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哺乳动物精子发生过程中的基因表达。III. 精子形成过程中mRNA群体的变化。

Gene expression during mammalian spermatogenesis. III. Changes in populations of mRNA during spermiogenesis.

作者信息

Stern L, Kleene K C, Gold B, Hecht N B

出版信息

Exp Cell Res. 1983 Jan;143(1):247-55. doi: 10.1016/0014-4827(83)90125-8.

Abstract

Round spermatids and elongating spermatids were purified from a suspension of mouse testicular cells by sedimentation at unit gravity coupled with density gradient centrifugation through Percoll. Following separation, the two cell types were fractionated into polysomal and non-polysomal compartments. By comparison with round spermatids, elongating spermatids contain about one-half as much cytoplasmic RNA per cell, one sixth as much poly(A)+ RNA per cell and one-half the concentration of poly (A)+ mRNA in their cytoplasm. About two-thirds of the poly(A)+ messenger RNA (mRNA) was in the non-polysomal fraction in both cell types. Polypeptides whose synthesis was directed by cell-free translation of purified mRNA from each cell fraction were analyzed by two-dimensional gel electrophoresis. At the level of detection provided by the electrophoretic methods used, the majority of peptides from the polysomal and non-polysomal compartments for each cell type were similar. However, between the two cell types, approx. 5-10% of the polypeptides in the polysomal and non-polysomal fractions differed markedly in abundance. When the polypeptides encoded by the polysomal and non-polysomal mRNA from round spermatids were compared to the polypeptides encoded in the equivalent fractions from elongating spermatids, a significant reduction in number of polypeptides from elongating spermatids was seen. The presence of specific mRNAs in the non-polysomal fraction of round spermatids and in the polysomal fraction of elongating spermatids suggests that storage of mRNA in the cytoplasm and subsequent utilization provides a source of mRNA for proteins expressed at a time during spermiogenesis when transcription has terminated.

摘要

通过单位重力沉降结合经Percoll密度梯度离心,从小鼠睾丸细胞悬液中纯化出圆形精子细胞和伸长精子细胞。分离后,将这两种细胞类型分为多核糖体和非多核糖体部分。与圆形精子细胞相比,伸长精子细胞每个细胞所含的细胞质RNA约为其一半,每个细胞所含的多聚腺苷酸(poly(A)+)RNA约为其六分之一,其细胞质中多聚腺苷酸(poly(A)+)mRNA的浓度为其一半。两种细胞类型中约三分之二的多聚腺苷酸(poly(A)+)信使RNA(mRNA)存在于非多核糖体部分。通过二维凝胶电泳分析了由各细胞部分纯化的mRNA的无细胞翻译所指导合成的多肽。在所使用的电泳方法提供的检测水平上,每种细胞类型的多核糖体和非多核糖体部分的大多数肽是相似的。然而,在两种细胞类型之间,多核糖体和非多核糖体部分中约5-10%的多肽在丰度上有显著差异。当将圆形精子细胞的多核糖体和非多核糖体mRNA编码的多肽与伸长精子细胞的等效部分编码的多肽进行比较时,发现伸长精子细胞的多肽数量显著减少。圆形精子细胞的非多核糖体部分和伸长精子细胞的多核糖体部分中存在特定的mRNA,这表明mRNA在细胞质中的储存及随后的利用为精子发生过程中转录终止时表达的蛋白质提供了mRNA来源。

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