Your search keyword '"Zhide Fang"' showing total 4 results

1. Inferring the expression variability of human transposable element-derived exons by linear model analysis of deep RNA sequencing data

Author

Kun Zhang, Zhide Fang, Prescott L. Deininger, Wei Fan, Andrea Edwards, and Wensheng Zhang

Subjects

Untranslated region, Alu element, Gene Expression, Biology, 03 medical and health sciences, Exon, 0302 clinical medicine, Genetic model, Genetics, Humans, RNA, Messenger, 030304 developmental biology, Expressed Sequence Tags, 0303 health sciences, Expressed sequence tag, Models, Genetic, Genome, Human, Sequence Analysis, RNA, High-Throughput Nucleotide Sequencing, Exons, 030220 oncology & carcinogenesis, DNA Transposable Elements, Linear Models, Human genome, Tandem exon duplication, DNA microarray, Biotechnology, Research Article

Abstract

Background: The exonization of transposable elements (TEs) has proven to be a significant mechanism for the creation of novel exons. Existing knowledge of the retention patterns of TE exons in mRNAs were mainly established by the analysis of Expressed Sequence Tag (EST) data and microarray data. Results: This study seeks to validate and extend previous studies on the expression of TE exons by an integrative statistical analysis of high throughput RNA sequencing data. We collected 26 RNA-seq datasets spanning multiple tissues and cancer types. The exon-level digital expressions (indicating retention rates in mRNAs) were quantified by a double normalized measure, called the rescaled RPKM (Reads Per Kilobase of exon model per Million mapped reads). We analyzed the distribution profiles and the variability (across samples and between tissue/disease groups) of TE exon expressions, and compared them with those of other constitutive or cassette exons. We inferred the effects of four genomic factors, including the location, length, cognate TE family and TE nucleotide proportion (RTE, see Methods section) of a TE exon, on the exons’ expression level and expression variability. We also investigated the biological implications of an assembly of highly-expressed TE exons. Conclusion: Our analysis confirmed prior studies from the following four aspects. First, with relatively high expression variability, most TE exons in mRNAs, especially those without exact counterparts in the UCSC RefSeq (Reference Sequence) gene tables, demonstrate low but still detectable expression levels in most tissue samples. Second, the TE exons in coding DNA sequences (CDSs) are less highly expressed than those in 3′ (5′) untranslated regions (UTRs). Third, the exons derived from chronologically ancient repeat elements, such as MIRs, tend to be highly expressed in comparison with those derived from younger TEs. Fourth, the previously observed negative relationship between the lengths of exons and the inclusion levels in transcripts is also true for exonized TEs. Furthermore, our study resulted in several novel findings. They include: (1) for the TE exons with non-zero expression and as shown in most of the studied biological samples, a high TE nucleotide proportion leads to their lower retention rates in mRNAs; (2) the considered genomic features (i.e. a continuous variable such as the exon length or a category indicator such as 3′UTR) influence the expression level and the expression variability (CV) of TE exons in an inverse manner; (3) not only the exons derived from Alu elements but also the exons from the TEs of other families were preferentially established in zinc finger (ZNF) genes.

Published

2013

2. Inferring the expression variability of human transposable element-derived exons by linear model analysis of deep RNA sequencing data.

Author

Wensheng Zhang, Edwards, Andrea, Wei Fan, Zhide Fang, Deininger, Prescott, and Kun Zhang

Subjects

TRANSPOSONS, EXONS (Genetics), LINEAR statistical models, NUCLEOTIDE sequence, MESSENGER RNA, EXPRESSED sequence tag (Genetics)

Abstract

Background: The exonization of transposable elements (TEs) has proven to be a significant mechanism for the creation of novel exons. Existing knowledge of the retention patterns of TE exons in mRNAs were mainly established by the analysis of Expressed Sequence Tag (EST) data and microarray data. Results: This study seeks to validate and extend previous studies on the expression of TE exons by an integrative statistical analysis of high throughput RNA sequencing data. We collected 26 RNA-seq datasets spanning multiple tissues and cancer types. The exon-level digital expressions (indicating retention rates in mRNAs) were quantified by a double normalized measure, called the rescaled RPKM (Reads Per Kilobase of exon model per Million mapped reads). We analyzed the distribution profiles and the variability (across samples and between tissue/disease groups) of TE exon expressions, and compared them with those of other constitutive or cassette exons. We inferred the effects of four genomic factors, including the location, length, cognate TE family and TE nucleotide proportion (RTE, see Methods section) of a TE exon, on the exons' expression level and expression variability. We also investigated the biological implications of an assembly of highly-expressed TE exons. Conclusion: Our analysis confirmed prior studies from the following four aspects. First, with relatively high expression variability, most TE exons in mRNAs, especially those without exact counterparts in the UCSC RefSeq (Reference Sequence) gene tables, demonstrate low but still detectable expression levels in most tissue samples. Second, the TE exons in coding DNA sequences (CDSs) are less highly expressed than those in 3' (5') untranslated regions (UTRs). Third, the exons derived from chronologically ancient repeat elements, such as MIRs, tend to be highly expressed in comparison with those derived from younger TEs. Fourth, the previously observed negative relationship between the lengths of exons and the inclusion levels in transcripts is also true for exonized TEs. Furthermore, our study resulted in several novel findings. They include: (1) for the TE exons with non-zero expression and as shown in most of the studied biological samples, a high TE nucleotide proportion leads to their lower retention rates in mRNAs; (2) the considered genomic features (i.e. a continuous variable such as the exon length or a category indicator such as 3'UTR) influence the expression level and the expression variability (CV) of TE exons in an inverse manner; (3) not only the exons derived from Alu elements but also the exons from the TEs of other families were preferentially established in zinc finger (ZNF) genes. [ABSTRACT FROM AUTHOR]

Published

2013

3. Rnnotator: an automated de novo transcriptome assembly pipeline from stranded RNA-Seq reads.

Author

Martin, Jeffrey, Bruno, Vincent M., Zhide Fang, Xiandong Meng, Blow, Matthew, Tao Zhang, Sherlock, Gavin, Snyder, Michael, and Zhong Wang

Subjects

MESSENGER RNA, GENOMES, GENOMICS, GENETIC research, MOLECULAR genetics

Abstract

Background: Comprehensive annotation and quantification of transcriptomes are outstanding problems in functional genomics. While high throughput mRNA sequencing (RNA-Seq) has emerged as a powerful tool for addressing these problems, its success is dependent upon the availability and quality of reference genome sequences, thus limiting the organisms to which it can be applied. Results: Here, we describe Rnnotator, an automated software pipeline that generates transcript models by de novo assembly of RNA-Seq data without the need for a reference genome. We have applied the Rnnotator assembly pipeline to two yeast transcriptomes and compared the results to the reference gene catalogs of these organisms. The contigs produced by Rnnotator are highly accurate (95%) and reconstruct full-length genes for the majority of the existing gene models (54.3%). Furthermore, our analyses revealed many novel transcribed regions that are absent from well annotated genomes, suggesting Rnnotator serves as a complementary approach to analysis based on a reference genome for comprehensive transcriptomics. Conclusions: These results demonstrate that the Rnnotator pipeline is able to reconstruct full-length transcripts in the absence of a complete reference genome. [ABSTRACT FROM AUTHOR]

Published

2010

4. Rnnotator: an automated de novo transcriptome assembly pipeline from stranded RNA-Seq reads

Author

Matthew J. Blow, Michael Snyder, Jeffrey Martin, Zhong Wang, Vincent M. Bruno, Zhide Fang, Gavin Sherlock, Xiandong Meng, and Tao Zhang

Subjects

lcsh:QH426-470, Transcription, Genetic, lcsh:Biotechnology, De novo transcriptome assembly, Sequence assembly, RNA-Seq, Computational biology, Biology, Genome, 03 medical and health sciences, Automation, 0302 clinical medicine, lcsh:TP248.13-248.65, Gene Expression Regulation, Fungal, Candida albicans, Genetics, RNA, Messenger, 030304 developmental biology, 0303 health sciences, Base Sequence, Sequence Analysis, RNA, Gene Expression Profiling, Methodology Article, lcsh:Genetics, MRNA Sequencing, DNA microarray, Functional genomics, 030217 neurology & neurosurgery, Software, Reference genome, Biotechnology

Abstract

Background Comprehensive annotation and quantification of transcriptomes are outstanding problems in functional genomics. While high throughput mRNA sequencing (RNA-Seq) has emerged as a powerful tool for addressing these problems, its success is dependent upon the availability and quality of reference genome sequences, thus limiting the organisms to which it can be applied. Results Here, we describe Rnnotator, an automated software pipeline that generates transcript models by de novo assembly of RNA-Seq data without the need for a reference genome. We have applied the Rnnotator assembly pipeline to two yeast transcriptomes and compared the results to the reference gene catalogs of these organisms. The contigs produced by Rnnotator are highly accurate (95%) and reconstruct full-length genes for the majority of the existing gene models (54.3%). Furthermore, our analyses revealed many novel transcribed regions that are absent from well annotated genomes, suggesting Rnnotator serves as a complementary approach to analysis based on a reference genome for comprehensive transcriptomics. Conclusions These results demonstrate that the Rnnotator pipeline is able to reconstruct full-length transcripts in the absence of a complete reference genome.