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Laser Scanning Confocal Microscopy for Arabidopsis Epidermal, Mesophyll and Vascular Parenchyma Cells.

Bio-protocol (2017-03-05)
Christian Elowsky, Yashitola Wamboldt, Sally Mackenzie
RESUMEN

Investigation of protein targeting to plastids in plants by confocal laser scanning microscopy (CLSM) can be complicated by numerous sources of artifact, ranging from misinterpretations from in vivo protein over-expression, false fluorescence in cells under stress, and organellar mis-identification. Our studies have focused on the plant-specific gene MSH1, which encodes a dual targeting protein that is regulated in its expression and resides within the nucleoid of a specialized plastid type ( Virdi et al., 2016 ). Therefore, our methods have been optimized to study protein dual targeting to mitochondria and plastids, spatial and temporal regulation of protein expression, and sub-organellar localization, producing a protocol and set of experimental standards that others may find useful for such studies.

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Glicerol, for molecular biology, ≥99.0%
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Fosfato de potasio dibasic, ACS reagent, ≥98%
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D-(+)-Glucosa, ≥99.5% (GC)
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Medio basal Murashige y Skoog, powder, suitable for plant cell culture
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Fosfato de potasio monobasic, powder, suitable for cell culture, suitable for insect cell culture, suitable for plant cell culture, ≥99.0%
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Sulfato de amonio, for molecular biology, ≥99.0%
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Cloruro de potasio, for molecular biology, ≥99.0%
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TWEEN® 20, viscous liquid
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Cloruro de calcio dihydrate, BioReagent, suitable for cell culture, suitable for insect cell culture, suitable for plant cell culture, ≥99.0%
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MES hydrate, BioPerformance Certified, suitable for cell culture, ≥99.5%
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3′,5′-Dimethoxy-4′-hydroxyacetophenone, 97%
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Sulfato de magnesio, BioReagent, suitable for cell culture, suitable for insect cell culture
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Seroalbúmina bovina, heat shock fraction, pH 7, ≥98%
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Citrato de sodio tribásico dihydrate, for molecular biology, ≥99%