Analysis of Water-Soluble Proteins by Two-Dimensional Electrophoresis in the Encystment Process of Colpoda cucullus Nag-1 and Cytoskeletal Dynamics

Assays of protein contained in water-soluble fraction of encysting cells Colpoda cucullus Nag-1 by two-dimensional electrophoresis (2-D PAGE) and mass spectrometry (MS) revealed that the amount of β-tubulin abruptly increased in 2.5–10 h after encystment induction. Judging from the results that tota...

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Bibliographic Details
Published inActa protozoologica Vol. 59; no. 3-4; pp. 107 - 120
Main Authors Sogame, Yoichiro, Kojima, Katsuhiko, Takeshita, Toshikazu, Kikuchi, Shiho, Shimada, Yuto, Nakamura, Rikiya, Arikawa, Mikihiko, Miyata, Seiji, Kinoshita, Eiji, Suizu, Futoshi, Matsuoka, Tatsuomi
Format Journal Article
LanguageEnglish
Published Warsaw Jagiellonian University-Jagiellonian University Press 01.03.2021
Subjects
Acids
Actin
Analytical methods
Cells
Cilia
Colpoda cucullus
Cysts
Cytoskeleton
Dynamics
Electrophoresis
Encystment
Gene expression
Immunofluorescence
Kinases
Mass spectrometry
Mass spectroscopy
Microscopy
Microtubules
Paclitaxel
Phalloidin
Phosphorylation
Proteins
Scientific imaging
Tubulin
Water analysis
United Kingdom > UK
United States > US
Japan
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Summary:Assays of protein contained in water-soluble fraction of encysting cells Colpoda cucullus Nag-1 by two-dimensional electrophoresis (2-D PAGE) and mass spectrometry (MS) revealed that the amount of β-tubulin abruptly increased in 2.5–10 h after encystment induction. Judging from the results that total α-tubulin content did not decrease much until 12 h after encystment induction, the result indicates that disassembly of microtubules may occur soon after encystment is induced. Therefore, we tried to visualize dynamics of microtubules. Immunofluorescence microscopy using anti-α-tubulin antibody indicated that disassembly of axonemal microtubules of cilia became within 1.5 h after encystment induction, and resorbed in 3 days. Although the cytoplasmic microtubules failed to be visualized clearly, encystmentdependent globulation of cells was promoted by taxol, an inhibitor of disassembly of microtubules. It is possible that a temporary formation of cytoplasmic microtubules may be involved in cell globulation. The phosphorylation level of actin (43 kDa) became slightly elevated just after encystment induction. Lepidosomes, the sticky small globes surrounding encysting cells, were vividly stained with Acti-stain 555 phalloidin, suggesting that 43-kDa actin or its homologues may be contained in lepidosomes.
ISSN:0065-1583
1689-0027
DOI:10.4467/16890027AP.20.009.13264