Glucocorticoid Cell Priming Enhances Transfection Outcomes in Adult Human Mesenchymal Stem Cells

Kelly, Abby M.; Plautz, Sarah A.; Zempleni, Janos; Pannier, Angela K.

doi:10.1038/mt.2015.195

Cited by 19 publications

(66 citation statements)

References 49 publications

(68 reference statements)

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“…Plasmids Bernasconi et al, 1997;Braun et al, 1999;Chen et al, 2011;Choi & Lee, 2005;Jain et al, 1999;Koster et al, 2002;Köster et al, 2006;Lin et al, 2003;Nair et al, 2002) compared to those seen here in hMSCs. Our results showing increased transgenic enzyme activity in addition to increased transgenic protein production (all relative to VCs) are probably not specific to only luciferase transgenes because we previously reported DEX-priming yielded 4-7-fold increases in transgenic β-galactosidase enzyme activity, whereas also increasing transgenic EGFP mean fluorescence intensity by about two-fold, all relative to VC (Kelly et al, 2016). Our results showing increased transgenic enzyme activity in addition to increased transgenic protein production (all relative to VCs) are probably not specific to only luciferase transgenes because we previously reported DEX-priming yielded 4-7-fold increases in transgenic β-galactosidase enzyme activity, whereas also increasing transgenic EGFP mean fluorescence intensity by about two-fold, all relative to VC (Kelly et al, 2016).…”

Section: Enhancement By Dex Is Pdna Sequence Element Independentmentioning

confidence: 48%

“…Although DEX increased transgenic luciferase activity normalized to total protein by about 10-fold in transfected hMSCs, DEX only increased the amount of transgenic luciferase protein by about two-fold, as quantified by western blot analysis normalized to total protein (Figure 1c,d), suggesting that DEX-priming somehow increases transgenic enzyme activity downstream of transgenic protein synthesis. It is likely that hMSC transfection could be primed with many other Gc drugs in addition to DEX, as our previous work demonstrated that priming with cortisol similarly resulted in significant enhancement of transgene expression in transfected hMSCs (Kelly et al, 2016). It is likely that hMSC transfection could be primed with many other Gc drugs in addition to DEX, as our previous work demonstrated that priming with cortisol similarly resulted in significant enhancement of transgene expression in transfected hMSCs (Kelly et al, 2016).…”

Section: Enhancement By Dex Is Pdna Sequence Element Independentmentioning

confidence: 88%

“…Most Gc effects within cells are mediated by binding and activation of the GR and we previously demonstrated that binding of the GR is required for DEX-mediated enhancement of transgene expression in hMSCs (Kelly et al, 2016). Since DEX has been shown to alter nuclear membrane permeability (Kastrup, Oberleithner, Ludwig, Schafer, & Shahin, 2006;Shahin, 2006;Shahin et al, 2005), and the GR has been shown to interact with similar transport and nuclear import pathways as pDNA, we quantified the number of plasmid copies in transfected hMSCs and isolated nuclei, with and without DEX-priming.…”

Section: Dex Ameliorates Hmsc Protein Synthesis Inhibition Induced mentioning

confidence: 99%

“…Specifically, we investigated anti-inflammatory glucocorticoid (Gc) drugs as priming candidates in hMSCs due to reports in other cell types that Gc can increase transfection efficiency by increasing plasmid DNA (pDNA) nuclear internalization or reducing the inflammatory response to transfection (Braun et al, 1999;Kim, Kim, Bae, Choi, & Lee, 2009). In hMSCs, derived from bone marrow stromal cells (BMSCs) of multiple donors, we showed that 90 to 360 nM dexamethasone (DEX), a Gc drug, delivered 0-30 min before delivery of pDNA lipoplexes increased the transgenic luciferase activity about 10-fold, increased transgenic enhanced green fluorescent protein (EGFP) mean fluorescence intensity of transfected cells about two-fold, increased transfection efficiency about three-fold (i.e., percent of EGFP + transfected cells), increased duration of transgene expression, and ameliorated transfection-induced metabolic decline, all while retaining differentiation capacity (Kelly, Plautz, Zempleni, & Pannier, 2016). Others have reported similar enhancement of transfection using steroids in other cell types.…”

mentioning

confidence: 99%

“…Since DEX-priming of hMSC transfection is mediated by binding of the glucocorticoid receptor (GR; Kelly et al, 2016), which makes use of similar intracellular transport mechanisms as transfected pDNA does (Davies, Ning, & Sánchez, 2002;Dhanoya, Wang, Keshavarz-Moore, Fassati, & Chain, 2013;Echeverria et al, 2009;Galigniana, Harrell, O'Hagen, Ljungman, & Pratt, 2004;Harrell et al, 2004;Lachish-Zalait et al, 2009), and GR modulates gene expression related to antiinflammatory and stress pathways (Ratman et al, 2013), we analyze nonviral gene delivery barriers and pathways in hMSCs including internalization, cytoplasmic transport, nuclear translocation, transgene transcription, translation, and cellular stress response, along with the effects of DEX-priming on each of these barriers and pathways. We also explore the effects of different pDNA regulatory sequences on transgene expression and DEX-priming.…”

mentioning

confidence: 99%

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Mechanisms of unprimed and dexamethasone‐primed nonviral gene delivery to human mesenchymal stem cells

Hamann

Broad

Nguyen

et al. 2018

Biotech & Bioengineering

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Human mesenchymal stem cells (hMSCs) are under intense study for applications of cell and gene therapeutics because of their unique immunomodulatory and regenerative properties. Safe and efficient genetic modification of hMSCs could increase their clinical potential by allowing functional expression of therapeutic transgenes or control over behavior and differentiation. Viral gene delivery is efficient, but suffers from safety issues, while nonviral methods are safe, but highly inefficient, especially in hMSCs. Our lab previously demonstrated that priming cells before delivery of DNA complexes with dexamethasone (DEX), an anti‐inflammatory glucocorticoid drug, significantly increases hMSC transfection success. This work systematically investigates the mechanisms of hMSC transfection and DEX‐mediated enhancement of transfection. Our results show that hMSC transfection and its enhancement by DEX are decreased by inhibiting classical intracellular transport and nuclear import pathways, but DEX transfection priming does not increase cellular or nuclear internalization of plasmid DNA (pDNA). We also show that hMSC transgene expression is largely affected by pDNA promoter and enhancer sequence changes, but DEX‐mediated enhancement of transfection is unaffected by any pDNA sequence changes. Furthermore, DEX‐mediated transfection enhancement is not the result of increased transgene messenger RNA transcription or stability. However, DEX‐priming increases total protein synthesis by preventing hMSC apoptosis induced by transfection, resulting in increased translation of transgenic protein. DEX may also promote further enhancement of transgenic reporter enzyme activity by other downstream mechanisms. Mechanistic studies of nonviral gene delivery will inform future rationally designed technologies for safe and efficient genetic modification of clinically relevant cell types.

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Section: Enhancement By Dex Is Pdna Sequence Element Independentmentioning

confidence: 48%

Section: Enhancement By Dex Is Pdna Sequence Element Independentmentioning

confidence: 88%

Section: Dex Ameliorates Hmsc Protein Synthesis Inhibition Induced mentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

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Mechanisms of unprimed and dexamethasone‐primed nonviral gene delivery to human mesenchymal stem cells

Hamann

Broad

Nguyen

et al. 2018

Biotech & Bioengineering

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High‐throughput screening of clinically approved drugs that prime polyethylenimine transfection reveals modulation of mitochondria dysfunction response improves gene transfer efficiencies

Nguyen

Beyersdorf

Riethoven

et al. 2016

Bioengineering & Transla Med

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Nonviral gene delivery methods are advantageous over viral vectors in terms of safety, cost, and flexibility in design and application, but suffer from lower gene transfer efficiency. In addition to modifications to nucleic acid design and nonviral carriers, new tools are sought to enhance transfection. Priming is the pharmacological modulation of transfection efficiency and transgene expression, and has demonstrated transfection increase in several compounds, for example, chloroquine and glucocorticoids. To develop a library of transfection priming compounds, a high‐throughput screen was performed of the NIH Clinical Collection (NCC) to identify clinical compounds that prime polyethylenimine (PEI) transfection. HEK293T cells were treated with priming compounds, then transfected with enhanced green fluorescent protein (EGFP)‐encoding plasmid by PEI. After 48‐hr culture, primed and transfected cells were assayed for transfection, cell proliferation, and cell viability by fluorescence measurement of EGFP reporter, Hoechst 33342 nuclei stain, and resazurin metabolic assay. From the microscope image analysis and microplate measurements, transfection fold‐changes were determined, and compounds resulting in statistically significant transfection fold‐change were identified. NCC compounds were clustered using PubChem fingerprint similarity by Tanimoto coefficients in ChemmineTools. Fold‐changes for each compound were linked to drug clusters, from which drug classes that prime transfection were identified. Among the identified drugs classes that primed transfection increases were antioxidants, GABAA receptor modulators, and glucocorticoids. Resveratrol and piceid, stilbenoid antioxidants found in grapes, and zolpidem, a GABAA modulator, increased transfection nearly three‐fold. Literature indicate interaction of the identified transfection priming drug clusters with mitochondria, which may modulate mitochondrial dysfunction known to be associated with PEI transfection.

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Modulating intracellular pathways to improve non-viral delivery of RNA therapeutics

Vyver

Smedt

Raemdonck

2022

Advanced Drug Delivery Reviews

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Glucocorticoid Cell Priming Enhances Transfection Outcomes in Adult Human Mesenchymal Stem Cells

Cited by 19 publications

References 49 publications

Mechanisms of unprimed and dexamethasone‐primed nonviral gene delivery to human mesenchymal stem cells

Mechanisms of unprimed and dexamethasone‐primed nonviral gene delivery to human mesenchymal stem cells

High‐throughput screening of clinically approved drugs that prime polyethylenimine transfection reveals modulation of mitochondria dysfunction response improves gene transfer efficiencies

Modulating intracellular pathways to improve non-viral delivery of RNA therapeutics

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