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Localization of sucrose synthase and callose in freeze-substituted secondary-wall-stage cotton fibers

机译:蔗糖合酶和call糖在冷冻取代的次生壁棉纤维中的定位

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摘要

Methods for cryogenic fixation, freeze substitution, and embedding were developed to preserve the cellular structure and protein localization of secondary-wall-stage cotton (Gossypium hirsutum L.) fibers accurately for the first time. Perturbation by specimen handling was minimized by freezing fibers still attached to a seed fragment within 2 min after removal of seeds from a boll still attached to the plant. These methods revealed native ultrastructure, including numerous active Golgi bodies, multivesicular bodies, and proplastids. Immunolocalization in the context of accurate structure was accomplished after freeze substitution in acetone only. Quantitation of immunolabeling identified sucrose synthase both near the cortical microtubules and plasma membrane and in a proximal exoplasmic zone about 0.2 μm thick. Immunolabeling also showed that callose (β-1,3-glucan) was codistributed with sucrose synthase within this exoplasmic zone. Similar results were obtained from cultured cotton fibers. The distribution of sucrose synthase is consistent with its having a dual role in cellulose and callose synthesis in secondary-wall-stage cotton fibers.
机译:开发了低温固定,冷冻替代和包埋的方法,以首次精确地保留次壁阶段棉(陆地棉)纤维的细胞结构和蛋白质定位。从仍然附着在植物上的棉铃中取出种子后2分钟内,将仍然附着在种子碎片上的纤维冷冻,从而将样品处理引起的干扰降到最低。这些方法揭示了天然的超微结构,包括许多活跃的高尔基体,多囊体和质体。仅在丙酮中冷冻替代后,即可在准确结构的背景下进行免疫定位。免疫标记的定量可在皮层微管和质膜附近以及约0.2μm厚的近端胞质区中识别出蔗糖合酶。免疫标记法还显示call质(β-1,3-葡聚糖)与蔗糖合酶在该胞质区内共分布。从培养的棉纤维获得类似的结果。蔗糖合酶的分布与其在次级壁阶段棉纤维中的纤维素和call质合成中具有双重作用一致。

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