Hydrodynamic Delivery of Cre Protein to Lineage-Mark or Time-Stamp Mouse Hepatocytes In situ

Sonsteng, Katherine M.; Prigge, Justin R.; Talago, Emily A.; June, Ronald K.; Schmidt, Edward E.

doi:10.1371/journal.pone.0091219

Cited by 6 publications

(6 citation statements)

References 41 publications

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“…However, some specificity may be added by adjusting the conditions of infusion. Indeed, as reported by others [43], we observed a lack of widespread Cre activity: TAT-Cre induces the DNA recombination close to the site of injection. Therefore, the flow rate, the site, and the volume of injection may influence the proportion of targeted tanycytes versus ependymal cells.…”

Section: Tat-cre Modelsupporting

confidence: 79%

Targeting Tanycytes: Balance between Efficiency and Specificity

Langlet¹

2020

Neuroendocrinology

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Tanycytes are peculiar ependymoglial cells lining the bottom and the lateral wall of the third ventricle. For a decade, the utilization of molecular genetic approaches allowed us to make important discoveries about their diverse physiological functions. Here, I review the current methods used to target tanycytes, focusing on their specificity, their efficiency, their limitations, as well as their potential future improvements.specificity? This mini-review aims to describe the current methods used to selectively target tanycytes and study their function. It will also discuss the specificity, the efficiency, and the limitations of these methods as well as new possibilities for their improvements.

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Section: Tat-cre Modelsupporting

confidence: 79%

Targeting Tanycytes: Balance between Efficiency and Specificity

Langlet¹

2020

Neuroendocrinology

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“…Mice were kept under specialized care conditions, including continuous-flow HEPA-filtered air cages (Tecniplast); sterilized bedding and enrichment; free access to sterilized feed (Picolabs 5058) and sterilized water; and on a 14:10 light:dark cycle. For hydrodynamic delivery of Cre to liver hepatocytes, mice received a single tail-vein injection of lactated Ringer’s solution equal to 10% of their body-weight, containing 5 µg of plasmid pCMVpCreSVtx 31 . For Tamoxifen-induced conversion of all hepatocytes in mice, ROSA mT-mG/mT-mG ; Txnrd1 cond/cond ; Gsr null/null ; Alb ICE/+ mice, having an allele of the Alb ICE (for Alb - I RES- C re E RT2) knock-in allele 32 (a generous gift from P. Chambon and D. Metzger, Illkirch, France), in which an i nternal r ibosomal e ntry s ite- (IRES-) driven second cistron targeted into the 3’ untranslated region of the endogenous Alb locus was used to provide strong hepatocyte-specific transcription and translation of the Tamoxifen-inducible CreERT2 protein.…”

Section: Methodsmentioning

confidence: 99%

Dietary methionine can sustain cytosolic redox homeostasis in the mouse liver

et al. 2015

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Across phyla, reduced nicotinamide adenine dinucleotide phosphate (NADPH) transfers intracellular reducing power to thioredoxin reductase-1 (TrxR1) and glutathione reductase (GR), thereby supporting fundamental housekeeping and antioxidant pathways. Here we show that a third, NADPH-independent, pathway can bypass the need for TrxR1 and GR in mammalian liver. Most mice genetically engineered to lack both TrxR1 and GR in all hepatocytes (“TR/GR-null livers”) remain long-term viable. TR/GR-null livers cannot reduce oxidized glutathione disulfide but still require continuous glutathione synthesis. Inhibition of cystathionine gamma-lyase causes rapid necrosis of TR/GR-null livers, indicating that methionine-fueled trans-sulfuration supplies the necessary cysteine precursor for glutathione synthesis via an NADPH-independent pathway. We further show that dietary methionine provides the cytosolic disulfide reducing power and all sulfur amino acids in TR/GR-null livers. Although NADPH is generally considered an essential reducing currency, these results indicate that hepatocytes can adequately sustain cytosolic redox homeostasis pathways using either NADPH or methionine.

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“…The intracellular delivery and cytoplasmic traffic mediated by TAT and penetratin resulted in genomic recombination in subpopulations of neurons in discrete areas of embryonic and adult neural tissues (Gitton et al, 2009). TAT-Cre recombinase fusion protein was also used by Sonsteng et al (2014) to target hepatocytes in vivo by means of hydrodynamic delivery in transgenic (ROSA nTnG ) mice. The transgenic mouse version that they developed localizes the dual red-and green-fluorescent reporter proteins to the nucleus (ROSA nTnG ) instead of the outer membrane, as originally displayed in mice bearing the ROSA mTmG genotype, i.e., cells carrying the floxed membrane-targeted tdTomato (tdT) cistron followed by a membrane-targeted, enhanced green fluorescent protein (EGFP) cistron.…”

Section: Cpp-mediated Transduction Of Cre Recombinasementioning

confidence: 99%

Cell-penetrating peptides (CPPs): From delivery of nucleic acids and antigens to transduction of engineered nucleases for application in transgenesis

Rádis‐Baptista

Campelo

Morlighem

et al. 2017

Journal of Biotechnology

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Cell-penetrating peptides (CPPs) have been studied for their capacity to translocate across the lipid membrane of several cell types. In membrane translocation, these peptides can remarkably transport biologically active hydrophilic molecules, such as pharmaceuticals, nucleic acids (DNA and RNA) and even high-molecular-weight proteins, Fig. 3 into the cell cytoplasm and organelles. The development of CPPs as transduction agents includes the modification of gene and protein expression, the reprogramming and differentiation of induced pluripotent stem cells and the preparation of cellular vaccines. A relatively recent field of CPP application is the transduction of plasmid DNA vectors and CPP-fusion proteins to modify genomes and introduce new traits in cells and organisms. CPP-mediated transduction of components for genome editing is an advantageous alternative to viral DNA vectors. Engineered site-specific nucleases, such as Cre recombinase, ZFN, TALENs and CRISPR associated protein (Cas), have been coupled to CPPs, and the fused proteins have been used to permeate targeted cells and tissues. The functionally active fusion CPP-nucleases subsequently home to the nucleus, incise genomic DNA at specific sites and induce repair and recombination. This review has the objective of discussing CPPs and elucidating the prospective use of CPP-mediated transduction technology, particularly in genome modification and transgenesis.

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Hydrodynamic Delivery of Cre Protein to Lineage-Mark or Time-Stamp Mouse Hepatocytes In situ

Cited by 6 publications

References 41 publications

Targeting Tanycytes: Balance between Efficiency and Specificity

Targeting Tanycytes: Balance between Efficiency and Specificity

Dietary methionine can sustain cytosolic redox homeostasis in the mouse liver

Cell-penetrating peptides (CPPs): From delivery of nucleic acids and antigens to transduction of engineered nucleases for application in transgenesis

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