myoblast Fusion during Myogenesis

Author

Zheng Xia, Wei Li, Marissa A. Scavuzzo, Christopher S. Bland, Jernej Ule, Auinash Kalsotra, Ravi K. Singh, Thomas A. Cooper, and Tomaz Curk

Subjects

Protein isoform, Exonic splicing enhancer, RNA-binding protein, Biology, Muscle Development, Article, Cell Line, Myoblasts, Mice, Myoblast fusion, Chlorocebus aethiops, Animals, Humans, Protein Isoforms, Molecular Biology, Conserved Sequence, Genetics, rho-Associated Kinases, MEF2 Transcription Factors, Sequence Analysis, RNA, Myogenesis, Alternative splicing, RNA-Binding Proteins, Cell Biology, Cell biology, Alternative Splicing, HEK293 Cells, Gene Expression Regulation, Organ Specificity, COS Cells, RNA splicing, RNA, ICLIP

Abstract

Alternative splicing plays important regulatory roles during periods of physiological change. During development, a large number of genes coordinately express protein isoform transitions regulated by alternative splicing; however, the mechanisms that coordinate splicing and the functional integration of the resultant tissue-specific protein isoforms are typically unknown. Here we show that the conserved Rbfox2 RNA binding protein regulates 30% of the splicing transitions observed during myogenesis and is required for the specific step of myoblast fusion. Integration of Rbfox2-dependent splicing outcomes from RNA-seq with Rbfox2 iCLIP data identified Mef2d and Rock2 as Rbfox2 splicing targets. Restored activities of Mef2d and Rock2 rescued myoblast fusion in Rbfox2-depleted cultures, demonstrating functional cooperation of protein isoforms generated by coordinated alterative splicing. The results demonstrate that coordinated alternative splicing by a single RNA binding protein modulates transcription (Mef2d) and cell signaling (Rock2) programs to drive tissue-specific functions (cell fusion) to promote a developmental transition.

Published

2014

11. Direct Competition between hnRNP C and U2AF65 Protects the Transcriptome from the Exonization of Alu Elements

Author

Mojca Tajnik, Alejandro Reyes, Isabelle Stévant, Inigo Martincorena, Sebastian Eustermann, Kathi Zarnack, Jernej Ule, Julian König, Simon Anders, and Nicholas M. Luscombe

Subjects

Alu element, Biology, General Biochemistry, Genetics and Molecular Biology, Evolution, Molecular, Transcriptome, 03 medical and health sciences, Splicing factor, Exon, 0302 clinical medicine, Alu Elements, Splicing Factor U2AF, Humans, Immunoprecipitation, 030304 developmental biology, Genetics, 0303 health sciences, Sequence Analysis, RNA, Biochemistry, Genetics and Molecular Biology(all), Gene Expression Profiling, Heterogeneous-Nuclear Ribonucleoprotein Group C, High-Throughput Nucleotide Sequencing, Nuclear Proteins, Exons, Ribonucleoproteins, Gene Knockdown Techniques, Human genome, RNA Splice Sites, ICLIP, 030217 neurology & neurosurgery, HeLa Cells, Minigene

Abstract

SummaryThere are ∼650,000 Alu elements in transcribed regions of the human genome. These elements contain cryptic splice sites, so they are in constant danger of aberrant incorporation into mature transcripts. Despite posing a major threat to transcriptome integrity, little is known about the molecular mechanisms preventing their inclusion. Here, we present a mechanism for protecting the human transcriptome from the aberrant exonization of transposable elements. Quantitative iCLIP data show that the RNA-binding protein hnRNP C competes with the splicing factor U2AF65 at many genuine and cryptic splice sites. Loss of hnRNP C leads to formation of previously suppressed Alu exons, which severely disrupt transcript function. Minigene experiments explain disease-associated mutations in Alu elements that hamper hnRNP C binding. Thus, by preventing U2AF65 binding to Alu elements, hnRNP C plays a critical role as a genome-wide sentinel protecting the transcriptome. The findings have important implications for human evolution and disease.

Published

2013

12. The mRNA-Bound Proteome and Its Global Occupancy Profile on Protein-Coding Transcripts

Author

Kevin Drew, Noah Youngs, Markus Schueler, Markus Landthaler, Alexandra Vasile, Matthias Selbach, Mathias Munschauer, Emanuel Wyler, Alexander G. Baltz, Björn Schwanhäusser, Christoph Dieterich, Duncan Penfold-Brown, Miha Milek, Richard Bonneau, and Yasuhiro Murakawa

Subjects

Genetics, Proteomics, Messenger RNA, Binding Sites, Sequence analysis, Sequence Analysis, RNA, Quantitative proteomics, RNA, RNA-Binding Proteins, Computational biology, Cell Biology, Biology, Mass Spectrometry, Cell Line, RNA splicing, Proteome, Humans, RNA, Messenger, Binding site, ICLIP, Molecular Biology

Abstract

Protein-RNA interactions are fundamental to core biological processes, such as mRNA splicing, localization, degradation, and translation. We developed a photoreactive nucleotide-enhanced UV crosslinking and oligo(dT) purification approach to identify the mRNA-bound proteome using quantitative proteomics and to display the protein occupancy on mRNA transcripts by next-generation sequencing. Application to a human embryonic kidney cell line identified close to 800 proteins. To our knowledge, nearly one-third were not previously annotated as RNA binding, and about 15% were not predictable by computational methods to interact with RNA. Protein occupancy profiling provides a transcriptome-wide catalog of potential cis-regulatory regions on mammalian mRNAs and showed that large stretches in 3' UTRs can be contacted by the mRNA-bound proteome, with numerous putative binding sites in regions harboring disease-associated nucleotide polymorphisms. Our observations indicate the presence of a large number of mRNA binders with diverse molecular functions participating in combinatorial posttranscriptional gene-expression networks.

Published

2012

13. Transcriptome-wide Identification of RNA-Binding Protein and MicroRNA Target Sites by PAR-CLIP

Author

Manuel Ascano, Andrea Rothballer, Anna-Carina Jungkamp, Markus Hafner, Jean Hausser, Lukas Burger, Thomas Tuschl, Mihaela Zavolan, Mohsen Khorshid, Alexander Ulrich, Greg S. Wardle, Mathias Munschauer, Philipp Berninger, Scott Dewell, and Markus Landthaler

Subjects

RNA, Untranslated, PROTEINS, Molecular Sequence Data, RNA-binding protein, Computational biology, Regulatory Sequences, Ribonucleic Acid, Biology, PAR-CLIP, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, 0302 clinical medicine, Humans, Point Mutation, 030304 developmental biology, Ribonucleoprotein, Genetics, 0303 health sciences, SYSBIO, Base Sequence, Biochemistry, Genetics and Molecular Biology(all), RNA-Binding Proteins, RNA, Nucleosides, 3. Good health, Ribonomics, HITS-CLIP, MicroRNAs, Cross-Linking Reagents, Genetic Techniques, Regulatory sequence, 030220 oncology & carcinogenesis, Sequence Alignment, ICLIP

Abstract

SummaryRNA transcripts are subject to posttranscriptional gene regulation involving hundreds of RNA-binding proteins (RBPs) and microRNA-containing ribonucleoprotein complexes (miRNPs) expressed in a cell-type dependent fashion. We developed a cell-based crosslinking approach to determine at high resolution and transcriptome-wide the binding sites of cellular RBPs and miRNPs. The crosslinked sites are revealed by thymidine to cytidine transitions in the cDNAs prepared from immunopurified RNPs of 4-thiouridine-treated cells. We determined the binding sites and regulatory consequences for several intensely studied RBPs and miRNPs, including PUM2, QKI, IGF2BP1-3, AGO/EIF2C1-4 and TNRC6A-C. Our study revealed that these factors bind thousands of sites containing defined sequence motifs and have distinct preferences for exonic versus intronic or coding versus untranslated transcript regions. The precise mapping of binding sites across the transcriptome will be critical to the interpretation of the rapidly emerging data on genetic variation between individuals and how these variations contribute to complex genetic diseases.

Published

2010

14. Modeling Protein-RNA Complexes

Author

Julie Bernauer, Adelene Sim, and Jinglin Chen

Subjects

Flexibility (engineering), Computer science, business.industry, Biophysics, RNA, Sampling (statistics), Bioinformatics, Machine learning, computer.software_genre, Identification (information), Ranking, Benchmark (computing), Artificial intelligence, business, Decoy, ICLIP, computer

Abstract

The advent of high-throughput technologies has led to the identification of many new in vivo protein-RNA interactions. While much work has been done to characterize these interactions based on secondary structures of RNA, less effort has been placed to identify three-dimensional (3D) motifs of RNA that are essential for protein-RNA recognition. This discrepancy in effort is not for lack of interest, but rather arises due to the significant challenges and complexities in modeling protein-RNA complexes in 3D. The challenges, in general, are twofold: i) sampling possible protein-RNA interactions and ii) ranking models based on their likelihood to exist in the cell; this process is also known as “scoring”. The former is often intractable - the flexibility of RNA adds significant complexity to the modeling process - but sampling search space can be reduced with experimental input of possible interacting regions (e.g. from HITS-CLIP, PAR-CLIP or iCLIP data). We designed a new 3D modeling protocol to generate reasonable models of protein-RNA complexes, by accounting for protein flexibility (using torsional angle sampling) and RNA flexibility (using previously developed “natural moves” for RNA). Using this protocol, we are able to obtain native-like protein-RNA interactions, even when modeling RNA structures starting from the unbound conformation. As expected, including experimental constraints significantly improves sampling efficiency. Because our protein-RNA models are robust and diverse, they serve as benchmark decoy datasets for evaluating protein-RNA scoring functions - the second aforementioned challenge. With our decoy set we are able to identify constructive features of different scoring functions, and also highlight limitations requiring further development. With improved scoring functions and known interacting regions probed from experiments, we foresee that our protocol can be used to effectively model novel protein-RNA complexes in 3D.

Published

2016