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dc.creatorZhang, Yonggang
dc.creatorArango, Gustavo
dc.creatorLi, Fang
dc.creatorXiao, Xiao
dc.creatorPutatunda, Raj
dc.creatorYu, Jun
dc.creatorYang, Xiao-Feng
dc.creatorWang, Hong
dc.creatorWatson, Layne T.
dc.creatorZhang, Liqing
dc.creatorHu, Wenhui
dc.date.accessioned2023-06-22T15:11:17Z
dc.date.available2023-06-22T15:11:17Z
dc.date.issued2018-09-10
dc.identifier.citationZhang, Y., Arango, G., Li, F. et al. Comprehensive off-target analysis of dCas9-SAM-mediated HIV reactivation via long noncoding RNA and mRNA profiling. BMC Med Genomics 11, 78 (2018). https://doi.org/10.1186/s12920-018-0394-2
dc.identifier.issn1755-8794
dc.identifier.doihttp://dx.doi.org/10.34944/dspace/8674
dc.identifier.urihttp://hdl.handle.net/20.500.12613/8710
dc.description.abstractBackground: CRISPR/CAS9 (epi)genome editing revolutionized the field of gene and cell therapy. Our previous study demonstrated that a rapid and robust reactivation of the HIV latent reservoir by a catalytically-deficient Cas9 (dCas9)-synergistic activation mediator (SAM) via HIV long terminal repeat (LTR)-specific MS2-mediated single guide RNAs (msgRNAs) directly induces cellular suicide without additional immunotherapy. However, potential off-target effect remains a concern for any clinical application of Cas9 genome editing and dCas9 epigenome editing. After dCas9 treatment, potential off-target responses have been analyzed through different strategies such as mRNA sequence analysis, and functional screening. In this study, a comprehensive analysis of the host transcriptome including mRNA, lncRNA, and alternative splicing was performed using human cell lines expressing dCas9-SAM and HIV-targeting msgRNAs. Results: The control scrambled msgRNA (LTR_Zero), and two LTR-specific msgRNAs (LTR_L and LTR_O) groups show very similar expression profiles of the whole transcriptome. Among 839 identified lncRNAs, none exhibited significantly different expression in LTR_L vs. LTR_Zero group. In LTR_O group, only TERC and scaRNA2 lncRNAs were significantly decreased. Among 142,791 mRNAs, four genes were differentially expressed in LTR_L vs. LTR_Zero group. There were 21 genes significantly downregulated in LTR_O vs. either LTR_Zero or LTR_L group and one third of them are histone related. The distributions of different types of alternative splicing were very similar either within or between groups. There were no apparent changes in all the lncRNA and mRNA transcripts between the LTR_L and LTR_Zero groups. Conclusion: This is an extremely comprehensive study demonstrating the rare off-target effects of the HIV-specific dCas9-SAM system in human cells. This finding is encouraging for the safe application of dCas9-SAM technology to induce target-specific reactivation of latent HIV for an effective “shock-and-kill” strategy.
dc.format.extent17 pages
dc.languageEnglish
dc.language.isoeng
dc.relation.ispartofFaculty/ Researcher Works
dc.relation.haspartBMC Medical Genomics, Vol. 11, No. 78
dc.relation.isreferencedbyBMC
dc.rightsAttribution CC BY
dc.rights.urihttps://creativecommons.org/licenses/by/4.0/
dc.subjectGenome editing
dc.subjectCRISPR
dc.subjectOff-target
dc.subjectRNA sequencing
dc.subjectTRanscriptome
dc.subjectHIV
dc.subjectLatency
dc.subjectShock and kill
dc.titleComprehensive off-target analysis of dCas9-SAM-mediated HIV reactivation via long noncoding RNA and mRNA profiling
dc.typeText
dc.type.genreJournal article
dc.contributor.groupCenter for Metabolic Disease Research (Temple University)
dc.description.departmentPathology and Laboratory Medicine
dc.relation.doihttps://doi.org/10.1186/s12920-018-0394-2
dc.ada.noteFor Americans with Disabilities Act (ADA) accommodation, including help with reading this content, please contact scholarshare@temple.edu
dc.description.schoolcollegeLewis Katz School of Medicine
dc.creator.orcidXiao|0000-0002-0077-1337
dc.creator.orcidYu|0000-0003-4530-2179
dc.creator.orcidWang, Hong|0000-0001-6258-4070
dc.temple.creatorZhang, Yonggang
dc.temple.creatorLi, Fang
dc.temple.creatorXiao, Xiao
dc.temple.creatorPutatunda, Raj
dc.temple.creatorYu, Jun
dc.temple.creatorYang, Xiao-Feng
dc.temple.creatorWang, Hong
dc.temple.creatorHu, Wenhui
refterms.dateFOA2023-06-22T15:11:17Z


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