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Membrane assembly modulates the stability of the meiotic spindle-pole body

机译:膜组件调节减数分裂纺锤体的稳定性

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摘要

Spore formation in Saccharomyces cerevisiae is driven by de novo assembly of new membranes termed prospore membranes. A vesicle-docking complex called the meiosis II outer plaque (MOP) forms on the cytoplasmic faces of the spindle-pole bodies at the onset of meiosis II and serves as the initiation site for membrane formation. In this study, a fluorescence-recovery assay was used to demonstrate that the dynamics of the MOP proteins change coincident with the coalescence of precursor vesicles into a membrane. Proteins within the MOP exchange freely with a soluble pool prior to membrane assembly, but after membranes are formed they remain stably within the MOP. By contrast, constitutive spindle-pole-body proteins display low exchange in both conditions. The MOP component Ady4p plays a role in maintaining the integrity of the MOP complex, but this role differs depending on whether the MOP is associated with docked vesicles or a fully formed membrane. These results suggest an architectural rearrangement of the MOP coincident with vesicle fusion.
机译:酿酒酵母中的孢子形成是由新膜的重新组装(称为新孢子膜)驱动的。在减数分裂II发生时,纺锤体的胞质表面上形成了称为减数分裂II外噬斑(MOP)的囊泡对接复合物,并作为膜形成的起始位点。在这项研究中,使用了荧光恢复测定法来证明MOP蛋白的动力学变化与前体囊泡聚结成膜相一致。在膜组装之前,MOP中的蛋白质与可溶性库自由交换,但是在膜形成后,它们稳定地保留在MOP中。相比之下,组成性纺锤极体蛋白在两种情况下均显示出低交换。 MOP组分Ady4p在维持MOP复合体的完整性中发挥作用,但是该作用因MOP是与对接的囊泡还是完整的膜相关而有所不同。这些结果表明MOP的体系结构重排与囊泡融合。

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