A CRISPR interference strategy for gene expression silencing in multiple myeloma cell lines

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dc.centroUniversidad Cardenal Herrera-CEU
dc.contributor.authorEscrivá Fernández, Josep
dc.contributor.authorBallester Lurbe, Begoña
dc.contributor.authorCueto Ureña, Cristina
dc.contributor.authorSolana Orts, Amalia
dc.contributor.authorLledó Feijoó, Elisa
dc.contributor.authorPoch Jiménez, Enric
dc.contributor.otherUCH. Departamento de Ciencias Biomédicas
dc.contributor.otherProducción Científica UCH 2023
dc.date.accessioned2024-02-28T15:15:38Z
dc.date.available2024-02-28T15:15:38Z
dc.date.issued2023-05-04
dc.description.abstractBackground: Multiple myeloma (MM) is the second most common hematologic neoplasm which is characterized by proliferation and infiltration of plasmatic cells in the bone marrow. Currently, MM is considered incurable due to resistance to treatment. The CRISPR/Cas9 system has emerged as a powerful tool for understanding the role of different genetic alterations in the pathogenesis of hematologic malignancies in both cell lines and mouse models. Despite current advances of gene editing tools, the use of CRISPR/Cas9 technology for gene editing of MM have not so far been extended. In this work, we want to repress Rnd3 expression, an atypical Rho GTPase involved in several cellular processes, in MM cell lines using a CRISPR interference strategy. Results: We have designed different guide RNAs and cloning them into a lentiviral plasmid, which contains all the machinery necessary for developing the CRISPR interference strategy. We co-transfected the HEK 293T cells with this lentiviral plasmid and 3rd generation lentiviral envelope and packaging plasmids to produce lentiviral particles. The lentiviral particles were used to transduce two different multiple myeloma cell lines, RPMI 8226 and JJN3, and downregulate Rnd3 expression. Additionally, the impact of Rnd3 expression absence was analyzed by a transcriptomic analysis consisting of 3' UTR RNA sequencing. The Rnd3 knock-down cells showed a different transcriptomic profile in comparison to control cells. Conclusions: We have developed a CRISPR interference strategy to generate stable Rnd3 knockdown MM cell lines by lentiviral transduction. We have evaluated this strategy in two MM cell lines, and we have demonstrated that Rnd3 silencing works both at transcriptional and protein level. Therefore, we propose CRISPR interference strategy as an alternative tool to silence gene expression in MM cell lines. Furthermore, Rnd3 silencing produces changes in the cellular transcriptomic profile.es_ES
dc.identifier.citationEscrivá-Fernández, J., Cueto-Ureña, C., Solana-Orts, A., Lledó, E., Ballester-Lurbe, B. & Poch, E. (2023). A CRISPR interference strategy for gene expression silencing in multiple myeloma cell lines. Journal of Biological Engineering, vol. 17, i. 1, art. 34. DOI: https://doi.org/10.1186/s13036-023-00347-7es_ES
dc.identifier.doihttps://doi.org/10.1186/s13036-023-00347-7
dc.identifier.issn1754-1611 (Electrónico)
dc.identifier.urihttp://hdl.handle.net/10637/15507
dc.language.isoenes_ES
dc.publisherSpringer Naturees_ES
dc.relationEste artículo de investigación ha sido financiado por la Conselleria d’ Innovació, Universitats, Ciència i Societat Digital de la Generalitat Valenciana (GV/2019/119) y por la Fundación Universitaria San Pablo CEU a través de la Universidad CEU Cardenal Herrera (FUSP-PPC-19-28A751CC).
dc.relationUCH. Financiación Autonómica
dc.relationUCH. Financiación Universidad
dc.relation.ispartofJournal of Biological Engineering, vol. 17, i. 1
dc.relation.projectIDGV/2019/119
dc.relation.projectIDFUSP-PPC-19-28A751CC
dc.rightsopen access
dc.rights.cchttps://creativecommons.org/licenses/by-nc-nd/4.0/deed.es
dc.subjectMédula óseaes_ES
dc.subjectBone marrowes_ES
dc.subjectTumorses_ES
dc.subjectTumorses_ES
dc.subjectTratamiento médicoes_ES
dc.subjectMedical treatmentes_ES
dc.subjectCélulaes_ES
dc.subjectCellses_ES
dc.titleA CRISPR interference strategy for gene expression silencing in multiple myeloma cell lineses_ES
dc.typeArtículoes_ES
dspace.entity.typePublicationes
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relation.isAuthorOfPublication.latestForDiscovery2a5b04e7-89fc-4daf-a9e4-b194a057ea56

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