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动粒微管通过前中期染色体动粒处亚基的丢失而缩短。

Kinetochore microtubules shorten by loss of subunits at the kinetochores of prometaphase chromosomes.

作者信息

Cassimeris L, Salmon E D

机构信息

Department of Biology, University of North Carolina, Chapel Hill 27599-3280.

出版信息

J Cell Sci. 1991 Feb;98 ( Pt 2):151-8. doi: 10.1242/jcs.98.2.151.

Abstract

The site of tubulin subunit dissociation was determined during poleward chromosome movement in prometaphase newt lung cell mitotic spindles using fluorescence photobleaching techniques and nocodazole-induced spindle shortening. Synchronous shortening of all kinetochore microtubules was produced by incubating cells in 17 microM nocodazole to block microtubule assembly. Under these conditions the spindle poles moved towards the metaphase plate at a rate of 3.6 +/- 0.4 microns min-1 (n = 3). On the basis of anti-tubulin immunofluorescent staining of cells fixed after incubation in nocodazole, we found that nonkinetochore microtubules rapidly disappeared and only kinetochore fibers were present after 60-90 s in nocodazole. To localize the site of tubulin subunit dissociation, a narrow bar pattern was photobleached across one half-spindle in prometaphase-metaphase cells previously microinjected with 5-(4,6-dichlorotriazin-2-yl) amino fluorescein (DTAF)-labeled tubulin. Immediately after photobleaching, cells were perfused with 17 microM nocodazole to produce shortening of kinetochore microtubules. Shortening was accompanied by a decrease in the distance between the bleach bar and the kinetochores. In contrast, there was little or no decrease in the distance between the bleach bar and the pole. Compared to their initial lengths, the average kinetochore to pole distance shortened by 18%, the bleach bar to kinetochore distance shortened by 28% and the average bleached bar to pole distance shortened by 1.6%. The data provide evidence that tubulin subunits dissociate from kinetochore microtubules at a site near the kinetochore during poleward chromosome movement. These results are consistent with models of poleward force generation for chromosome movement in which prometaphase-metaphase poleward force is generated in association with the kinetochore.

摘要

利用荧光漂白技术和诺考达唑诱导的纺锤体缩短,在蝾螈肺细胞有丝分裂纺锤体前中期向极染色体移动过程中,确定了微管蛋白亚基解离的位点。通过将细胞置于17微摩尔/升的诺考达唑中孵育以阻断微管组装,使所有动粒微管同步缩短。在这些条件下,纺锤体极以3.6±0.4微米/分钟的速度移向中期板(n = 3)。基于对在诺考达唑中孵育后固定的细胞进行抗微管蛋白免疫荧光染色,我们发现非动粒微管迅速消失,在诺考达唑中孵育60 - 90秒后仅存在动粒纤维。为了定位微管蛋白亚基解离的位点,在先前显微注射了5 -(4,6 - 二氯三嗪 - 2 - 基)氨基荧光素(DTAF)标记微管蛋白的前中期 - 中期细胞中,在半个纺锤体上对一个窄条图案进行光漂白。光漂白后立即用17微摩尔/升的诺考达唑灌注细胞,以使动粒微管缩短。缩短伴随着漂白条与动粒之间距离的减小。相比之下,漂白条与纺锤体极之间的距离几乎没有减小或没有减小。与它们的初始长度相比,动粒到极的平均距离缩短了18%,漂白条到动粒的距离缩短了28%,平均漂白条到极的距离缩短了1.6%。这些数据提供了证据,表明在向极染色体移动过程中,微管蛋白亚基在靠近动粒的位点从动粒微管上解离。这些结果与染色体移动的向极力产生模型一致,在该模型中,前中期 - 中期向极力与动粒相关产生。

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