Your search keyword '"S. Chan Baek"' showing total 6 results

1. ERH facilitates microRNA maturation through the interaction with the N-terminus of DGCR8

Author

Jeesoo Kim, S. Chan Baek, Suman Wang, V. Narry Kim, Jihye Yang, Siyuan Shen, Fudong Li, Yunyu Shi, Jong-Seo Kim, Kijun Kim, S. Chul Kwon, and Harim Jang

Subjects

AcademicSubjects/SCI00010, Protein Conformation, DGCR8, Cell Cycle Proteins, Primary transcript, Microprocessor complex, 03 medical and health sciences, 0302 clinical medicine, Protein structure, microRNA, RNA and RNA-protein complexes, Genetics, Humans, Ribonuclease III, RNA Processing, Post-Transcriptional, Enhancer, Drosha, 030304 developmental biology, 0303 health sciences, biology, RNA-Binding Proteins, HCT116 Cells, Cell biology, MicroRNAs, HEK293 Cells, biology.protein, K562 Cells, 030217 neurology & neurosurgery, Protein Binding, Transcription Factors

Abstract

The microprocessor complex cleaves the primary transcript of microRNA (pri-miRNA) to initiate miRNA maturation. Microprocessor is known to consist of RNase III DROSHA and dsRNA-binding DGCR8. Here, we identify Enhancer of Rudimentary Homolog (ERH) as a new component of Microprocessor. Through a crystal structure and biochemical experiments, we reveal that ERH uses its hydrophobic groove to bind to a conserved region in the N-terminus of DGCR8, in a 2:2 stoichiometry. Knock-down of ERH or deletion of the DGCR8 N-terminus results in a reduced processing of suboptimal pri-miRNAs in polycistronic miRNA clusters. ERH increases the processing of suboptimal pri-miR-451 in a manner dependent on its neighboring pri-miR-144. Thus, the ERH dimer may mediate ‘cluster assistance’ in which Microprocessor is loaded onto a poor substrate with help from a high-affinity substrate in the same cluster. Our study reveals a role of ERH in the miRNA biogenesis pathway.

Published

2020

2. A quantitative map of human primary microRNA processing sites

Author

Carolien Bastiaanssen, Kijun Kim, Young-Yoon Lee, Haedong Kim, V. Narry Kim, S. Chan Baek, and Jeesoo Kim

Subjects

Ribonuclease III, Primary MicroRNA, Binding Sites, biology, Serine-Arginine Splicing Factors, DGCR8, Genome, Human, Processing efficiency, Cell Biology, Computational biology, Primary transcript, MiRBase, MicroRNAs, HEK293 Cells, microRNA, biology.protein, Humans, RNA Interference, RNA Processing, Post-Transcriptional, Molecular Biology, Drosha

Abstract

Summary Maturation of canonical microRNA (miRNA) is initiated by DROSHA that cleaves the primary transcript (pri-miRNA). More than 1,800 miRNA loci are annotated in humans, but it remains largely unknown whether and at which sites pri-miRNAs are cleaved by DROSHA. Here, we performed in vitro processing on a full set of human pri-miRNAs (miRBase version 21) followed by sequencing. This comprehensive profiling enabled us to classify miRNAs on the basis of DROSHA dependence and map their cleavage sites with respective processing efficiency measures. Only 758 pri-miRNAs are confidently processed by DROSHA, while the majority may be non-canonical or false entries. Analyses of the DROSHA-dependent pri-miRNAs show key cis-elements for processing. We observe widespread alternative processing and unproductive cleavage events such as “nick” or “inverse” processing. SRSF3 is a broad-acting auxiliary factor modulating alternative processing and suppressing unproductive processing. The profiling data and methods developed in this study will allow systematic analyses of miRNA regulation.

Published

2021

3. L1 retrotransposons exploit RNA m6A modification as an evolutionary driving force

Author

Sung-Yeon Hwnag, Hyunchul Jung, Seyoung Mun, Sungwon Lee, S. Chan Baek, Hyungseok Moon, Baekgyu Kim, Yongkuk Choi, Young-Hyun Go, Wanxiangfu Tang, Jongsu Choi, Jung Kyoon Choi, Hyuk-Jin Cha, Hye Yoon Park, Ping Liang, V. Narry Kim, Kyudong Han, and Kwangseog Ahn

Abstract

L1 retrotransposons can pose a threat to genome integrity. The host has evolved to restrict L1 replication. However, mechanisms underlying L1 propagation out of the host surveillance remains unclear. Here, we propose a novel survival strategy of L1, which exploits RNA m6A modification. We discover that m6A ‘writer’ METTL3 facilitates L1 retrotransposition, whereas m6A ‘eraser’ ALKBH5 suppresses it. The essential m6A cluster that is located on L1 5′ UTR serves as a docking site for eukaryotic initiation factor 3 (eIF3), enhances translational efficiency and promotes the formation of L1 ribonucleoprotein. Furthermore, through the comparative analysis of human- and primate-specific L1 lineages, we find that the most functional m6A motif-containing L1s have been positively selected and became a distinctive feature of evolutionarily young L1s. Thus, our findings demonstrate that L1 retrotransposons hijack RNA m6A modification system for its successful replication.

Published

2020

4. ERH as a component of the Microprocessor facilitates the maturation of suboptimal microRNAs

Author

Jihye Yang, V. Narry Kim, Jong-Seo Kim, S. Chul Kwon, S. Chan Baek, Harim Jang, and Jeesoo Kim

Subjects

Microprocessor complex, Gene knockdown, biology, DGCR8, Chemistry, microRNA, biology.protein, Ribonuclease III, Primary transcript, Enhancer, Drosha, Cell biology

Abstract

The Microprocessor complex cleaves the primary transcript of microRNA (pri-miRNA) to initiate miRNA maturation. Microprocessor is known to consist of RNase III DROSHA and dsRNA-binding DGCR8. Here we identify Enhancer of Rudimentary Homolog (ERH) as a new component of the Microprocessor. ERH binds to a conserved region in the N-terminus of DGCR8. Knockdown of ERH or deletion of the DGCR8 N-terminus results in a decrease of processing of primary miRNAs with suboptimal hairpin structures that reside in polycistronic miRNA clusters. ERH increases the processing of suboptimal pri-miR-451 in a manner dependent on its neighboring pri-miR-144. Thus, the ERH dimer may mediate “cluster assistance” in which the Microprocessor is loaded onto a poor substrate with help from a high-affinity substrate in the same cluster. Our study reveals a role of ERH in the miRNA pathway.

Published

2020

5. Genomic Clustering Facilitates Nuclear Processing of Suboptimal Pri-miRNA Loci

Author

S. Chan Baek, V. Narry Kim, Eric C. Lai, Renfu Shang, Boseon Kim, and Kijun Kim

Subjects

Ribonuclease III, Operon, DGCR8, Computational biology, Biology, Article, Terminal loop, 03 medical and health sciences, 0302 clinical medicine, microRNA, Humans, RNA Processing, Post-Transcriptional, Molecular Biology, Drosha, 030304 developmental biology, Cell Nucleus, 0303 health sciences, Tethering, RNA-Binding Proteins, Genomics, Cell Biology, MicroRNAs, biology.protein, 030217 neurology & neurosurgery, Biogenesis

Abstract

Nuclear processing of most miRNAs is mediated by Microprocessor, comprised of RNase III enzyme Drosha and its cofactor DGCR8. Here, we uncover a hidden layer of Microprocessor regulation via studies of Dicer-independent mir-451, which is clustered with canonical mir-144. Although mir-451 is fully dependent on Drosha/DGCR8, its short stem and small terminal loop render it an intrinsically weak Microprocessor substrate. Thus, it must reside within a cluster for normal biogenesis, although the identity and orientation of its neighbor are flexible. We use DGCR8 tethering assays and operon structure-function assays to demonstrate that local recruitment and transfer of Microprocessor enhances suboptimal substrate processing. This principle applies more broadly since genomic analysis indicates suboptimal canonical miRNAs are enriched in operons, and we validate several of these experimentally. Proximity-based enhancement of suboptimal hairpin processing provides a rationale for genomic retention of certain miRNA operons, and may explain preferential evolutionary emergence of miRNA operons.

Published

2020

6. Molecular Basis for the Single-Nucleotide Precision of Primary microRNA Processing

Author

S. Chan Baek, Jae Sung Woo, Yeon Gil Choi, Jihye Yang, Young-suk Lee, V. Narry Kim, and S. Chul Kwon

Subjects

Models, Molecular, Ribonuclease III, DGCR8, Computational biology, Cleavage (embryo), Substrate Specificity, 03 medical and health sciences, Structure-Activity Relationship, 0302 clinical medicine, microRNA, Gene silencing, Humans, Protein Interaction Domains and Motifs, Nucleotide Motifs, RNA Processing, Post-Transcriptional, Molecular Biology, Drosha, 030304 developmental biology, 0303 health sciences, biology, Rational design, High-Throughput Nucleotide Sequencing, RNA-Binding Proteins, Cell Biology, HCT116 Cells, MicroRNAs, HEK293 Cells, biology.protein, Nucleic Acid Conformation, 030217 neurology & neurosurgery, Biogenesis

Abstract

Microprocessor, composed of DROSHA and its cofactor DGCR8, initiates microRNA (miRNA) biogenesis by processing the primary transcripts of miRNA (pri-miRNAs). Here we investigate the mechanism by which Microprocessor selects the cleavage site with single-nucleotide precision, which is crucial for the specificity and functionality of miRNAs. By testing ∼40,000 pri-miRNA variants, we find that for some pri-miRNAs the cleavage site is dictated mainly by the mGHG motif embedded in the lower stem region of pri-miRNA. Structural modeling and deep-sequencing-based complementation experiments show that the double-stranded RNA-binding domain (dsRBD) of DROSHA recognizes mGHG to place the catalytic center in the appropriate position. The mGHG motif as well as the mGHG-recognizing residues in DROSHA dsRBD are conserved across eumetazoans, suggesting that this mechanism emerged in an early ancestor of the animal lineage. Our findings provide a basis for the understanding of miRNA biogenesis and rational design of accurate small-RNA-based gene silencing.

Published

2018