Your search keyword '"Bao, Xichen"' showing total 8 results

1. Cryo-EM structures of Thogoto virus polymerase reveal unique RNA transcription and replication mechanisms among orthomyxoviruses.

Author

Xue L, Chang T, Li Z, Wang C, Zhao H, Li M, Tang P, Wen X, Yu M, Wu J, Bao X, Wang X, Gong P, He J, Chen X, and Xiong X

Subjects

Humans, RNA, Messenger metabolism, RNA, Messenger genetics, Viral Proteins metabolism, Viral Proteins genetics, Viral Proteins chemistry, Viral Proteins ultrastructure, Cryoelectron Microscopy, Thogotovirus genetics, Thogotovirus metabolism, Thogotovirus ultrastructure, RNA, Viral metabolism, RNA, Viral genetics, Virus Replication genetics, Transcription, Genetic

Abstract

Influenza viruses and thogotoviruses account for most recognized orthomyxoviruses. Thogotoviruses, exemplified by Thogoto virus (THOV), are capable of infecting humans using ticks as vectors. THOV transcribes mRNA without the extraneous 5' end sequences derived from cap-snatching in influenza virus mRNA. Here, we report cryo-EM structures to characterize THOV polymerase RNA synthesis initiation and elongation. The structures demonstrate that THOV RNA transcription and replication are able to start with short dinucleotide primers and that the polymerase cap-snatching machinery is likely non-functional. Triggered by RNA synthesis, asymmetric THOV polymerase dimers can form without the involvement of host factors. We confirm that, distinctive from influenza viruses, THOV-polymerase RNA synthesis is weakly dependent of the host factors ANP32A/B/E in human cells. This study demonstrates varied mechanisms in RNA synthesis and host factor utilization among orthomyxoviruses, providing insights into the mechanisms behind thogotoviruses' broad-infectivity range., (© 2024. The Author(s).)

Published

2024

2. Capture of the newly transcribed RNA interactome using click chemistry.

Author

Guo X, Tariq M, Lai Y, Kanwal S, Lv Y, Wang X, Li N, Jiang M, Meng J, Hu J, Yuan J, Luo Z, Ward C, Volpe G, Wang D, Yin M, Qin B, Zhang B, Bao X, and Esteban MA

Subjects

Humans, Biotinylation, Proteomics methods, Transcription, Genetic, High-Throughput Nucleotide Sequencing methods, Click Chemistry methods, RNA-Binding Proteins metabolism, RNA metabolism, RNA chemistry

Abstract

Application of synthetic nucleoside analogues to capture newly transcribed RNAs has unveiled key features of RNA metabolism. Whether this approach could be adapted to isolate the RNA-bound proteome (RNA interactome) was, however, unexplored. We have developed a new method (capture of the newly transcribed RNA interactome using click chemistry, or RICK) for the systematic identification of RNA-binding proteins based on the incorporation of 5-ethynyluridine into newly transcribed RNAs followed by UV cross-linking and click chemistry-mediated biotinylation. The RNA-protein adducts are then isolated by affinity capture using streptavidin-coated beads. Through high-throughput RNA sequencing and mass spectrometry, the RNAs and proteins can be elucidated globally. A typical RICK experimental procedure takes only 1 d, excluding the steps of cell preparation, 5-ethynyluridine labeling, validation (silver staining, western blotting, quantitative reverse-transcription PCR (qRT-PCR) or RNA sequencing (RNA-seq)) and proteomics. Major advantages of RICK are the capture of RNA-binding proteins interacting with any type of RNA and, particularly, the ability to discern between newly transcribed and steady-state RNAs through controlled labeling. Thanks to its versatility, RICK will facilitate the characterization of the total and newly transcribed RNA interactome in different cell types and conditions., (© 2021. Springer Nature Limited.)

Published

2021

3. JMJD3 acts in tandem with KLF4 to facilitate reprogramming to pluripotency.

Author

Huang Y, Zhang H, Wang L, Tang C, Qin X, Wu X, Pan M, Tang Y, Yang Z, Babarinde IA, Lin R, Ji G, Lai Y, Xu X, Su J, Wen X, Satoh T, Ahmed T, Malik V, Ward C, Volpe G, Guo L, Chen J, Sun L, Li Y, Huang X, Bao X, Gao F, Liu B, Zheng H, Jauch R, Lai L, Pan G, Chen J, Testa G, Akira S, Hu J, Pei D, Hutchins AP, Esteban MA, and Qin B

Subjects

Animals, Catalysis, Cell Proliferation, Cellular Senescence, Demethylation, Enhancer Elements, Genetic genetics, Epithelial Cells metabolism, Fibroblasts cytology, Fibroblasts metabolism, Gene Expression Regulation, Developmental, Genome, Histones metabolism, Kruppel-Like Factor 4, Lysine metabolism, Mice, Models, Biological, Promoter Regions, Genetic, Transcriptional Activation genetics, Cellular Reprogramming, Jumonji Domain-Containing Histone Demethylases metabolism, Kruppel-Like Transcription Factors metabolism, Pluripotent Stem Cells cytology, Pluripotent Stem Cells metabolism

Abstract

The interplay between the Yamanaka factors (OCT4, SOX2, KLF4 and c-MYC) and transcriptional/epigenetic co-regulators in somatic cell reprogramming is incompletely understood. Here, we demonstrate that the histone H3 lysine 27 trimethylation (H3K27me3) demethylase JMJD3 plays conflicting roles in mouse reprogramming. On one side, JMJD3 induces the pro-senescence factor Ink4a and degrades the pluripotency regulator PHF20 in a reprogramming factor-independent manner. On the other side, JMJD3 is specifically recruited by KLF4 to reduce H3K27me3 at both enhancers and promoters of epithelial and pluripotency genes. JMJD3 also promotes enhancer-promoter looping through the cohesin loading factor NIPBL and ultimately transcriptional elongation. This competition of forces can be shifted towards improved reprogramming by using early passage fibroblasts or boosting JMJD3's catalytic activity with vitamin C. Our work, thus, establishes a multifaceted role for JMJD3, placing it as a key partner of KLF4 and a scaffold that assists chromatin interactions and activates gene transcription.

Published

2020

4. MyoD induced enhancer RNA interacts with hnRNPL to activate target gene transcription during myogenic differentiation.

Author

Zhao Y, Zhou J, He L, Li Y, Yuan J, Sun K, Chen X, Bao X, Esteban MA, Sun H, and Wang H

Subjects

Animals, Cell Differentiation genetics, Cell Line, Male, Mice, Muscle, Skeletal cytology, Muscle, Skeletal growth & development, Myoblasts physiology, Promoter Regions, Genetic genetics, RNA, Messenger metabolism, Transcription, Genetic, Enhancer Elements, Genetic genetics, Gene Expression Regulation, Developmental, Heterogeneous-Nuclear Ribonucleoprotein L genetics, Muscle Development genetics, MyoD Protein metabolism, RNA, Messenger genetics

Abstract

Emerging evidence supports roles of enhancer RNAs (eRNAs) in regulating target gene. Here, we study eRNA regulation and function during skeletal myoblast differentiation. We provide a panoramic view of enhancer transcription and categorization of eRNAs. Master transcription factor MyoD is crucial in activating eRNA production. Super enhancer (se) generated seRNA-1 and -2 promote myogenic differentiation in vitro and in vivo. seRNA-1 regulates expression levels of two nearby genes, myoglobin (Mb) and apolipoprotein L6 (Apol6), by binding to heterogeneous nuclear ribonucleoprotein L (hnRNPL). A CAAA tract on seRNA-1 is essential in mediating seRNA-1/hnRNPL binding and function. Disruption of seRNA-1-hnRNPL interaction attenuates Pol II and H3K36me3 deposition at the Mb locus, in coincidence with the reduction of its transcription. Furthermore, analyses of hnRNPL binding transcriptome-wide reveal its association with eRNAs is a general phenomenon in multiple cells. Collectively, we propose that eRNA-hnRNPL interaction represents a mechanism contributing to target mRNA activation.

Published

2019

5. Capturing the interactome of newly transcribed RNA.

Author

Bao X, Guo X, Yin M, Tariq M, Lai Y, Kanwal S, Zhou J, Li N, Lv Y, Pulido-Quetglas C, Wang X, Ji L, Khan MJ, Zhu X, Luo Z, Shao C, Lim DH, Liu X, Li N, Wang W, He M, Liu YL, Ward C, Wang T, Zhang G, Wang D, Yang J, Chen Y, Zhang C, Jauch R, Yang YG, Wang Y, Qin B, Anko ML, Hutchins AP, Sun H, Wang H, Fu XD, Zhang B, and Esteban MA

Subjects

Animals, Embryonic Stem Cells cytology, Embryonic Stem Cells metabolism, HeLa Cells, High-Throughput Nucleotide Sequencing methods, Humans, Mass Spectrometry methods, Mice, Protein Interaction Maps, RNA genetics, RNA-Binding Proteins genetics, Uridine analogs & derivatives, Uridine chemistry, Click Chemistry methods, Proteome metabolism, RNA metabolism, RNA-Binding Proteins metabolism

Abstract

We combine the labeling of newly transcribed RNAs with 5-ethynyluridine with the characterization of bound proteins. This approach, named capture of the newly transcribed RNA interactome using click chemistry (RICK), systematically captures proteins bound to a wide range of RNAs, including nascent RNAs and traditionally neglected nonpolyadenylated RNAs. RICK has identified mitotic regulators amongst other novel RNA-binding proteins with preferential affinity for nonpolyadenylated RNAs, revealed a link between metabolic enzymes/factors and nascent RNAs, and expanded the known RNA-bound proteome of mouse embryonic stem cells. RICK will facilitate an in-depth interrogation of the total RNA-bound proteome in different cells and systems.

Published

2018

6. Linc-YY1 promotes myogenic differentiation and muscle regeneration through an interaction with the transcription factor YY1.

Author

Zhou L, Sun K, Zhao Y, Zhang S, Wang X, Li Y, Lu L, Chen X, Chen F, Bao X, Zhu X, Wang L, Tang LY, Esteban MA, Wang CC, Jauch R, Sun H, and Wang H

Subjects

Animals, Cell Line, Embryo, Mammalian, Gene Expression Regulation physiology, Humans, Male, Mice, Mice, Inbred mdx, RNA, Long Noncoding genetics, Regeneration physiology, YY1 Transcription Factor genetics, Muscle Development physiology, RNA, Long Noncoding metabolism, YY1 Transcription Factor metabolism

Abstract

Little is known how lincRNAs are involved in skeletal myogenesis. Here we describe the discovery of Linc-YY1 from the promoter of the transcription factor (TF) Yin Yang 1 (YY1) gene. We demonstrate that Linc-YY1 is dynamically regulated during myogenesis in vitro and in vivo. Gain or loss of function of Linc-YY1 in C2C12 myoblasts or muscle satellite cells alters myogenic differentiation and in injured muscles has an impact on the course of regeneration. Linc-YY1 interacts with YY1 through its middle domain, to evict YY1/Polycomb repressive complex (PRC2) from target promoters, thus activating the gene expression in trans. In addition, Linc-YY1 also regulates PRC2-independent function of YY1. Finally, we identify a human Linc-YY1 orthologue with conserved function and show that many human and mouse TF genes are associated with lincRNAs that may modulate their activity. Altogether, we show that Linc-YY1 regulates skeletal myogenesis and uncover a previously unappreciated mechanism of gene regulation by lincRNA.

Published

2015

7. Generation of integration-free neural progenitor cells from cells in human urine.

Author

Wang L, Wang L, Huang W, Su H, Xue Y, Su Z, Liao B, Wang H, Bao X, Qin D, He J, Wu W, So KF, Pan G, and Pei D

Subjects

Animals, Animals, Newborn, Biomarkers metabolism, Blotting, Western, Gene Expression Profiling, Humans, Immunoenzyme Techniques, Neural Stem Cells transplantation, Neuroglia cytology, Oligonucleotide Array Sequence Analysis, RNA, Messenger genetics, Rats, Real-Time Polymerase Chain Reaction, Reverse Transcriptase Polymerase Chain Reaction, Stem Cell Transplantation, Urine chemistry, Brain cytology, Cell Differentiation, Cellular Reprogramming, Epithelial Cells cytology, Neural Stem Cells cytology, Tissue Engineering methods, Urine cytology

Abstract

Human neural stem cells hold great promise for research and therapy in neural disease. We describe the generation of integration-free and expandable human neural progenitor cells (NPCs). We combined an episomal system to deliver reprogramming factors with a chemically defined culture medium to reprogram epithelial-like cells from human urine into NPCs (hUiNPCs). These transgene-free hUiNPCs can self-renew and can differentiate into multiple functional neuronal subtypes and glial cells in vitro. Although functional in vivo analysis is still needed, we report that the cells survive and differentiate upon transplant into newborn rat brain.

Published

2013

8. Generation of human induced pluripotent stem cells from urine samples.

Author

Zhou T, Benda C, Dunzinger S, Huang Y, Ho JC, Yang J, Wang Y, Zhang Y, Zhuang Q, Li Y, Bao X, Tse HF, Grillari J, Grillari-Voglauer R, Pei D, and Esteban MA

Subjects

Cell Culture Techniques, Humans, Cell Separation methods, Epithelial Cells cytology, Induced Pluripotent Stem Cells cytology, Kidney cytology, Urine cytology

Abstract

Human induced pluripotent stem cells (iPSCs) have been generated with varied efficiencies from multiple tissues. Yet, acquiring donor cells is, in most instances, an invasive procedure that requires laborious isolation. Here we present a detailed protocol for generating human iPSCs from exfoliated renal epithelial cells present in urine. This method is advantageous in many circumstances, as the isolation of urinary cells is simple (30 ml of urine are sufficient), cost-effective and universal (can be applied to any age, gender and race). Moreover, the entire procedure is reasonably quick--around 2 weeks for the urinary cell culture and 3-4 weeks for the reprogramming--and the yield of iPSC colonies is generally high--up to 4% using retroviral delivery of exogenous factors. Urinary iPSCs (UiPSCs) also show excellent differentiation potential, and thus represent a good choice for producing pluripotent cells from normal individuals or patients with genetic diseases, including those affecting the kidney.

Published

2012