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Summary

XB-LINE-1914

Line Name: Xtr.Tg(mlc2:dnfosl1-eGFP)Qi

Line Images

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Whole heart isolated from adult Xtr.Tg(mlc2:DNfosl1-EGFP) line frog, at 3 days post injury, showing eGFP fluorescence in cardiomyocytes of the heart ventricle.

Validation of eGFP expression in the ventricular section from the dnFosl1 heart

Summary

Synonym: Xtr.Tg(Mlc2-dnFosl1-T2A-EGFP)

Species: Xenopus tropicalis

Background Strain: Unknown

Paternal Line:

Maternal Line:

Description: Fosl1 protein was mutated and truncated to generate 3 mutant polypeptides which then cloned into pcDNA3.1 plasmid (pcDNA-Fosl1-NT, pcDNA-Fosl1∆DB, and pcDNA-Fosl1∆LZ ). Full length of Fos, FosB, and Fosl2 were amplified from X. tropicalis cDNA library and cloned into pcDNA3 plasmid to construct pcDNA-Fos, pcDNA-FosB, and pcDNA-Fosl2 plasmids. Fosl1-NT with the maximum capacity to inhibit Fosl1-driven luciferase activity was used as the dnFosl1 due to its safety for other Fos proteins The DNA fragment of dnFosl1 was then fused with a T2A-EGFP coding sequence and cloned into a I-SceI transgenesis vector downstream of the 3 kb mlc2 promoter to construct the transgenesis plasmid pMlc2-dnFosl1-T2A-EGFP. The transgenesis plasmid and I-Sce1 enzyme were then injected into the animal pole of X. tropicalis embryos at one-cell stage to generate a transgenic line. Founder X. tropicalis were identified and propagated to establish this stable line.

Phenotype Description: Adult frogs have eGFP expression in cardiac myocytes of the heart ventricle.

Color Morph: pigmented

Breeding Type: OUTBRED

Lab of Origin: Qi lab, Key Laboratory of Regenerative Medicine

Line Type: Mutant, Transgenic

Mutated Gene(s): fosl1

MTA Required: No

Public: Yes

Catalogue Number:

Stock Center RRID Generation Availability Mutant Details Information

NXR (US)

EXRC (Europe)

NBRP (Japan)

XLRRI (US)

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Summary
Synonym:	Xtr.Tg(Mlc2-dnFosl1-T2A-EGFP)
Species:	Xenopus tropicalis
Background Strain:	Unknown
Paternal Line:
Maternal Line:
Description:	Fosl1 protein was mutated and truncated to generate 3 mutant polypeptides which then cloned into pcDNA3.1 plasmid (pcDNA-Fosl1-NT, pcDNA-Fosl1∆DB, and pcDNA-Fosl1∆LZ ). Full length of Fos, FosB, and Fosl2 were amplified from X. tropicalis cDNA library and cloned into pcDNA3 plasmid to construct pcDNA-Fos, pcDNA-FosB, and pcDNA-Fosl2 plasmids. Fosl1-NT with the maximum capacity to inhibit Fosl1-driven luciferase activity was used as the dnFosl1 due to its safety for other Fos proteins The DNA fragment of dnFosl1 was then fused with a T2A-EGFP coding sequence and cloned into a I-SceI transgenesis vector downstream of the 3 kb mlc2 promoter to construct the transgenesis plasmid pMlc2-dnFosl1-T2A-EGFP. The transgenesis plasmid and I-Sce1 enzyme were then injected into the animal pole of X. tropicalis embryos at one-cell stage to generate a transgenic line. Founder X. tropicalis were identified and propagated to establish this stable line.
Phenotype Description:	Adult frogs have eGFP expression in cardiac myocytes of the heart ventricle.
Color Morph:	pigmented
Breeding Type:	OUTBRED
Lab of Origin:	Qi lab, Key Laboratory of Regenerative Medicine
Line Type:	Mutant, Transgenic
Mutated Gene(s):	fosl1
MTA Required:	No
Public:	Yes
Catalogue Number: