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促卵泡激素处理的大鼠支持细胞中基因表达的寡核苷酸微阵列分析。

Oligonucleotide microarray analysis of gene expression in follicle-stimulating hormone-treated rat Sertoli cells.

作者信息

McLean Derek J, Friel Patrick J, Pouchnik Derek, Griswold Michael D

机构信息

School of Molecular Biosciences, Center for Reproductive Biology, Washington State University, Pullman, WA 99164, USA.

出版信息

Mol Endocrinol. 2002 Dec;16(12):2780-92. doi: 10.1210/me.2002-0059.

Abstract

Spermatogenesis requires the presence of functional somatic Sertoli cells in the seminiferous tubules of the testis. Sertoli cells provide support and factors necessary for the successful progression of germ cells into spermatozoa. Sertoli cells are regulated to a large degree by the glycoprotein hormone FSH, which is required for the testis to acquire full size and spermatogenic capacity. Signaling events initiated by the binding of FSH to its receptor lead to an alteration of Sertoli cell gene expression. To characterize the changes in gene expression in FSH-treated Sertoli cells, we used the mRNA from these cells to screen Affymetrix U34A rat GeneChip oligonucleotide microarrays. Sertoli cells from 20-d-old rats were cultured in the presence of 25 ng/ml ovine FSH. At 0, 2, 4, 8, and 24 h after the addition of FSH, total RNA was purified and used to prepare biotinylated target, which was hybridized to the U34A rat microarray containing approximately 9000 rat genes. Analysis identified 100-300 transcripts at each time point that were up-regulated or down-regulated by 2-fold or greater. Genes previously reported to be FSH or cAMP regulated in rat Sertoli cells were identified, in addition to numerous genes not reported to be expressed or FSH regulated in Sertoli cells. The expression patterns of five of these genes, encoding nerve growth factor inducible gene B, PRL-1, PC3 nerve growth factor-inducible antiproliferative putative secreted protein, diacylglycerol acyltransferase, and an expressed sequence tag, in FSH- and N,O'-dibutyryl cAMP-treated rat Sertoli cells were confirmed and characterized by Northern blot analysis. Thus, we have begun to define the transcriptome induced and repressed by FSH in rat Sertoli cells, and we have generated datasets of genes available for further analysis in regard to spermatogenesis and Sertoli cell signaling.

摘要

精子发生需要睾丸生精小管中功能性支持细胞的存在。支持细胞为生殖细胞成功发育成精子提供支持和必要因子。支持细胞在很大程度上受糖蛋白激素促卵泡激素(FSH)调节,FSH是睾丸发育至完整大小和获得生精能力所必需的。FSH与其受体结合引发的信号事件会导致支持细胞基因表达发生改变。为了表征FSH处理的支持细胞中基因表达的变化,我们使用这些细胞的mRNA筛选Affymetrix U34A大鼠基因芯片寡核苷酸微阵列。将20日龄大鼠的支持细胞在含有25 ng/ml绵羊FSH的条件下培养。添加FSH后0、2、4、8和24小时,纯化总RNA并用于制备生物素化靶标,将其与包含约9000个大鼠基因的U34A大鼠微阵列杂交。分析确定在每个时间点有100 - 300个转录本上调或下调2倍或更多。除了许多以前未报道在支持细胞中表达或受FSH调节的基因外,还鉴定出了先前报道在大鼠支持细胞中受FSH或cAMP调节的基因。通过Northern印迹分析证实并表征了其中五个基因在FSH和N,O'-二丁酰环磷腺苷(dbcAMP)处理的大鼠支持细胞中的表达模式,这五个基因分别编码神经生长因子诱导基因B、PRL-1、PC3神经生长因子诱导的抗增殖假定分泌蛋白、二酰基甘油酰基转移酶和一个表达序列标签。因此,我们已开始确定FSH在大鼠支持细胞中诱导和抑制的转录组,并生成了可用于精子发生和支持细胞信号传导进一步分析的基因数据集。

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