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Myosin II is not required for Drosophila tracheal branch elongation and cell intercalation

机译:果蝇II不需要果蝇气管分支伸长率和细胞嵌入

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摘要

The Drosophila tracheal system consists of an interconnected network of monolayered epithelial tubes that ensures oxygen transport in the larval and adult body. During tracheal dorsal branch (DB) development, individual DBs elongate as a cluster of cells, led by tip cells at the front and trailing cells in the rear. Branch elongation is accompanied by extensive cell intercalation and cell lengthening of the trailing stalk cells. Although cell intercalation is governed by Myosin II (MyoII)-dependent forces during tissue elongation in the Drosophila embryo that lead to germ-band extension, it remained unclear whether MyoII plays a similar active role during tracheal branch elongation and intercalation. Here, we have used a nanobody-based approach to selectively knock down MyoII in tracheal cells. Our data show that, despite the depletion of MyoII function, tip cell migration and stalk cell intercalation (SCI) proceed at a normal rate. This confirms a model in which DB elongation and SCI in the trachea occur as a consequence of tip cell migration, which produces the necessary forces for the branching process.
机译:果蝇气管系统由互连的单层上皮管组成,可确保幼虫和成人体内的氧气运输。在气管背部分支(DB)开发期间,单独的DBS作为一组细胞,由前部的前部和后尾电池处的尖端电池引起。分支伸长率伴随着尾茎细胞的广泛细胞嵌入和细胞延长。虽然细胞嵌入受肌球蛋白II(MyoII) - 在果蝇胚胎中的组织伸长期间的依赖性,但导致生殖器延伸的组织伸长,但它仍然不清楚MyoII在气管分支伸长率和嵌入期间在气管伸长和嵌入中发挥着类似的积极作用。在这里,我们使用了基于纳米体的方法来选择性地击落气管细胞中的myOI。我们的数据表明,尽管MyoI函数的耗尽,尖端单元迁移和茎电池嵌入(SCI)以正常速率进行。这证实了一种模型,其中气管中的DB伸长率和SCI作为尖端电池迁移发生,这产生了支化过程的必要力。

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