Establishing super-resolution imaging for proteins in diatom biosilica

被引:17
作者
Groger, Philip [1 ]
Poulsen, Nicole [1 ]
Klemm, Jennifer [1 ]
Kroger, Nils [1 ,2 ]
Schlierf, Michael [1 ]
机构
[1] Tech Univ Dresden, B CUBE Ctr Mol Bioengn, Arnoldstr 18, D-01307 Dresden, Germany
[2] Tech Univ Dresden, Dept Chem & Food Chem, Arnoldstr 18, D-01307 Dresden, Germany
关键词
FLUORESCENT PROTEINS; THALASSIOSIRA-PSEUDONANA; ELECTRON-MICROSCOPY; LIGHT; RESOLUTION; SILAFFINS; UV;
D O I
10.1038/srep36824
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
The intricate, genetically controlled biosilica nano- and micropatterns produced by diatoms are a testimony for biology's ability to control mineral formation (biomineralization) at the nanoscale and regarded as paradigm for nanotechnology. Previously, several protein families involved in diatom biosilica formation have been identified, and many of them remain tightly associated with the final biosilica structure. Determining the locations of biosilica-associated proteins with high precision is, therefore expected to provide clues to their roles in biosilica morphogenesis. To achieve this, we introduce here single-molecule localization microscopy to diatoms based on photo-activated light microscopy (PALM) to overcome the diffraction limit. We identified six photo-convertible fluorescent proteins (FPs) that can be utilized for PALM in the cytoplasm of model diatom Thalassiosira pseudonana. However, only three FPs were also functional when embedded in diatom biosilica. These were employed for PALM-based localization of the diatom biosilica-associated protein Silaffin-3 (tpSil3) with a mean precision of 25 nm. This allowed for the identification of distinct accumulation areas of Sil3 in the biosilica, which cannot be resolved by confocal fluorescence microscopy. The enhanced microscopy technique introduced here for diatoms will aid in elucidating the molecular mechanism of silica biomineralization as well as other aspects of diatom cell biology.
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页数:8
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