Reference: Makino S, et al. (2015)
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Abstract
The CCR4-NOT complex, the major deadenylase in eukaryotes, plays crucial roles in gene expression at the levels of transcription, mRNA decay, and protein degradation. GW182/TNRC6 proteins, which are core components of the microRNA-induced silencing complex in animals, stimulate deadenylation and repress translation via recruitment of the CCR4-NOT complex. Here we report a heterologous experimental system that recapitulates the recruitment of CCR4-NOT complex by TNRC6 in S. cerevisiae. Using this system, we characterize conserved functions of the CCR4-NOT complex. The complex stimulates degradation of mRNA from the 5' end by Xrn1, in a manner independent of both translation and deadenylation. This degradation pathway is probably conserved in miRNA-mediated gene silencing in zebrafish. Furthermore, the mRNA fate modulators Dhh1 and Pat1 redundantly stimulate mRNA decay, but both factors are required for poly(A) tail-independent translation repression by tethered TNRC6A. Our tethering-based reconstitution system reveals that the conserved architecture of Not1/CNOT1 provides a binding surface for TNRC6, thereby connecting microRNA-induced silencing complex to the decapping machinery as well as the translation apparatus.
- Reference Type
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Journal Article |
Research Support, Non-U.S. Gov't
- Authors
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Makino S,
Mishima Y,
Inoue K,
Inada T
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- PAT1 | XRN1 | DHH1 | CCR4-NOT mRNA deadenylase complex
Gene Ontology Annotations
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| Interactor | Interactor | Assay | Annotation | Action | Modification |
| CDC39 | DHH1 | Affinity Capture-Western | manually curated | Hit-Bait | No Modification |
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