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促性腺激素释放激素激动剂作用下,垂体促性腺细胞中G(q/11)α的重新分布。

Redistribution of G(q/11)alpha in the pituitary gonadotrope in response to a gonadotropin-releasing hormone agonist.

作者信息

Cornea A, Janovick J A, Stanislaus D, Conn P M

机构信息

Oregon Regional Primate Research Center, Beaverton 97006, USA.

出版信息

Endocrinology. 1998 Jan;139(1):397-402. doi: 10.1210/endo.139.1.5687.

Abstract

In the present study, we took advantage of high-resolution multilaser confocal microscopy to examine the distribution of the alpha-subunit of the guanyl nucleotide binding protein subfamily G(q/11) (G(q/11)alpha). Dispersed cultures of pituitary cells were prepared from female weanling rats, fixed, permeabilized, and then stained with monoclonal antiserum (mouse) to the gonadotrope-specific form of secretogranin (SIIp), which was then tagged with Texas Red. Accordingly, the subpopulation of gonadotropes (approximately 15% of total cells) could be identified against a background of other pituitary cell types. G(q/11)alpha was localized with antiserum made in rabbit, then tagged with fluorescein. Hoechst 33258 nuclear stain was also used in some experiments for topological reference. The data indicate localization of the G(q/11)alpha in a cellular region near the plasma membrane and external to the border of the layer occupied by secretory granules. In the absence of activation, there were an average of six clusters of G(q/11)alpha in a section 1 microm thick and through the center of the cell. This corresponds to an average of 60 clusters per cell, assuming a mean gonadotrope diameter of 10 microm. Following continuous treatment with 0.1 microg/ml Buserelin, a metabolically stable GnRH agonist, the average number of clusters increased to 200/cell after 40 min and remained approximately constant for 120 min. This increase was blocked by the protein synthesis inhibitor, cycloheximide. In response to Buserelin, there was an additional increase in the number of clusters inside the cell in the area occupied by the secretory granules and in the perinuclear area. Prolonged (24 h) treatment with Buserelin, sufficient to provoke the onset of desensitization, did not significantly change total numbers of G(q/11)alpha clusters, although more were located in the peripheral compartment, an increase that occurred at the expense of the cytoplasmic compartment. Redistribution of the G(q/11)alpha family may be functionally significant, because this moiety may be rate limiting at the site of regulation of signal transduction.

摘要

在本研究中,我们利用高分辨率多激光共聚焦显微镜来检测鸟苷酸结合蛋白亚家族G(q/11)(G(q/11)α)的α亚基的分布情况。从雌性断奶大鼠制备垂体细胞的分散培养物,进行固定、通透处理,然后用针对促性腺激素细胞特异性形式的分泌粒蛋白(SIIp)的单克隆抗血清(小鼠)染色,再用德克萨斯红标记。因此,在其他垂体细胞类型的背景下,可以识别出促性腺激素细胞亚群(约占总细胞的15%)。用兔抗血清定位G(q/11)α,然后用荧光素标记。在一些实验中还使用了Hoechst 33258核染色作为拓扑参考。数据表明G(q/11)α定位于靠近质膜且在分泌颗粒所占层边界之外的细胞区域。在未激活的情况下,在厚度为1微米且穿过细胞中心的切片中,平均有6个G(q/11)α簇。假设促性腺激素细胞的平均直径为10微米,这相当于每个细胞平均有60个簇。在用0.1微克/毫升布舍瑞林(一种代谢稳定的GnRH激动剂)持续处理后,40分钟后簇的平均数量增加到200/细胞,并在120分钟内大致保持恒定。这种增加被蛋白质合成抑制剂环己酰亚胺阻断。对布舍瑞林的反应中,在分泌颗粒所占区域和核周区域的细胞内簇的数量有额外增加。用布舍瑞林进行长时间(24小时)处理足以引发脱敏作用,尽管更多的簇位于外周区,以细胞质区为代价增加,但G(q/11)α簇的总数没有显著变化。G(q/11)α家族的重新分布可能具有功能意义,因为该部分可能在信号转导调节位点起限速作用。

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