An optical marker based on the UV-induced green-to-red photoconversion of a fluorescent protein

Ando, Ryoko; Hama, Hiroshi; Yamamoto-Hino, Miki; Mizuno, Hideaki; Miyawaki, Atsushi

doi:10.1073/pnas.202320599

Cited by 946 publications

(896 citation statements)

References 20 publications

(16 reference statements)

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“…To label cellular and subcellular structures, mRNAs encoding the following fusion proteins were injected at one-cell stage after being synthetized with the SP6 mMessenger mMachine kit (Ambion): H2B-mCherry or H2B-GFP (100-150 pg) 47 , Pard3-GFP or Pard3-RFP (50-75 pg) 48,49 , Lyn-EGFP (membrane-GFP 100-150 pg) 50 , membrane-mCherry (100-150 pg) 51 , Lifeact-RFP or Lifeact-GFP (150 pg) 52 , hZO1-GFP (100 pg) 53 , GFP and Kaede (50 pg) 54 . To interfere with endogenous expression, embryos were injected at one-cell stage with 1.6 ng per embryo of emi1 translation blocking morpholino (5 0 -GTAGTTTGGACACTTCATATTGAGG-3 0 ) (ref.…”

Section: Methodsmentioning

confidence: 99%

Mitotic cell rounding and epithelial thinning regulate lumen growth and shape

et al. 2015

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Many organ functions rely on epithelial cavities with particular shapes. Morphogenetic anomalies in these cavities lead to kidney, brain or inner ear diseases. Despite their relevance, the mechanisms regulating lumen dimensions are poorly understood. Here, we perform live imaging of zebrafish inner ear development and quantitatively analyse the dynamics of lumen growth in 3D. Using genetic, chemical and mechanical interferences, we identify two new morphogenetic mechanisms underlying anisotropic lumen growth. The first mechanism involves thinning of the epithelium as the cells change their shape and lose fluids in concert with expansion of the cavity, suggesting an intra-organ fluid redistribution process. In the second mechanism, revealed by laser microsurgery experiments, mitotic rounding cells apicobasally contract the epithelium and mechanically contribute to expansion of the lumen. Since these mechanisms are axis specific, they not only regulate lumen growth but also the shape of the cavity.

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Section: Methodsmentioning

confidence: 99%

Mitotic cell rounding and epithelial thinning regulate lumen growth and shape

et al. 2015

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“…In our experience, the effect of introducing a second UAS transgene on the expression of another is generally minimal. For example, in one case, we expressed homozygous or heterozygous Kaede (a fl uorescent protein, [ 35 ] ) with one or two copies of the elav -GAL4 driver and compared the Kaede intensities in eye discs (Fig. 5a, b ).…”

Section: Different Transgenes and Chromosomal Position Effectsmentioning

confidence: 99%

Morphometric Analysis of Huntington’s Disease Neurodegeneration in Drosophila

Song

Smith

Syed

et al. 2013

Methods in Molecular Biology

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Huntington's disease (HD) is an autosomal dominant neurodegenerative disorder. The HD gene encodes the huntingtin protein (HTT) that contains polyglutamine tracts of variable length. Expansions of the CAG repeat near the amino terminus to encode 40 or more glutamines (polyQ) lead to disease. At least eight other expanded polyQ diseases have been described [1]. HD can be faithfully modeled in Drosophila with the key features of the disease such as late onset, slowly progressing degeneration, formation of abnormal protein aggregates and the dependence on polyQ length being evident. Such invertebrate model organisms provide powerful platforms to explore neurodegenerative mechanisms and to productively speed the identi fi cation of targets and agents that are likely to be effective at treating diseases in humans. Here we describe an optical pseudopupil method that can be readily quanti fi ed to provide a fast and sensitive assay for assessing the degree of HD neurodegeneration in vivo . We discuss detailed crossing schemes as well as factors including different drivers, various constructs, the number of UAS sites, genetic background, and temperature that can in fl uence the result of pseudopupil measurements.

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“…To investigate the role of local b-actin mRNA translation in growth cone turning, Holt and colleagues constructed an axonal translation reporter by fusing the photoconvertible protein, Kaede, to the b-actin 3 0 UTR, which contains cis-acting elements responsible for RNA localization and translational control (Leung et al 2006). Kaede is a fluorescent protein that was isolated from the stony coral, Trachyphyllia geoffroyi, and undergoes an irreversible photoconversion (green to red) on irradiation with UV light that results in a 2000-fold increase in red-to-green fluorescent signal (Ando et al 2002). In growth cones expressing the Kaede reporter, new translation was observed on the side of the growth cone that was closest to an external gradient of the netrin-1 guidance cue (Fig.…”

Section: Fluorescent Protein Reportersmentioning

confidence: 99%

Imaging Translation in Single Cells Using Fluorescent Microscopy

Chao

Yoon

Singer

2012

Cold Spring Harbor Perspectives in Biology

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The regulation of translation provides a mechanism to control not only the abundance of proteins, but also the precise time and subcellular location that they are synthesized. Much of what is known concerning the molecular basis for translational control has been gleaned from experiments (e.g., luciferase assays and polysome analysis) that measure average changes in the protein synthesis of a population of cells, however, mechanistic insights can be obscured in ensemble measurements. The development of fluorescent microscopy techniques and reagents has allowed translation to be studied within its cellular context. Here we highlight recent methodologies that can be used to study global changes in protein synthesis or regulation of specific mRNAs in single cells. Imaging of translation has provided direct evidence for local translation of mRNAs at synapses in neurons and will become an important tool for studying translational control.

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An optical marker based on the UV-induced green-to-red photoconversion of a fluorescent protein

Cited by 946 publications

References 20 publications

Mitotic cell rounding and epithelial thinning regulate lumen growth and shape

Mitotic cell rounding and epithelial thinning regulate lumen growth and shape

Morphometric Analysis of Huntington’s Disease Neurodegeneration in Drosophila

Imaging Translation in Single Cells Using Fluorescent Microscopy

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