Your search keyword '"Xiaohui Xie"' showing total 5 results

1. Transcriptome-wide analyses of CstF64–RNA interactions in global regulation of mRNA alternative polyadenylation.

Author

Chengguo Yao, Biesinger, Jacob, Ji Wan, Lingjie Weng, Vi Xing, Xiaohui Xie, and Yongsheng Shi

Subjects

RNA, ADENYLATION (Biochemistry), GENETIC transcription, NUCLEOTIDES, IMMUNOPRECIPITATION, ULTRAVIOLET radiation, CROSSLINKING (Polymerization)

Abstract

Cleavage stimulation factor 64 kDa (CstF64) is an essential premRNA 3' processing factor and an important regulator of alternative polyadenylation (APA). Here we characterized CstF64-RNA interactions in vivo at the transcriptome level and investigated the role of CstF64 in global APA regulation through individual nucleotide resolution UV crosslinking and immunoprecipitation sequencing and direct RNA sequencing analyses. We observed highly specific CstF64-RNA interactions at poly(A) sites (PASs). and we provide evidence that such interactions are widely variable in affinity and may be differentially required for PAS recognition. Depletion of CstF64 by RNAi has a relatively small effect on the global APA profile, but codepletion of the CstF64 paralog CstF64c leads to greater APA changes, most of which are characterized by the increased relative use of distal PASs. Finally, we found that CstF64 binds to thousands of dormant intronic PASs that are suppressed, at least in part, by U1 small nuclear ribonucleoproteins. Taken together, our findings provide insight into the mechanisms of PAS recognition and identify CstF64 as an important global regulator of APA. [ABSTRACT FROM AUTHOR]

Published

2012

2. Genome-wide analysis of SREBP-1 binding in mouse liver chromatin reveals a preference for promoter proximal binding to a new motif.

Author

Young-Kyo Seo, Hansook Kim Chong, Infante, Aniello M., Seung-Soon Im, Xiaohui Xie, and Osborne, Timothy F.

Subjects

GENE mapping, NUCLEOTIDE sequence, GENOMES, CARRIER proteins, CHROMATIN, IMMUNE serums

Abstract

Lipid homeostasis in vertebrates is regulated by 3 sterol regulatory element binding protein (SREBP) isoforms. Here, we identify targets of SREBP-1 in mammalian liver using chromatin immunoprecipitation-high-throughput DNA sequencing. Antisera to SREBP-1 were used with liver chromatin from mice fed a high-carbohydrate diet after a fast, which leads to superinduction of hepatic SREBP-lc expression. SREBP-1-DNA complexes were subjected to massive parallel DNA sequencing using the Illumina Genome Analyzer II, resulting in 5.7 million sequence reads. Mapping these reads to the mouse reference genome identified 426 peaks of SREBP-1 binding vs. a control antibody. These binding peaks show a striking enrichment in proximal promoter regions, with 52% located within 1 kb upstream of a transcription start site. A previously undescribed sequence motif (5′-ACTACANNTCCC-3′) was present in 76% of the total peaks, and we show that it is a functional SREBP-1 response element. Our analysis also reveals that an Spi consensus site is present as a "coregulatory" motif in 50% of the SREBP-1 binding peaks, consistent with previous functional studies. SREBP-1 bound not only to many well-characterized SREBP-1 target genes but to several other previously unknown targets in lipid and carbohydrate metabolism as well as many putative target genes in other diverse biological pathways. [ABSTRACT FROM AUTHOR]

Published

2009

3. Distinguishing protein-coding and noncoding genes in the human genome.

Author

Clamp, Michele, Fry, Ben, Kamal, Mike, Xiaohui Xie, Cuff, James, Lin, Michael F., Kellis, Manolis, Lindblad-Toh, Kerstin, and Lander, Eric S.

Subjects

HUMAN genome, RNA synthesis, GENES, PROTEIN analysis, MICE, ANIMAL models in research

Abstract

Although the Human Genome Project was completed 4 years ago, the catalog of human protein-coding genes remains a matter of controversy. Current catalogs list a total of ≈24,500 putative protein-coding genes. It is broadly suspected that a large fraction of these entries are functionally meaningless ORFs present by chance in RNA transcripts, because they show no evidence of evolutionary conservation with mouse or dog. However, there is currently no scientific justification for excluding ORFs simply because they fail to show evolutionary conservation: the alternative hypothesis is that most of these ORFs are actually valid human genes that reflect gene innovation in the primate lineage or gene loss in the other lineages. Here, we reject this hypothesis by carefully analyzing the nonconserved ORFs—specifically, their properties in other primates. We show that the vast majority of these ORFs are random occurrences. The analysis yields, as a by-product, a major revision of the current human catalogs, cutting the number of protein-coding genes to ≈20,500. Specifically, it suggests that nonconserved ORFs should be added to the human gene catalog only if there is clear evidence of an encoded protein. It also provides a principled methodology for evaluating future proposed additions to the human gene catalog. Finally, the results indicate that there has been relatively little true innovation in mammalian protein-coding genes. [ABSTRACT FROM AUTHOR]

Published

2007

4. Systematic discovery of regulatory motifs in conserved regions of the human genome, including thousands of CTCF insulator sites.

Author

Xiaohui Xie, Mikkelsen, Tarjei S., Gnirke, Andreas, Lindblad-Toh, Kerstin, Kellis, Manolis, and Lander, Eric S.

Subjects

*HUMAN genome, *HUMAN chromosomes, *HEREDITY, *GENE expression, *HUMAN genetics

Abstract

Conserved noncoding elements (CNEs) constitute the majority of sequences under purifying selection in the human genome, yet their function remains largely unknown. Experimental evidence suggests that many of these elements play regulatory roles, but little is known about regulatory motifs contained within them. Here we describe a systematic approach to discover and characterize regulatory motifs within mammalian CNEs by searching for long motifs (12-22 nt) with significant enrichment in CNEs and studying their biochemical and genomic properties. Our analysis identifies 233 long motifs (LMs), matching a total of ≈60,000 conserved instances across the human genome. These motifs include 16 previously known regulatory elements, such as the histone 3'-UTR motif and the neuron-restrictive silencer element, as well as striking examples of novel functional elements. The most highly enriched motif (LM1) corresponds to the X-box motif known from yeast and nematode. We show that it is bound by the RFX1 protein and identify thousands of conserved motif instances, suggesting a broad role for the RFX family in gene regulation. A second group of motifs (LM2*) does not match any previously known motif. We demonstrate by biochemical and computational methods that it defines a binding site for the CTCF protein, which is involved in insulator function to limit the spread of gene activation. We identify nearly 15,000 conserved sites that likely serve as insulators, and we show that nearby genes separated by predicted CTCF sites show markedly reduced correlation in gene expression. These sites may thus partition the human genome into domains of expression. [ABSTRACT FROM AUTHOR]

Published

2007

5. A large family of ancient repeat elements in the human genome is under strong selection.

Author

Kamal, Michael, Xiaohui Xie, and Lander, Eric S.

Subjects

*HUMAN genome, *HUMAN chromosomes, *NUCLEOTIDE sequence, *NUCLEIC acid analysis, *NUCLEOTIDE analysis, *GENOMES

Abstract

Although conserved noncoding elements (CNEs) constitute the majority of sequences under purifying selection in the human genome, they remain poorly understood. CNEs seem to be largely unique, with no large families of similar elements reported to date. Here, we search for CNEs among the ancestral repeat classes in the human genome and report the discovery of a large CNE family containing >900 members. This family belongs to the MER121 class of repeats. Although the MER121 family members show considerable sequence variation among one another, the individual copies show striking conservation in orthologous locations across the human, dog, mouse, and rat genomes. The element is also present and conserved in orthologous locations in the marsupial, but its genome-wide dispersal postdates the divergence from birds. The comparative genomic data indicate that MER121 does not encode a family of either protein-coding or RNA genes. Although the precise function of these elements remains unknown, the evidence suggests that this unusual family may play a cis-regulatory or structural role in mammalian genomes. [ABSTRACT FROM AUTHOR]

Published

2006