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小鼠精子发生过程中精子细胞核仁的乙醇-磷钨酸和铋染色

Ethanol-phosphotungstic acid and bismuth staining of spermatid nucleoli in mouse spermiogenesis.

作者信息

Takeuchi I K, Takeuchi Y K

机构信息

Department of Embryology, Institute for Developmental Research, Aichi Prefectural Colony, Japan.

出版信息

J Struct Biol. 1990 Apr;103(2):104-12. doi: 10.1016/1047-8477(90)90014-4.

Abstract

The nucleoli of developing mouse spermatids were examined with ethanol-phosphotungstic acid (E-PTA) staining, and also with bismuth staining following formaldehyde fixation (FA-Bi staining) and glutaraldehyde fixation (GA-Bi staining). Only the cortical zone of the nucleolar dense fibrillar component (DFC) in the round spermatids was stained with E-PTA, while the inner area remained either faintly (early Golgi-phase spermatids) or completely unstained (cap-phase spermatids). Incubation of the fixed testis with dithiothreitol before E-PTA staining resulted in homogeneously intense staining of the DFC. The facts suggest that numerous E-PTA-positive basic proteins were present in the DFC, but disulfide crosslinks formed in the DFC proteins prevent penetration of PTA into the DFC interior. The DFC was stained with bismuth after FA-Bi and GA-Bi staining until the disappearance of the nucleoli occurring in acrosome-phase spermatids. The fibrillar center, homogeneously stained using E-PTA, FA-Bi, and GA-Bi methods was present in the nucleoli of Golgi-phase and early cap-phase spermatids, but disappeared in the nucleoli of late cap-phase spermatids. These results are discussed based on the previous studies dealing with the ribosomal RNA synthesis in mouse spermiogenesis.

摘要

采用乙醇-磷钨酸(E-PTA)染色法,以及甲醛固定后的铋染色法(FA-Bi染色)和戊二醛固定后的铋染色法(GA-Bi染色),对发育中的小鼠精子细胞的核仁进行了检查。只有圆形精子细胞核仁致密纤维成分(DFC)的皮质区能被E-PTA染色,而内部区域要么染色很浅(早期高尔基体期精子细胞),要么完全不染色(帽期精子细胞)。在E-PTA染色前用二硫苏糖醇处理固定的睾丸,会导致DFC出现均匀强烈的染色。这些事实表明,DFC中存在大量E-PTA阳性碱性蛋白,但DFC蛋白中形成的二硫键交联阻止了磷钨酸进入DFC内部。在FA-Bi和GA-Bi染色后,DFC在顶体期精子细胞中核仁消失之前一直被铋染色。使用E-PTA、FA-Bi和GA-Bi方法均匀染色的纤维中心,存在于高尔基体期和早期帽期精子细胞的核仁中,但在晚期帽期精子细胞的核仁中消失。基于之前关于小鼠精子发生过程中核糖体RNA合成的研究,对这些结果进行了讨论。

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