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人类睾丸中PRM1、PRM2和TNP2多基因座的协同表达。

Coordinate expression of the PRM1, PRM2, and TNP2 multigene locus in human testis.

作者信息

Wykes S M, Nelson J E, Visscher D W, Djakiew D, Krawetz S A

机构信息

Department of Obstetrics and Gynecology, Wayne State University School of Medicine 48201.

出版信息

DNA Cell Biol. 1995 Feb;14(2):155-61. doi: 10.1089/dna.1995.14.155.

DOI:10.1089/dna.1995.14.155
PMID:7865133
Abstract

Maintenance of the transcriptionally inert state of the mature human spermatozoon requires the expression of the various members of the human protamine gene cluster prior to the final stages of spermatogenesis. During this process, known as spermiogenesis, round spermatids morphologically differentiate into mature spermatozoa. The expression of the PRM1, PRM2, and TNP2 genes facilitates the compaction and condensation of the genetic material within the developing spermatid. To understand better the coordinate control governing this transformation, we have examined the localization and distribution of the human protamines PRM1 and PRM2 and transition protein TNP2 transcripts during human spermatogenesis. The stage-specific expression of these transcripts was determined by in situ hybridization analysis using [alpha-35S]-labeled cRNA probes. PRM1, PRM2, and TNP2 transcripts were abundant in association with round and elongating spermatids, located in the adluminal region of the seminiferous epithelium. They were not observed in association with spermatogonia, spermatocytes, Sertoli cells, or interstitial cells. These data indicate that the human PRM1, PRM2, and TNP2 transcripts are expressed postmeiotically in round and elongating spermatids. The quantitative evaluation of each transcript was determined as a function of the relative optical density per unit area. In all cases examined, the relative level of each transcript was consistent with the following pattern, PRM2 > PRM1 congruent to TNP2.

摘要

成熟人类精子转录惰性状态的维持需要在精子发生的最后阶段之前表达人类鱼精蛋白基因簇的各个成员。在这个被称为精子形成的过程中,圆形精子细胞在形态上分化为成熟精子。PRM1、PRM2和TNP2基因的表达促进了发育中的精子细胞内遗传物质的压缩和浓缩。为了更好地理解控制这种转变的协调机制,我们研究了人类鱼精蛋白PRM1和PRM2以及过渡蛋白TNP2转录本在人类精子发生过程中的定位和分布。这些转录本的阶段特异性表达通过使用[α-35S]标记的cRNA探针进行原位杂交分析来确定。PRM1、PRM2和TNP2转录本在位于生精上皮近腔区域的圆形和伸长精子细胞中大量存在。在精原细胞、精母细胞、支持细胞或间质细胞中未观察到它们的存在。这些数据表明,人类PRM1、PRM2和TNP2转录本在减数分裂后在圆形和伸长精子细胞中表达。每种转录本的定量评估是根据每单位面积的相对光密度来确定的。在所有检查的病例中,每种转录本的相对水平与以下模式一致:PRM2 > PRM1 ≈ TNP2。

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