Your search keyword '"Zhang, Shoudong"' showing total 5 results

1. Use of NAD tagSeq II to identify growth phase-dependent alterations in E. coli RNA NAD+ capping

Author

Zhang, Hailei, Zhong, Huan, Wang, Xufeng, Zhang, Shoudong, Shao, Xiaojian, Hu, Hao, Yu, Zhiling, Cai, Zongwei, Chen, Xuemei, and Xia, Yiji

Subjects

Genetics, Underpinning research, 1.1 Normal biological development and functioning, Generic health relevance, Cell Cycle, Click Chemistry, Cycloaddition Reaction, Escherichia coli, NAD, RNA Processing, Post-Transcriptional, RNA, Messenger, Transcriptome, NAD(+)-capped RNAs, E. coli, gene regulation, SPAAC, NAD tagSeq II, NAD+-capped RNAs

Abstract

Recent findings regarding nicotinamide adenine dinucleotide (NAD+)-capped RNAs (NAD-RNAs) indicate that prokaryotes and eukaryotes employ noncanonical RNA capping to regulate gene expression. Two methods for transcriptome-wide analysis of NAD-RNAs, NAD captureSeq and NAD tagSeq, are based on copper-catalyzed azide-alkyne cycloaddition (CuAAC) click chemistry to label NAD-RNAs. However, copper ions can fragment/degrade RNA, interfering with the analyses. Here we report development of NAD tagSeq II, which uses copper-free, strain-promoted azide-alkyne cycloaddition (SPAAC) for labeling NAD-RNAs, followed by identification of tagged RNA by single-molecule direct RNA sequencing. We used this method to compare NAD-RNA and total transcript profiles of Escherichia coli cells in the exponential and stationary phases. We identified hundreds of NAD-RNA species in E. coli and revealed genome-wide alterations of NAD-RNA profiles in the different growth phases. Although no or few NAD-RNAs were detected from some of the most highly expressed genes, the transcripts of some genes were found to be primarily NAD-RNAs. Our study suggests that NAD-RNAs play roles in linking nutrient cues with gene regulation in E. coli.

Published

2021

2. NAD tagSeq reveals that NAD+-capped RNAs are mostly produced from a large number of protein-coding genes in Arabidopsis

Author

Zhang, Hailei, Zhong, Huan, Zhang, Shoudong, Shao, Xiaojian, Ni, Min, Cai, Zongwei, Chen, Xuemei, and Xia, Yiji

Subjects

Biotechnology, Genetics, 1.1 Normal biological development and functioning, Underpinning research, Generic health relevance, 5' Untranslated Regions, Arabidopsis, Gene Expression, NAD, RNA Caps, RNA, Messenger, Sequence Analysis, RNA, NAD(+) cap, RNA cap, NAD tagSeq, Oxford Nanopore sequencing, NAD+ cap

Abstract

The 5' end of a eukaryotic mRNA transcript generally has a 7-methylguanosine (m7G) cap that protects mRNA from degradation and mediates almost all other aspects of gene expression. Some RNAs in Escherichia coli, yeast, and mammals were recently found to contain an NAD+ cap. Here, we report the development of the method NAD tagSeq for transcriptome-wide identification and quantification of NAD+-capped RNAs (NAD-RNAs). The method uses an enzymatic reaction and then a click chemistry reaction to label NAD-RNAs with a synthetic RNA tag. The tagged RNA molecules can be enriched and directly sequenced using the Oxford Nanopore sequencing technology. NAD tagSeq can allow more accurate identification and quantification of NAD-RNAs, as well as reveal the sequences of whole NAD-RNA transcripts using single-molecule RNA sequencing. Using NAD tagSeq, we found that NAD-RNAs in Arabidopsis were produced by at least several thousand genes, most of which are protein-coding genes, with the majority of these transcripts coming from

Published

2019

3. NAD tagSeq reveals that NAD⁺-capped RNAs are mostly produced from a large number of proteincoding genes in Arabidopsis

Author

Zhang, Hailei, Zhong, Huan, Zhang, Shoudong, Shao, Xiaojian, Ni, Min, Cai, Zongwei, Chen, Xuemei, and Xia, Yiji

Published

2019

4. Use of NAD tagSeq II to identify growth phase-dependent alterations in E. coli RNA NAD + capping.

Author

Zhang H, Zhong H, Wang X, Zhang S, Shao X, Hu H, Yu Z, Cai Z, Chen X, and Xia Y

Subjects

Cell Cycle, Escherichia coli, NAD chemistry, RNA, Messenger chemistry, RNA, Messenger metabolism, Click Chemistry methods, Cycloaddition Reaction methods, NAD metabolism, RNA Processing, Post-Transcriptional, Transcriptome

Abstract

Recent findings regarding nicotinamide adenine dinucleotide (NAD + )-capped RNAs (NAD-RNAs) indicate that prokaryotes and eukaryotes employ noncanonical RNA capping to regulate gene expression. Two methods for transcriptome-wide analysis of NAD-RNAs, NAD captureSeq and NAD tagSeq, are based on copper-catalyzed azide-alkyne cycloaddition (CuAAC) click chemistry to label NAD-RNAs. However, copper ions can fragment/degrade RNA, interfering with the analyses. Here we report development of NAD tagSeq II, which uses copper-free, strain-promoted azide-alkyne cycloaddition (SPAAC) for labeling NAD-RNAs, followed by identification of tagged RNA by single-molecule direct RNA sequencing. We used this method to compare NAD-RNA and total transcript profiles of Escherichia coli cells in the exponential and stationary phases. We identified hundreds of NAD-RNA species in E. coli and revealed genome-wide alterations of NAD-RNA profiles in the different growth phases. Although no or few NAD-RNAs were detected from some of the most highly expressed genes, the transcripts of some genes were found to be primarily NAD-RNAs. Our study suggests that NAD-RNAs play roles in linking nutrient cues with gene regulation in E. coli ., Competing Interests: The authors declare no competing interest., (Copyright © 2021 the Author(s). Published by PNAS.)

Published

2021

5. NAD tagSeq reveals that NAD + -capped RNAs are mostly produced from a large number of protein-coding genes in Arabidopsis .

Author

Zhang H, Zhong H, Zhang S, Shao X, Ni M, Cai Z, Chen X, and Xia Y

Subjects

5' Untranslated Regions genetics, Gene Expression genetics, Sequence Analysis, RNA, Arabidopsis genetics, NAD genetics, RNA Caps genetics, RNA, Messenger genetics

Abstract

The 5' end of a eukaryotic mRNA transcript generally has a 7-methylguanosine (m 7 G) cap that protects mRNA from degradation and mediates almost all other aspects of gene expression. Some RNAs in Escherichia coli , yeast, and mammals were recently found to contain an NAD + cap. Here, we report the development of the method NAD tagSeq for transcriptome-wide identification and quantification of NAD + -capped RNAs (NAD-RNAs). The method uses an enzymatic reaction and then a click chemistry reaction to label NAD-RNAs with a synthetic RNA tag. The tagged RNA molecules can be enriched and directly sequenced using the Oxford Nanopore sequencing technology. NAD tagSeq can allow more accurate identification and quantification of NAD-RNAs, as well as reveal the sequences of whole NAD-RNA transcripts using single-molecule RNA sequencing. Using NAD tagSeq, we found that NAD-RNAs in Arabidopsis were produced by at least several thousand genes, most of which are protein-coding genes, with the majority of these transcripts coming from <200 genes. For some Arabidopsis genes, over 5% of their transcripts were NAD capped. Gene ontology terms overrepresented in the 2,000 genes that produced the highest numbers of NAD-RNAs are related to photosynthesis, protein synthesis, and responses to cytokinin and stresses. The NAD-RNAs in Arabidopsis generally have the same overall sequence structures as the canonical m 7 G-capped mRNAs, although most of them appear to have a shorter 5' untranslated region (5' UTR). The identification and quantification of NAD-RNAs and revelation of their sequence features can provide essential steps toward understanding the functions of NAD-RNAs., Competing Interests: The authors declare no conflict of interest., (Copyright © 2019 the Author(s). Published by PNAS.)

Published

2019