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雄性和雌性脊椎动物减数分裂过程中染色质上Rad51分布的动态变化。

Dynamic changes in Rad51 distribution on chromatin during meiosis in male and female vertebrates.

作者信息

Ashley T, Plug A W, Xu J, Solari A J, Reddy G, Golub E I, Ward D C

机构信息

Department of Genetics, Yale University School of Medicine, New Haven, CT 06510, USA.

出版信息

Chromosoma. 1995 Oct;104(1):19-28. doi: 10.1007/BF00352222.

Abstract

Antibodies against human Rad51 protein were used to examine the distribution of Rad51 on meiotic chromatin in mouse spermatocytes and oocytes as well as chicken oocytes during sequential stages of meiosis. We observed the following dynamic changes in distribution of Rad51 during meiosis: (1) in early leptotene nuclei there are multiple, apparently randomly distributed, foci that by late leptonema become organized into tracks of foci. (2) These foci persist into zygonema, but most foci are now localized on Rad51-positive axes that correspond to lateral elements of the synaptonemal complex. As homologs synapse foci from homologous axes fuse. The distribution and involvement of Rad51 foci as contact points between homologs suggest that they may be components to early recombination nodules. (3) As pachynema progresses the number of foci drops dramatically; the temporal occurrence (mice) and physical and numerical distribution of foci on axes (chickens) suggest that they may be a component of late recombination nodules. (4) In early pachynema there are numerous Rad51 foci on the single axis of the X (mouse spermatocytes) or the Z (chicken oocytes) chromosomes that neither pair, nor recombine. (5) In late pachynema in mouse spermatocytes, but not oocytes, the Rad51 signal is preferentially enhanced at both ends of all the bivalents. As bivalents in spermatocytes, but not oocytes, begin to desynapse at diplonema they are often held together at these Rad51-positive termini. These observations parallel observations that recombination rates are exceptionally high near chromosome ends in male but not female eutherian mammals. (6) From diakinesis through metaphase I, Rad51 protein is detected as low-intensity fluorescent doublets that localize with CREST-specific antigens (kinetochores), suggesting that Rad51 participates, at least as a structural component of the materials involved, in sister kinetochore cohesiveness. Finally, the changes in Rad51 distribution during meiosis do not appear to be species specific, but intrinsic to the meiotic process.

摘要

利用抗人Rad51蛋白的抗体,研究了减数分裂过程中,小鼠精母细胞、卵母细胞以及鸡卵母细胞中Rad51在减数分裂染色质上的分布情况。我们观察到减数分裂过程中Rad51分布的如下动态变化:(1)在细线期早期细胞核中,有多个明显随机分布的焦点,到细线期末期这些焦点会组织成焦点轨迹。(2)这些焦点持续到偶线期,但此时大多数焦点定位在与联会复合体侧生元件相对应的Rad51阳性轴上。随着同源染色体配对,同源轴上的焦点融合。Rad51焦点作为同源染色体之间的接触点的分布和参与情况表明,它们可能是早期重组结节的组成部分。(3)随着粗线期的推进,焦点数量急剧下降;焦点在时间上的出现(小鼠)以及在轴上的物理和数量分布(鸡)表明,它们可能是晚期重组结节的组成部分。(4)在粗线期早期,X染色体(小鼠精母细胞)或Z染色体(鸡卵母细胞)的单轴上有许多Rad51焦点,这些染色体既不配对也不重组。(5)在小鼠精母细胞的粗线期末期,而非卵母细胞中,所有二价体两端的Rad51信号优先增强。由于精母细胞而非卵母细胞中的二价体在双线期开始解联会,它们常常在这些Rad51阳性末端处保持在一起。这些观察结果与以下观察结果一致:在雄性而非雌性真兽类哺乳动物中,染色体末端附近的重组率异常高。(6)从终变期到中期I,检测到Rad51蛋白为低强度荧光双联体,其与CREST特异性抗原(动粒)共定位,这表明Rad51至少作为所涉及物质的结构成分,参与了姐妹动粒的黏连。最后,减数分裂过程中Rad51分布的变化似乎并非物种特异性的,而是减数分裂过程所固有的。

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