Abstract
Reporter proteins comprising granzyme B (GrB) fused to eGFP, ecliptic pHluorin or mCherry, were generated and used to study granule (lysosome) distribution and properties in COS-1 cells and natural killer cells. The reporters resembled native GrB in biosynthesis and localization, and accumulated in granules. In live cells both the eGFP and pHluorin reporters were dark in lysosomes, but fluoresced when the granule integrity or pH was perturbed by Leu-Leu methyl ester, hydrogen peroxide, naphthazarin, or sphingosine treatment. By contrast, fluorescence of the mCherry reporter was not pH-dependent. The quenching of eGFP within granules indicates that this commonly-used fluorescent protein is not appropriate as a vital intra-lysosomal marker.
Publication types
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Research Support, Non-U.S. Gov't
MeSH terms
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Animals
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COS Cells
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Cell Line
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Chlorocebus aethiops
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Enzyme Precursors / genetics
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Enzyme Precursors / metabolism
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Genes, Reporter*
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Granzymes / genetics
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Granzymes / metabolism*
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Green Fluorescent Proteins / genetics
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Green Fluorescent Proteins / metabolism
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Humans
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Hydrogen-Ion Concentration
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Killer Cells, Natural
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Luminescent Proteins / genetics
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Luminescent Proteins / metabolism*
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Lysosomes / enzymology*
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Microscopy, Fluorescence
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Protein Sorting Signals
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Protein Transport*
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Recombinant Fusion Proteins / metabolism
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Red Fluorescent Protein
Substances
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Enzyme Precursors
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Luminescent Proteins
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PHluorin
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Protein Sorting Signals
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Recombinant Fusion Proteins
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enhanced green fluorescent protein
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Green Fluorescent Proteins
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GZMB protein, human
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Granzymes