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Cre Reporter Mice. C Representative confocal images show that the Rosa26-based Cre reporter line Ai95 expresses GCaMP6f in cholinergic neurons when crossed to Chat-IRES-Cre mice however native GCaMP6f fluorescence in fixed sections is undetectable compared to TIGRE20 lines compare panels A. By using the CreloxP system a series of double reporter mice expressing a combination of reporter genes including CAG-CAT-Z chloramphenicol acetyltransferaselacZ 51 ZEG lacZEGFP 52 ZAP lacZhuman alkaline phosphatase 53 have been generated. The CreloxP system has been used extensively for conditional mutagenesis in mice. The Allen Institute for Brain Science AIBS website has specific characterization information for several Cre Driver and Cre Reporter lines.

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Mechanism of Cre-loxP system. The resultant allele Mcm3-lox was intended as a conditional KO as Mcm3 expression could be ablated with Cre recombinase. So far the most commonly used locus for generating Cre-responder mice is the Gt ROSA26Sor Rosa26 locus 17. Her e we describe mTmG a double-ßuores cent Cre reporter mouse that expre sses membrane-targeted tandem. These Cre random reporter mice are capable of monitoring Cre activity in diverse tissues and cell types. The day of the vaginal plug was defined as embryonic day 0 and tissues from newborn and embryonic mice were processed for ISH or β-gal and alkaline phosphatase staining as described Lobe et al 1999.

Expressing the red fluorescent protein variant tdTomato following Cre-mediated recombination.

Importantly the donating investigator reports that very low levels of tdTomato expression may be present prior to introduction of Cre recombinase - but the tdTomato expression levels after Cre recombination are significantly greater than those baseline levels. To determine the time of onset of Cre activity Thy1-Cre transgenic mice were time-mated with ZAP Lobe et al 1999 or ROSA26 Soriano 1999 reporter mice. The Allen Institute for Brain Science AIBS website has specific characterization information for several Cre Driver and Cre Reporter lines. These results reveal that PA-Cre 30 is. Spatial information on Cre recombinase activity can be gained using Cre reporter mice in which a reporter gene eg GFP YFP lacZ is inserted at a ubiquitously expressed locus but preceded by a loxP-flanked transcriptional termination. In most Cre-reporter mouse.

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A A modified mouse Mcm3 allele was designed with loxP sites flanking exons 1417 and a luciferase reporter inserted at the 3 UTR under the control of an IRES element. To determine the time of onset of Cre activity Thy1-Cre transgenic mice were time-mated with ZAP Lobe et al 1999 or ROSA26 Soriano 1999 reporter mice. The day of the vaginal plug was defined as embryonic day 0 and tissues from newborn and embryonic mice were processed for ISH or β-gal and alkaline phosphatase staining as described Lobe et al 1999. CRE-Luc GPCR Reporter Mouse Platform An in vitroin vivo luciferase reporter platform for profiling of leads in GPCR drug development. Reporters of Cre activity are important for defining the spatial and temporal extent of Cre-mediated recombination.

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A global double-fluorescent Cre reporter mouse. These results reveal that PA-Cre 30 is. To determine the time of onset of Cre activity Thy1-Cre transgenic mice were time-mated with ZAP Lobe et al 1999 or ROSA26 Soriano 1999 reporter mice. The resultant allele Mcm3-lox was intended as a conditional KO as Mcm3 expression could be ablated with Cre recombinase. β-Galactosidase staining of 105 dpc embryos is done in whole mount.

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These Ai9 mice are useful as a Cre reporter strain - expressing tdTomato fluorescence following Cre-mediated recombination. The resultant allele Mcm3-lox was intended as a conditional KO as Mcm3 expression could be ablated with Cre recombinase. Terization of Cre expression in each different mouse model is therefore essential to generate meaningful data. A A modified mouse Mcm3 allele was designed with loxP sites flanking exons 1417 and a luciferase reporter inserted at the 3 UTR under the control of an IRES element. Tissue specific expression eg CNS pancreas etc of CRE-Luc reporter.

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The CreloxP system has been used exten-sively for conditional mutagenesis in mice. The day of the vaginal plug was defined as embryonic day 0 and tissues from newborn and embryonic mice were processed for ISH or β-gal and alkaline phosphatase staining as described Lobe et al 1999. Tissue specific expression eg CNS pancreas etc of CRE-Luc reporter. This dual labeling allows the visualization of mitotic events cell shapes and intracellular vesicle behaviors. The resultant allele Mcm3-lox was intended as a conditional KO as Mcm3 expression could be ablated with Cre recombinase.

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Terization of Cre expression in each different mouse model is therefore essential to generate meaningful data. As successful CreloxP genome alteration depends on Cre-driver mice Cre-reporter mice are essential for validation of Cre gene expression in vivo. 38 kDa Cre recombinase recognizes the loxP sites of specific 34 bp DNA sequences. However there is currently no established database of the reporter mouse lines available for live imaging such as the Cre transgenic lines Cre-X-Mice. β-Galactosidase staining of 105 dpc embryos is done in whole mount.

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So far the most commonly used locus for generating Cre-responder mice is the Gt ROSA26Sor Rosa26 locus 17. Here we generate a R26 dual fluorescent protein reporter mouse activated by Cre-mediated DNA recombination labeling target cells with a chromatin-specific enhanced green fluorescence protein EGFP and a plasma membrane-anchored monomeric cherry fluorescent protein mCherry. CRE-Luc GPCR Reporter Mouse Platform An in vitroin vivo luciferase reporter platform for profiling of leads in GPCR drug development. Tissue specific expression eg CNS pancreas etc of CRE-Luc reporter. The Allen Institute for Brain Science AIBS website has specific characterization information for several Cre Driver and Cre Reporter lines.

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The day of the vaginal plug was defined as embryonic day 0 and tissues from newborn and embryonic mice were processed for ISH or β-gal and alkaline phosphatase staining as described Lobe et al 1999. The CreloxP system has been used extensively for conditional mutagenesis in mice. Her e we describe mTmG a double-ßuores cent Cre reporter mouse that expre sses membrane-targeted tandem. By using the CreloxP system a series of double reporter mice expressing a combination of reporter genes including CAG-CAT-Z chloramphenicol acetyltransferaselacZ 51 ZEG lacZEGFP 52 ZAP lacZhuman alkaline phosphatase 53 have been generated. In most Cre-reporter mouse.

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Spatial information on Cre recombinase activity can be gained using Cre reporter mice in which a reporter gene eg GFP YFP lacZ is inserted at a ubiquitously expressed locus but preceded by a loxP-flanked transcriptional termination. Her e we describe mTmG a double-ßuores cent Cre reporter mouse that expre sses membrane-targeted tandem. C Representative confocal images show that the Rosa26-based Cre reporter line Ai95 expresses GCaMP6f in cholinergic neurons when crossed to Chat-IRES-Cre mice however native GCaMP6f fluorescence in fixed sections is undetectable compared to TIGRE20 lines compare panels A. Here we describe mTmG a double-fluorescent Cre reporter mouse that expresses membrane-targeted tand. The CreloxP system is a strategy for controlling temporal andor spatial gene expression through genome alteration in mice.

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A panel of luciferase reporter mice to assay GPCR ligand binding and pathway activation in various tissues. Also we found that the mice injected with PA-Cre 30 showed higher recombination efficiency and tdTomato reporter expressions than the original PA-Cre. Ent reporter mouse lines that express a variety of fluorescent markers for imaging. Importantly the donating investigator reports that very low levels of tdTomato expression may be present prior to introduction of Cre recombinase - but the tdTomato expression levels after Cre recombination are significantly greater than those baseline levels. The resultant allele Mcm3-lox was intended as a conditional KO as Mcm3 expression could be ablated with Cre recombinase.

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In principle one mouse must have a tissue-specific driven cre gene and another mouse have loxP flanked floxed alleles of interest gene. Here we describe mTmG a double-fluorescent Cre reporter mouse that expresses membrane-targeted tandem dimer Tomato mT prior to Cre-mediated excision and. The JAX Cre Repository uses a lacZ Cre-reporter strain B6129S4-GtROSA26Sor tm1Sor J to assess cre activity. A An overview of Cre-loxP system. Her e we describe mTmG a double-ßuores cent Cre reporter mouse that expre sses membrane-targeted tandem.

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The resultant allele Mcm3-lox was intended as a conditional KO as Mcm3 expression could be ablated with Cre recombinase. Tissue specific expression eg CNS pancreas etc of CRE-Luc reporter. Spatial information on Cre recombinase activity can be gained using Cre reporter mice in which a reporter gene eg GFP YFP lacZ is inserted at a ubiquitously expressed locus but preceded by a loxP-flanked transcriptional termination. The day of the vaginal plug was defined as embryonic day 0 and tissues from newborn and embryonic mice were processed for ISH or β-gal and alkaline phosphatase staining as described Lobe et al 1999. Here we describe mTmG a double-fluorescent Cre reporter mouse that expresses membrane-targeted tandem dimer Tomato mT prior to Cre-mediated excision and.

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Because of tissue size 155 dpc embryos postnatal day 7 pups and 8 week old adult mice are cryo-sectioned prior to staining of frozen sections. So far the most commonly used locus for generating Cre-responder mice is the Gt ROSA26Sor Rosa26 locus 17. Expressing the red fluorescent protein variant tdTomato following Cre-mediated recombination. The resultant allele Mcm3-lox was intended as a conditional KO as Mcm3 expression could be ablated with Cre recombinase. Because of tissue size 155 dpc embryos postnatal day 7 pups and 8 week old adult mice are cryo-sectioned prior to staining of frozen sections.

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In most Cre-reporter mouse. The Allen Institute for Brain Science AIBS website has specific characterization information for several Cre Driver and Cre Reporter lines. A An overview of Cre-loxP system. A A modified mouse Mcm3 allele was designed with loxP sites flanking exons 1417 and a luciferase reporter inserted at the 3 UTR under the control of an IRES element. Tissue specific expression eg CNS pancreas etc of CRE-Luc reporter.

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These Cre random reporter mice are capable of monitoring Cre activity in diverse tissues and cell types. In principle one mouse must have a tissue-specific driven cre gene and another mouse have loxP flanked floxed alleles of interest gene. Because of tissue size 155 dpc embryos postnatal day 7 pups and 8 week old adult mice are cryo-sectioned prior to staining of frozen sections. To determine the time of onset of Cre activity Thy1-Cre transgenic mice were time-mated with ZAP Lobe et al 1999 or ROSA26 Soriano 1999 reporter mice. C Representative confocal images show that the Rosa26-based Cre reporter line Ai95 expresses GCaMP6f in cholinergic neurons when crossed to Chat-IRES-Cre mice however native GCaMP6f fluorescence in fixed sections is undetectable compared to TIGRE20 lines compare panels A.

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Reporters of Cre activity are important for defining the spatial and temporal extent of Cre-mediated recombination. These Ai9 mice are useful as a Cre reporter strain. A A modified mouse Mcm3 allele was designed with loxP sites flanking exons 1417 and a luciferase reporter inserted at the 3 UTR under the control of an IRES element. The CreloxP system is a strategy for controlling temporal andor spatial gene expression through genome alteration in mice. As successful CreloxP genome alteration depends on Cre-driver mice Cre-reporter mice are essential for validation of Cre gene expression in vivo.

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These Cre random reporter mice are capable of monitoring Cre activity in diverse tissues and cell types. Tissue specific expression eg CNS pancreas etc of CRE-Luc reporter. Because of tissue size 155 dpc embryos postnatal day 7 pups and 8 week old adult mice are cryo-sectioned prior to staining of frozen sections. Terization of Cre expression in each different mouse model is therefore essential to generate meaningful data. Here we describe mTmG a double-fluorescent Cre reporter mouse that expresses membrane-targeted tandem dimer Tomato mT prior to Cre-mediated excision and.

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Terization of Cre expression in each different mouse model is therefore essential to generate meaningful data. The day of the vaginal plug was defined as embryonic day 0 and tissues from newborn and embryonic mice were processed for ISH or β-gal and alkaline phosphatase staining as described Lobe et al 1999. Also we found that the mice injected with PA-Cre 30 showed higher recombination efficiency and tdTomato reporter expressions than the original PA-Cre. The CreloxP system has been used extensively for conditional mutagenesis in mice. In principle one mouse must have a tissue-specific driven cre gene and another mouse have loxP flanked floxed alleles of interest gene.

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To determine the time of onset of Cre activity Thy1-Cre transgenic mice were time-mated with ZAP Lobe et al 1999 or ROSA26 Soriano 1999 reporter mice. Terization of Cre expression in each different mouse model is therefore essential to generate meaningful data. The resultant allele Mcm3-lox was intended as a conditional KO as Mcm3 expression could be ablated with Cre recombinase. These Ai9 mice are useful as a Cre reporter strain - expressing tdTomato fluorescence following Cre-mediated recombination. Sively for conditional mutagenesis in mice.

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