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苔藓角齿藓原丝体中的微丝分布

Microfilament distribution in protonemata of the moss Ceratodon.

作者信息

Walker L M, Sack F D

机构信息

Department of Plant Biology, The Ohio State University, Columbus, USA.

出版信息

Protoplasma. 1995;189(3-4):229-37. doi: 10.1007/BF01280177.

Abstract

Microfilaments were visualized in dark-grown protonemata of the moss Ceratodon to assess their possible role in tip growth and gravitropism. The relative effectiveness of rhodamine phalloidin (with or without m-maleimidobenzoyl-N-hydroxysuccinimide ester (MBS)) and of immunofluorescence (using the C4 antibody) was evaluated for actin localization in the same cell type. Using immunofluorescence, microfilaments were primarily in an axial orientation within the apical cell. However, a more complex network of microfilaments was observed using rhodamine phalloidin after MBS pretreatment, especially when viewed by confocal laser scanning microscopy. This method revealed a rich three dimensional network of fine microfilaments throughout the apical cell, including the extreme apex. Although there were numerous internal microfilaments, peripheral microfilaments were more abundant. No major redistribution of microfilaments was detected after gravistimulation. The combination of MBS, rhodamine phalloidin, and confocal laser scanning microscopy preserves and reveals microfilaments remarkably well and documents perhaps the most extensive F-actin network visualized to date in any tip-growing cell.

摘要

在藓类植物角齿藓黑暗生长的原丝体中观察微丝,以评估它们在顶端生长和向重力性中可能发挥的作用。评估了罗丹明鬼笔环肽(有或没有间马来酰亚胺苯甲酰 - N - 羟基琥珀酰亚胺酯(MBS))和免疫荧光(使用C4抗体)在同一细胞类型中对肌动蛋白定位的相对有效性。使用免疫荧光法,微丝主要在顶端细胞内呈轴向排列。然而,在MBS预处理后使用罗丹明鬼笔环肽观察到更复杂的微丝网络,尤其是通过共聚焦激光扫描显微镜观察时。该方法揭示了整个顶端细胞,包括顶端最前端,存在丰富的三维精细微丝网络。虽然有许多内部微丝,但周边微丝更为丰富。重力刺激后未检测到微丝的主要重新分布。MBS、罗丹明鬼笔环肽和共聚焦激光扫描显微镜的结合能很好地保存和显示微丝,并记录了迄今为止在任何顶端生长细胞中观察到的最广泛的F - 肌动蛋白网络。

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