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使用非放射性核糖探针通过原位杂交检测大鼠过渡蛋白2 mRNA的阶段特异性表达以及其在第7步精子细胞类核体中的可能定位。

Stage-specific expression of rat transition protein 2 mRNA and possible localization to the chromatoid body of step 7 spermatids by in situ hybridization using a nonradioactive riboprobe.

作者信息

Saunders P T, Millar M R, Maguire S M, Sharpe R M

机构信息

MRC Reproductive Biology Unit, Edinburgh, United Kingdom.

出版信息

Mol Reprod Dev. 1992 Dec;33(4):385-91. doi: 10.1002/mrd.1080330404.

DOI:10.1002/mrd.1080330404
PMID:1472370
Abstract

The present study has used methoxyacetic acid (MAA)-induced depletion of specific germ cell types in the rat and in situ hybridization with nonradioactive riboprobes to determine the stages of the spermatogenic cycle at which there is expression of the mRNA for the basic chromosomal protein transition protein 2 (TP2). On Northern blots, an abundant mRNA was detectable in samples from control adult rats, but the amount of message was markedly reduced when RNA was extracted from the testes of rats treated 14 and 21 days previously with methoxyacetic acid. These testes were depleted specifically of step 7-12 spermatids, suggesting that these cells contain TP2 mRNA. When tissue sections were subjected to in situ hybridization, the TP2 mRNA was localized at the cellular and subcellular levels. Messenger RNA for TP2 was first detectable in spermatids at step 7. In these spermatids, at high magnification, in addition to some positive reaction in the cytoplasm, intense staining was located to a perinuclear structure consistent with localization of mRNA within the chromatoid body. The amount of TP2 mRNA in the cytoplasm increased as remodelling of the early spermatid nucleus progressed and was highest in step 10 and 11 spermatids at stages X and XI. Thereafter, the mRNA decreased until it was undetectable in step 14 spermatids at stage XIV. The localization of TP2 mRNA to the chromatoid body of step 7 spermatids would be consistent with this organelle being a storage site for long-lived mRNAs utilized later in spermiogenesis.

摘要

本研究利用甲氧基乙酸(MAA)诱导大鼠特定生殖细胞类型的耗竭,并使用非放射性核糖探针进行原位杂交,以确定生精周期中碱性染色体蛋白过渡蛋白2(TP2)mRNA表达的阶段。在Northern印迹上,在成年对照大鼠的样本中可检测到丰富的mRNA,但当从14天和21天前用甲氧基乙酸处理的大鼠睾丸中提取RNA时,mRNA的量明显减少。这些睾丸中特异性地缺失了7-12步的精子细胞,表明这些细胞含有TP2 mRNA。当对组织切片进行原位杂交时,TP2 mRNA在细胞和亚细胞水平上定位。TP2的mRNA在第7步的精子细胞中首次可检测到。在这些精子细胞中,在高倍显微镜下,除了细胞质中有一些阳性反应外,强烈的染色位于与类染色质体内mRNA定位一致的核周结构中。随着早期精子细胞核重塑的进展,细胞质中TP2 mRNA的量增加,在X期和XI期的第10步和第11步精子细胞中最高。此后,mRNA减少,直到在XIV期的第14步精子细胞中检测不到。TP2 mRNA定位于第7步精子细胞的类染色质体,这与该细胞器作为精子发生后期使用的长寿命mRNA的储存位点是一致的。

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