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ASPM and citron kinase co-localize to the midbody ring during cytokinesis.

机译:在胞质分裂过程中,ASPM和柚子激酶共定位于中体环。

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摘要

Mutations in ASPM (abnormal spindle-like microcephaly associated) and citron kinase (CITK) cause primary microcephaly in humans and rodents, respectively. Both proteins are expressed during neurogenesis and play important roles in neuronal progenitor cell division. ASPM is localized to the spindle pole, and is essential for maintaining proliferative cell division. CITK is present at the cytokinesis furrow and midbody ring, and it is essential for cellular abscission. We report here that ASPM also localizes to the midbody ring in mammalian cells. ASPM co-localizes with CITK at the midbody ring and coimmunoprecipitates with CITK in lysates prepared from HeLa cells and embryonic neuroepithelium. Furthermore, a GFP-tagged fragment of the N-terminus of ASPM localizes to centrosomes and spindle poles, while a GFP-tagged fragment of the C-terminus localizes to midbodies. All reported ASPM mutations that cause microcephaly involve a truncation or mutation of the C-terminus. In addition, at least two other microcephaly-related proteins, CENPJ and CDK5RAP2, previously localized to spindle poles, also localize to midbodies. Together our observations support a model of neurogenesis in which spindle dynamics and cellular abscission are coordinated.
机译:ASPM(异常的纺锤状小头畸形)和柚子激酶(CITK)的突变分别导致人类和啮齿动物原发性小头畸形。两种蛋白均在神经发生过程中表达,并在神经元祖细胞分裂中发挥重要作用。 ASPM定位于纺锤极,对于维持增殖性细胞分裂至关重要。 CITK存在于胞质分裂沟和中体环处,对于细胞脱落至关重要。我们在这里报告ASPM还定位到哺乳动物细胞中体环。 ASPM在中体环处与CITK共定位,并在从HeLa细胞和胚胎神经上皮细胞制备的裂解物中与CITK共免疫沉淀。此外,ASPM N末端的一个带GFP标记的片段定位于中心体和纺锤体极,而C末端的一个带GFP标记的片段定位于中体。所有报告的引起小头畸形的ASPM突变都涉及C末端的截短或突变。此外,至少两个其他与小头畸形相关的蛋白,CENPJ和CDK5RAP2,以前定位于纺锤体极,也定位于中体。我们的观察结果共同支持了一种神经发生模型,其中纺锤体动力学和细胞脱落是协调的。

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