小鼠精母细胞突触复合体中减数分裂内聚蛋白亚基RAD21L和REC8分别位于外侧元件和横向细丝之间的不同区域

M. Rong, A. Matsuda, Y. Hiraoka, Jibak Lee
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引用次数: 23

摘要

含有减数分裂特异性α-柔素亚基RAD21L或REC8的内聚蛋白在减数分裂染色体动力学的各个方面发挥作用,包括轴向元件(ae)的形成、突触复合体(SC)的组装、同源染色体(homologs)的重组和姐妹染色单体的内聚。然而,单个α-克莱辛蛋白的确切功能仍有待阐明。在这里,我们通过超分辨率显微镜3D-SIM检测了RAD21L和REC8在SC中的定位。我们发现RAD21L和REC8都定位于厚肺膜的横向纤维(LEs)和横向纤维(tf)之间的连接位点,RAD21L位于REC8位点的内部。RAD21L和REC8在突触同源物上不对称,说明不同黏结蛋白的排列并不是沿所有染色体轴严格固定的。有趣的是,一些RAD21L信号,而不是REC8信号,在颧膜ae的未突触区域之间被观察到,好像它们形成了同源物之间的桥梁。重组中间体与RAD21L的信号重叠程度大于与REC8的信号重叠程度。这些结果突出了两种减数分裂α-粘连蛋白的不同性质,并有力地支持了先前的观点,即RAD21L是一种非典型粘连蛋白,它在同源物而不是姐妹染色单体之间建立了联系。
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Meiotic cohesin subunits RAD21L and REC8 are positioned at distinct regions between lateral elements and transverse filaments in the synaptonemal complex of mouse spermatocytes
Cohesins containing a meiosis-specific α-kleisin subunit, RAD21L or REC8, play roles in diverse aspects of meiotic chromosome dynamics including formation of axial elements (AEs), assembly of the synaptonemal complex (SC), recombination of homologous chromosomes (homologs), and cohesion of sister chromatids. However, the exact functions of individual α-kleisins remain to be elucidated. Here, we examined the localization of RAD21L and REC8 within the SC by super-resolution microscopy, 3D-SIM. We found that both RAD21L and REC8 were localized at the connection sites between lateral elements (LEs) and transverse filaments (TFs) of pachynema with RAD21L locating interior to REC8 sites. RAD21L and REC8 were not symmetrical in terms of synaptic homologs, suggesting that the arrangement of different cohesins is not strictly fixed along all chromosome axes. Intriguingly, some RAD21L signals, but not REC8 signals, were observed between unsynapsed regions of AEs of zygonema as if they formed a bridge between homologs. Furthermore, the signals of recombination intermediates overlapped with those of RAD21L to a greater degree than with those of REC8. These results highlight the different properties of two meiotic α-kleisins, and strongly support the previous proposition that RAD21L is an atypical cohesin that establishes the association between homologs rather than sister chromatids.
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