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区分 Bicoid mRNA 定位因子的直接和间接作用。

Distinguishing direct from indirect roles for bicoid mRNA localization factors.

机构信息

UMC Utrecht, Department of Cell Biology, Cell Microscopy Centre, AZU H02.313, Heildelberglaan 100, 3584 CX, Utrecht, The Netherlands.

出版信息

Development. 2010 Jan;137(1):169-76. doi: 10.1242/dev.044867.

Abstract

Localization of bicoid mRNA to the anterior of the Drosophila oocyte is essential for patterning the anteroposterior body axis in the early embryo. bicoid mRNA localizes in a complex multistep process involving transacting factors, molecular motors and cytoskeletal components that remodel extensively during the lifetime of the mRNA. Genetic requirements for several localization factors, including Swallow and Staufen, are well established, but the precise roles of these factors and their relationship to bicoid mRNA transport particles remains unresolved. Here we use live cell imaging, super-resolution microscopy in fixed cells and immunoelectron microscopy on ultrathin frozen sections to study the distribution of Swallow, Staufen, actin and dynein relative to bicoid mRNA during late oogenesis. We show that Swallow and bicoid mRNA are transported independently and are not colocalized at their final destination. Furthermore, Swallow is not required for bicoid transport. Instead, Swallow localizes to the oocyte plasma membrane, in close proximity to actin filaments, and we present evidence that Swallow functions during the late phase of bicoid localization by regulating the actin cytoskeleton. In contrast, Staufen, dynein and bicoid mRNA form nonmembranous, electron dense particles at the oocyte anterior. Our results exclude a role for Swallow in linking bicoid mRNA to the dynein motor. Instead we propose a model for bicoid mRNA localization in which Swallow is transported independently by dynein and contributes indirectly to bicoid mRNA localization by organizing the cytoskeleton, whereas Staufen plays a direct role in dynein-dependent bicoid mRNA transport.

摘要

果蝇卵子中 bicoid mRNA 的定位于胚胎早期的前后体轴模式形成至关重要。bicoid mRNA 的定位涉及多个步骤,涉及反式作用因子、分子马达和细胞骨架成分,这些成分在 mRNA 的寿命内广泛重塑。几个定位因子的遗传要求,包括 Swallow 和 Staufen,已经得到很好的确立,但这些因子的确切作用及其与 bicoid mRNA 运输颗粒的关系仍未解决。在这里,我们使用活细胞成像、固定细胞的超分辨率显微镜和超薄冷冻切片的免疫电子显微镜,研究了在晚期卵发生过程中,Swallow、Staufen、肌动蛋白和动力蛋白相对于 bicoid mRNA 的分布。我们表明,Swallow 和 bicoid mRNA 是独立运输的,并且不在它们的最终目的地共定位。此外,Swallow 不参与 bicoid 的运输。相反,Swallow 定位于卵母细胞质膜,与肌动蛋白丝紧密接近,并且我们提供了证据表明,Swallow 通过调节肌动蛋白细胞骨架在 bicoid 定位的晚期阶段发挥作用。相比之下,Staufen、动力蛋白和 bicoid mRNA 在卵母细胞的前体形成非膜状的、电子致密颗粒。我们的结果排除了 Swallow 将 bicoid mRNA 与动力蛋白连接的作用。相反,我们提出了一个 bicoid mRNA 定位模型,其中 Swallow 由动力蛋白独立运输,并通过组织细胞骨架间接促进 bicoid mRNA 的定位,而 Staufen 在动力蛋白依赖性 bicoid mRNA 运输中发挥直接作用。

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本文引用的文献

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