Literature DB >> 34074768

Cell-type-specific, multicolor labeling of endogenous proteins with split fluorescent protein tags in Drosophila.

Rie Kamiyama1, Kota Banzai1, Peiwei Liu1, Abhijit Marar2, Ryo Tamura1, Fangchao Jiang3, Miyuki A Fitch1, Jin Xie3, Daichi Kamiyama4.   

Abstract

The impact of the Drosophila experimental system on studies of modern biology cannot be understated. The ability to tag endogenously expressed proteins is essential to maximize the use of this model organism. Here, we describe a method for labeling endogenous proteins with self-complementing split fluorescent proteins (split FPs) in a cell-type-specific manner in Drosophila A short fragment of an FP coding sequence is inserted into a specific genomic locus while the remainder of the FP is expressed using an available GAL4 driver line. In consequence, complementation fluorescence allows examination of protein localization in particular cells. Besides, when inserting tandem repeats of the short FP fragment at the same genomic locus, we can substantially enhance the fluorescence signal. The enhanced signal is of great value in live-cell imaging at the subcellular level. We can also accomplish a multicolor labeling system with orthogonal split FPs. However, other orthogonal split FPs do not function for in vivo imaging besides split GFP. Through protein engineering and in vivo functional studies, we report a red split FP that we can use for duplexed visualization of endogenous proteins in intricate Drosophila tissues. Using the two orthogonal split FP systems, we have simultaneously imaged proteins that reside in distinct subsynaptic compartments. Our approach allows us to study the proximity between and localization of multiple proteins endogenously expressed in essentially any cell type in Drosophila.

Entities:  

Keywords:  Drosophila; fluorescence microscopy; fluorescent protein; neuron; tissue

Mesh:

Substances:

Year:  2021        PMID: 34074768      PMCID: PMC8201798          DOI: 10.1073/pnas.2024690118

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  72 in total

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2.  Spatiotemporal Monitoring of Pseudomonas syringae Effectors via Type III Secretion Using Split Fluorescent Protein Fragments.

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3.  Improving the photostability of bright monomeric orange and red fluorescent proteins.

Authors:  Nathan C Shaner; Michael Z Lin; Michael R McKeown; Paul A Steinbach; Kristin L Hazelwood; Michael W Davidson; Roger Y Tsien
Journal:  Nat Methods       Date:  2008-05-04       Impact factor: 28.547

4.  Efa6 protects axons and regulates their growth and branching by inhibiting microtubule polymerisation at the cortex.

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Journal:  Elife       Date:  2019-11-13       Impact factor: 8.140

5.  Dscam expression levels determine presynaptic arbor sizes in Drosophila sensory neurons.

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6.  Structural Insight into the Photochemistry of Split Green Fluorescent Proteins: A Unique Role for a His-Tag.

Authors:  Alan Deng; Steven G Boxer
Journal:  J Am Chem Soc       Date:  2017-12-21       Impact factor: 15.419

Review 7.  Imaging dynamic cell signaling in vivo with new classes of fluorescent reporters.

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Journal:  Curr Opin Chem Biol       Date:  2019-11-01       Impact factor: 8.822

Review 8.  Bimolecular fluorescence complementation (BiFC) analysis as a probe of protein interactions in living cells.

Authors:  Tom K Kerppola
Journal:  Annu Rev Biophys       Date:  2008       Impact factor: 12.981

9.  A rapidly maturing far-red derivative of DsRed-Express2 for whole-cell labeling.

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Journal:  Biochemistry       Date:  2009-09-08       Impact factor: 3.162

10.  Genome engineering of Drosophila with the CRISPR RNA-guided Cas9 nuclease.

Authors:  Scott J Gratz; Alexander M Cummings; Jennifer N Nguyen; Danielle C Hamm; Laura K Donohue; Melissa M Harrison; Jill Wildonger; Kate M O'Connor-Giles
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  1 in total

1.  A Genetic Toolkit for Simultaneous Generation of LexA- and QF-Expressing Clones in Selected Cell Types in Drosophila.

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  1 in total

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