Literature DB >> 15732910

Firefly luciferase enzyme fragment complementation for imaging in cells and living animals.

Ramasamy Paulmurugan1, Sanjiv S Gambhir.   

Abstract

We identified different fragments of the firefly luciferase gene based on the crystal structure of firefly luciferase. These split reporter genes which encode for protein fragments, unlike the fragments currently used for studying protein-protein interactions, can self-complement and provide luciferase enzyme activity in different cell lines in culture and in living mice. The comparison of the fragment complementation associated recovery of firefly luciferase enzyme activity with intact firefly luciferase was estimated for different fragment combinations and ranged from 0.01 to 4% of the full firefly luciferase activity. Using a cooled optical charge-coupled device camera, the analysis of firefly luciferase fragment complementation in transiently transfected subcutaneous 293T cell implants in living mice showed significant detectable enzyme activity upon injecting d-luciferin, especially from the combinations of fragments identified (Nfluc and Cfluc are the N and C fragments of the firefly luciferase gene, respectively): Nfluc (1-475)/Cfluc (245-550), Nfluc (1-475)/Cfluc (265-550), and Nfluc (1-475)/Cfluc (300-550). The Cfluc (265-550) fragment, upon expression with the nuclear localization signal (NLS) peptide of SV40, shows reduced enzyme activity when the cells are cotransfected with the Nfluc (1-475) fragment expressed without NLS. We also proved in this study that the complementing fragments could be efficiently used for screening macromolecule delivery vehicles by delivering TAT-Cfluc (265-550) to cells stably expressing Nfluc (1-475) and recovering signal. These complementing fragments should be useful for many reporter-based assays including intracellular localization of proteins, studying cellular macromolecule delivery vehicles, studying cell-cell fusions, and also developing intracellular phosphorylation sensors based on fragment complementation.

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Year:  2005        PMID: 15732910      PMCID: PMC4154832          DOI: 10.1021/ac0484777

Source DB:  PubMed          Journal:  Anal Chem        ISSN: 0003-2700            Impact factor:   6.986


  39 in total

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2.  Monitoring protein-protein interactions in live mammalian cells by beta-galactosidase complementation.

Authors:  F M Rossi; B T Blakely; C A Charlton; H M Blau
Journal:  Methods Enzymol       Date:  2000       Impact factor: 1.600

3.  Protein-protein interactions monitored in mammalian cells via complementation of beta -lactamase enzyme fragments.

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4.  Simultaneous visualization of multiple protein interactions in living cells using multicolor fluorescence complementation analysis.

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5.  Molecular imaging of drug-modulated protein-protein interactions in living subjects.

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6.  Oligomerization domain-directed reassembly of active dihydrofolate reductase from rationally designed fragments.

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Authors:  D L Graham; N Bevan; P N Lowe; M Palmer; S Rees
Journal:  J Biomol Screen       Date:  2001-12

9.  Cloning of firefly luciferase cDNA and the expression of active luciferase in Escherichia coli.

Authors:  J R de Wet; K V Wood; D R Helinski; M DeLuca
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10.  Regulation of Cre recombinase by ligand-induced complementation of inactive fragments.

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  30 in total

1.  Combinatorial library screening for developing an improved split-firefly luciferase fragment-assisted complementation system for studying protein-protein interactions.

Authors:  Ramasamy Paulmurugan; Sanjiv S Gambhir
Journal:  Anal Chem       Date:  2007-02-13       Impact factor: 6.986

2.  Firefly luciferase complementation imaging assay for protein-protein interactions in plants.

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3.  Noninvasive bioluminescence imaging in small animals.

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4.  Ionizing radiation induces prostate cancer neuroendocrine differentiation through interplay of CREB and ATF2: implications for disease progression.

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Journal:  Cancer Res       Date:  2008-12-01       Impact factor: 12.701

5.  Sustained accurate recording of intracellular acidification in living tissues with a photo-controllable bioluminescent protein.

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6.  Microscopy and image analysis.

Authors:  George McNamara; Michael J Difilippantonio; Thomas Ried
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Review 7.  Genetically encodable fluorescent biosensors for tracking signaling dynamics in living cells.

Authors:  Robert H Newman; Matthew D Fosbrink; Jin Zhang
Journal:  Chem Rev       Date:  2011-04-01       Impact factor: 60.622

8.  Lowering of amyloid beta peptide production with a small molecule inhibitor of amyloid-β precursor protein dimerization.

Authors:  Pauline Pl So; Ella Zeldich; Kathleen I Seyb; Mickey M Huang; John B Concannon; Gwendalyn D King; Ci-Di Chen; Gregory D Cuny; Marcie A Glicksman; Carmela R Abraham
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9.  In vitro and in vivo molecular imaging of estrogen receptor α and β homo- and heterodimerization: exploration of new modes of receptor regulation.

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10.  Dynamic analysis of GH receptor conformational changes by split luciferase complementation.

Authors:  Ying Liu; Philip A Berry; Yue Zhang; Jing Jiang; Peter E Lobie; Ramasamy Paulmurugan; John F Langenheim; Wen Y Chen; Kurt R Zinn; Stuart J Frank
Journal:  Mol Endocrinol       Date:  2014-09-04
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