An Optimized microRNA Backbone for Effective Single-Copy RNAi

Fellmann, Christof; Hoffmann, Thomas; Sridhar, Vaishali; Hopfgartner, Barbara; Muhar, Matthias; Roth, Mareike; Lai, Dan Yu; Barbosa, Inês; Kwon, Jung Shick; Guan, Yuanzhe; Sinha, Nishi; Zuber, Johannes

doi:10.1016/j.celrep.2013.11.020

Cited by 580 publications

(641 citation statements)

References 38 publications

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“…27990, or on request) (Zuber et al 2011a;Fellmann et al 2013). To produce Tet-on murine HCC MP1 cells, liver progenitor cells from p53 Loxp/Loxp mice were transduced with CreER and Myc-IRES-rtTA3.…”

Section: Plasmidsmentioning

confidence: 99%

“…Control (Renilla and Myc) and Cdk9 shRNAs were subcloned into miR-E, an optimized miR-30-based backbone that increases knockdown efficiency, particularly for those shRNAs with intermediate potency (Supplemental Fig. 2B,C;Fellmann et al 2013). All three experimental murine HCC cell lines that overexpressed Myc (MP1, MP-CH, and Myc-AL) were highly sensitive to Cdk9 inhibition, while murine HCC cells expressing mutant Kras G12D , Hepa1-6 hepatoma cells, NIH-3T3 fibroblasts, and iMEFs showed modest to no sensitivity (Fig.…”

Section: Rnai Screen For Genes Encoding Known Drug Targetsmentioning

confidence: 99%

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CDK9-mediated transcription elongation is required for MYC addiction in hepatocellular carcinoma

et al. 2014

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One-year survival rates for newly diagnosed hepatocellular carcinoma (HCC) are <50%, and unresectable HCC carries a dismal prognosis owing to its aggressiveness and the undruggable nature of its main genetic drivers. By screening a custom library of shRNAs directed toward known drug targets in a genetically defined Myc-driven HCC model, we identified cyclin-dependent kinase 9 (Cdk9) as required for disease maintenance. Pharmacological or shRNA-mediated CDK9 inhibition led to robust anti-tumor effects that correlated with MYC expression levels and depended on the role that both CDK9 and MYC exert in transcription elongation. Our results establish CDK9 inhibition as a therapeutic strategy for MYC-overexpressing liver tumors and highlight the relevance of transcription elongation in the addiction of cancer cells to MYC.

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Section: Plasmidsmentioning

confidence: 99%

Section: Rnai Screen For Genes Encoding Known Drug Targetsmentioning

confidence: 99%

CDK9-mediated transcription elongation is required for MYC addiction in hepatocellular carcinoma

et al. 2014

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“…No changes in PAK1 and PAK2 levels were detectable (Fig S3). Stable knockdown of PAK1 , PAK2 , or both genes was achieved using an established, miR30‐shRNA‐based system (Zuber et al , 2011; Fellmann et al , 2013; Putz et al , 2013, 2014; Berger et al , 2014; Scheicher et al , 2015). Knockdown efficiencies were verified by qPCR and immunoblotting (Fig 2A and B).…”

Section: Resultsmentioning

confidence: 99%

Expansion of BCR/ABL1⁺ cells requires PAK2 but not PAK1

et al. 2017

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SummaryThe p21‐activated kinases (PAKs) are key nodes in oncogenic signalling pathways controlling growth, survival, and motility of cancer cells. Their activity is increased in many human cancers and is associated with poor prognosis. To date, PAK deregulation has mainly been studied in solid tumours, where PAK1 and PAK4 are the main isoforms deregulated. We show that PAK1 and PAK2 are the critical isoforms in a BCR/ABL1 + haematopoietic malignancy. In suspension, leukaemic cells deficient for PAK1 and PAK2 undergo apoptosis, while the loss of either protein is well tolerated. Transfer of medium conditioned by shPAK2‐ but not shPAK1‐expressing leukaemic cells interferes with endothelial cell growth. We found that leukaemic cells produce exosomes containing PAK2. Transfer of isolated exosomes supports endothelial cell proliferation. In parallel, we found that leukaemic cells explicitly require PAK2 to grow towards an extracellular matrix. PAK2‐deficient cells fail to form colonies in methylcellulose and to induce lymphomas in vivo. PAK2 might therefore be the critical isoform in leukaemic cells by controlling tumour growth in a dual manner: vascularization via exosome‐mediated transfer to endothelial cells and remodelling of the extracellular matrix. This finding suggests that the PAK2 isoform represents a promising target for the treatment of haematological diseases.

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“…However, it is important to note any possibility of off-target effects of the RNAi in this system. Whereas our model exploits a recently developed inducible shRNA system, wherein the shRNA is expressed in a miR-E cassette to allow physiological processing and reduced off-target effects [22], currently we only use one targeting sequence. As such it will be important to develop further RNAi models targeting alternative sequences of Atg5 , or other key autophagy genes, for further validation of newly described phenotypes.…”

Section: Discussionmentioning

confidence: 99%

“…We tested knockdown efficiency of those shRNAs in NIH3T3 cells, and an shRNA showing the strongest knockdown even with the highest dilution (1% v:v) viral supernatant was taken forward for LSL-ATG5i mouse generation by Mirimus Inc. Briefly, the shRNA ( Atg5 _ 1065; Guide sequence: TATGAAGAAAGTTATCTGGGTA) in a miR-E design (an improved design variant of miR30) [22] was inserted downstream of the Col1a1 locus via recombinase-mediated cassette exchange which enables efficient targeting of a transgene to a specific genomic site 500 base pairs downstream of the 3ʹ UTR in D34 ES cells expressing CAG-rtTA3 knocked into the Rosa26 locus (Fig. S1) [29,30].…”

Section: Methodsmentioning

confidence: 99%

A novel Atg5-shRNA mouse model enables temporal control of Autophagy in vivo

et al. 2018

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Macroautophagy/autophagy is an evolutionarily conserved catabolic pathway whose modulation has been linked to diverse disease states, including age-associated disorders. Conventional and conditional whole-body knockout mouse models of key autophagy genes display perinatal death and lethal neurotoxicity, respectively, limiting their applications for in vivo studies. Here, we have developed an inducible shRNA mouse model targeting Atg5, allowing us to dynamically inhibit autophagy in vivo, termed ATG5i mice. The lack of brain-associated shRNA expression in this model circumvents the lethal phenotypes associated with complete autophagy knockouts. We show that ATG5i mice recapitulate many of the previously described phenotypes of tissue-specific knockouts. While restoration of autophagy in the liver rescues hepatomegaly and other pathologies associated with autophagy deficiency, this coincides with the development of hepatic fibrosis. These results highlight the need to consider the potential side effects of systemic anti-autophagy therapies.

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An Optimized microRNA Backbone for Effective Single-Copy RNAi

Cited by 580 publications

References 38 publications

CDK9-mediated transcription elongation is required for MYC addiction in hepatocellular carcinoma

CDK9-mediated transcription elongation is required for MYC addiction in hepatocellular carcinoma

Expansion of BCR/ABL1⁺ cells requires PAK2 but not PAK1

A novel Atg5-shRNA mouse model enables temporal control of Autophagy in vivo

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An Optimized microRNA Backbone for Effective Single-Copy RNAi

Cited by 580 publications

References 38 publications

CDK9-mediated transcription elongation is required for MYC addiction in hepatocellular carcinoma

CDK9-mediated transcription elongation is required for MYC addiction in hepatocellular carcinoma

Expansion of BCR/ABL1+ cells requires PAK2 but not PAK1

A novel Atg5-shRNA mouse model enables temporal control of Autophagy in vivo

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Expansion of BCR/ABL1⁺ cells requires PAK2 but not PAK1