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ID 31915
JaLCDOI
フルテキストURL
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著者
Watanabe, Sadahiro Okayama University
Takehara, Yoshiki Okayama University
Fujii, Yoshitaka Okayama University
Okimasu, Eiji Okayama University
Moromizato, Yasunori Okayama University
Sasaki, Junzo Okayama University Kaken ID publons researchmap
抄録

To investigate the involvement of actin filaments in concanavalin A (Con A)-induced cap formation and cytochalasin B (CB)-induced zeiotic knob migration, the distribution of F-actin was studied in Con A-treated and CB-treated Ehrlich ascites tumor cells (EATC) by fluorescence microscopy using heavy meromyosin conjugated with a fluorescent dye, N-(7-dimethylamino-4-methylcoumarinyl) maleimide, (DACM-HMM). In non-treated cells, the diffuse fluorescence of DACM-HMM was observed in the cytoplasm, particularly intensely under the plasma membrane and around the nucleus. In Con A- and CB-treated cells, the fluorescence was seen at Con A-induced-capped and CB-induced-knob-accumulated regions. This fluorescence was more intense in CB-treated cells. To study the actin filaments in these fluorescent regions more clearly, the soluble components of the cells were eliminated by treatment with Triton X-100 or saponin solution containing a low concentration of glutaraldehyde, and the detergent-treated and saponin-treated cells were observed under a transmission electron microscope. Concentrated actin filaments were observed directly beneath the Con A-induced capping area and CB-induced zeiotic knob-accumulation area. The area of concentrated actin filaments appeared to correspond to the electron dense area observed in the identical region in the cells fixed without detergent treatment. More actin filaments were observed in CB-treated cells than in Con A-treated ones.

キーワード
DACM-HMM
Ehrlich ascites tumor cells
concanavalin A
cytochalasin B
actim
capping
Amo Type
Article
出版物タイトル
Acta Medica Okayama
発行日
1986-12
40巻
6号
出版者
Okayama University Medical School
開始ページ
301
終了ページ
311
ISSN
0386-300X
NCID
AA00508441
資料タイプ
学術雑誌論文
言語
英語
論文のバージョン
publisher
査読
有り
PubMed ID
Web of Science KeyUT