Predicting effective microRNA target sites in mammalian mRNAs

Agarwal, Vikram; Bell, George W.; Nam, Jin Wu; Bartel, David P.

doi:10.7554/elife.05005

Cited by 5,858 publications

(5,257 citation statements)

References 122 publications

(355 reference statements)

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“…Hexokinase II Is a Direct Target of the let-7a-1/let-7d/ let-7f-1 Cluster and Promotes B Cell Glycolysis To further investigate the underlying mechanism through which the let-7adf cluster regulates glycolysis in B cells, we screened for messenger RNAs with 3 0 untranslated regions (UTRs) that could be putative targets of let-7d, using the TargetScan algorithm predictions (Agarwal et al, 2015). We identified Hk2 and Pdk1 (pyruvate dehydrogenase kinase 1), critical enzymes in the glycolysis pathway, as potential targets of let-7d in B cells ( Figure 4A; only the Hk2 3 0 UTR is shown).…”

Section: Comprehensive Repression Of All Let-7 Mirnas Enhances Igm Prmentioning

confidence: 99%

Let-7 Suppresses B Cell Activation through Restricting the Availability of Necessary Nutrients

et al. 2018

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Section: Comprehensive Repression Of All Let-7 Mirnas Enhances Igm Prmentioning

confidence: 99%

Let-7 Suppresses B Cell Activation through Restricting the Availability of Necessary Nutrients

et al. 2018

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“…It predicts biological targets of miRNAs by searching for the presence of conserved 8mer, 7mer, and 6mer sites that match the seed region of each miRNA but there is also an optional search for poorly conserved sites. Its development included also scoring for binding sites with mismatches in the seed region that are compensated by 3' end pairing (Friedman et al, 2009) an improved quantitative model of canonical targeting (Agarwal et al, 2015) and addition other features. The current version considers a site type and fourteen other features and, according to authors, it outperforms other tools and matches high-throughput in vivo crosslinking approaches (Agarwal et al, 2015).…”

Section: Targetscan (Http://wwwtargetscanorg/vert_71/)mentioning

confidence: 99%

Literature review of baseline information to support the risk assessment of RNAi‐based GM plants

Pačes

Nič²,

Novotný³

et al. 2017

EFSA Supporting Publications

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This report is the outcome of an EFSA procurement aiming at investigating and summarising the state of knowledge on (I) the mode-of-action of dsRNA and miRNA pathways, (II) the potential for nontarget gene regulation by dsRNA-derived siRNAs or miRNAs, (III) the determination of siRNA pools in plant tissues and the importance of individual siRNAs for silencing. The report is based on a comprehensive and systematic literature search, starting with the identification and retrieval of~190,000 publications related to the research area and further filtered down with keywords to produce focused collections used for subsequent screening of titles and abstracts. The report is comprised of an (I) Introduction to the field of small RNAs, (II) a Data and Methodologies section containing strategies used for literature search and study selection, and (III) the Results of the literature review organized according to the three main procurement tasks. The outcome of the first task reviews dsRNA and miRNA pathways in mammals (including humans), birds, fish, arthropods, annelids, molluscs, nematodes, and plants. Eight taxon-dedicated chapters are based on~1,400 cumulative references chosen from~10,000 inspected titles and abstracts. We review conserved and divergent aspects of small RNA pathways and dsRNA responses in animals and plants including structure and function of key proteins as well as four basic mechanisms: genome-encoded posttranscriptional regulations (miRNA), degradation of RNAs by short interfering RNA pools generated from long dsRNA (RNAi), transcriptional silencing, and sequence-independent responses to dsRNA. The outcome of the second task focuses on base pairing between small RNAs and their target RNAs and predictability of biological effects of small RNAs in animals and plants. The outcome of the last task reviews methodology, siRNA pools, and movement of small RNAs in plants. Potential transfer of small RNAs between species and circulating miRNAs in mammals is described in the final chapter.

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“…To predict the target gene of miR-149, bioinformatics software (TargetScan 7.1) was used (17). As demonstrated in Fig.…”

Section: Sp1 Was a Direct Target Gene Of Mir-149 In Vitromentioning

confidence: 99%

MicroRNA-149 targets specificity protein 1 to suppress human tongue squamous cell carcinoma cell proliferation and motility

Chen

2016

Oncology Letters

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Predicting effective microRNA target sites in mammalian mRNAs

Cited by 5,858 publications

References 122 publications

Let-7 Suppresses B Cell Activation through Restricting the Availability of Necessary Nutrients

Let-7 Suppresses B Cell Activation through Restricting the Availability of Necessary Nutrients

Literature review of baseline information to support the risk assessment of RNAi‐based GM plants

MicroRNA-149 targets specificity protein 1 to suppress human tongue squamous cell carcinoma cell proliferation and motility

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