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荧光标记肌动蛋白在活体盘基网柄菌变形虫中的空间分布。

Spatial distribution of fluorescently labeled actin in living Dictyostelium amoebae.

作者信息

Yumura S

机构信息

Department of Biology, Faculty of Science, Yamaguchi University, Japan.

出版信息

Cell Struct Funct. 1996 Jun;21(3):189-97. doi: 10.1247/csf.21.189.

Abstract

Actin from Dictyostelium was labeled with iodoacetamide tetramethylrhodamine (IAR). The labeled actin retained the ability to polymerize into filaments. The labeled actin was introduced into Dictyostelium cells by electroporation. The introduced IAR-labeled actin was diffusely distributed in the cytoplasm but some of it was concentrated in small and large projections at the cell periphery. IAR-labeled actin was concentrated in pseudopods and in the tail cortical region in actively migrating cells. Intense fluorescence due to labeled actin appeared rapidly and disappeared during the extension and retention of pseudopods. During cytokinesis, IAR-labeled actin was concentrated in both polar regions and slightly concentrated in the furrow region. However, the ratio of intensities due to IAR-labeled actin and fluorescently labeled bovine serum albumin that had been introduced simultaneously into cells showed the absence of any concentration of IAR-labeled actin in the furrow region. Staining of fixed cells with fluorescently labeled phalloidin revealed that filamentous actin was rich in the furrow region. These observations indicate that actin is concentrated at this region in higher ratio of filamentous actin to monomeric actin than in other regions of the cytoplasm. Image analysis revealed that the concentration of IAR-labeled actin was high in a pseudopod of an actively migrating cell. Comparisons with staining by fluorescently labeled phalloidin of fixed cells revealed that there was a decreasing gradient in the concentration of filamentous actin from the tip to the base of a pseudopod. These results reveal the high rate at which actin is coordinately organized during mitosis and locomotion in highly motile Dictyostelium cells.

摘要

用碘乙酰胺四甲基罗丹明(IAR)标记盘基网柄菌的肌动蛋白。标记后的肌动蛋白保留了聚合成丝的能力。通过电穿孔将标记的肌动蛋白导入盘基网柄菌细胞。导入的IAR标记肌动蛋白在细胞质中呈弥散分布,但其中一些集中在细胞周边的大小突起中。在活跃迁移的细胞中,IAR标记肌动蛋白集中在伪足和尾部皮质区域。在伪足伸展和保留期间,标记肌动蛋白产生的强烈荧光迅速出现并消失。在胞质分裂期间,IAR标记肌动蛋白集中在两个极区,并在沟区略有集中。然而,同时导入细胞的IAR标记肌动蛋白和荧光标记牛血清白蛋白的强度比显示,沟区不存在IAR标记肌动蛋白的任何集中现象。用荧光标记的鬼笔环肽对固定细胞进行染色显示,丝状肌动蛋白在沟区丰富。这些观察结果表明,与细胞质的其他区域相比,肌动蛋白在该区域以更高的丝状肌动蛋白与单体肌动蛋白比例集中。图像分析显示,在活跃迁移细胞的伪足中,IAR标记肌动蛋白的浓度很高。与固定细胞用荧光标记鬼笔环肽染色的比较显示,从伪足顶端到基部,丝状肌动蛋白的浓度存在递减梯度。这些结果揭示了在高度运动的盘基网柄菌细胞有丝分裂和运动过程中肌动蛋白协同组织的高速率。

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