首页> 外文OA文献 >Generation and synchronization of gonadotropin-releasing hormone (GnRH) pulses: intrinsic properties of the GT1-1 GnRH neuronal cell line.
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Generation and synchronization of gonadotropin-releasing hormone (GnRH) pulses: intrinsic properties of the GT1-1 GnRH neuronal cell line.

机译:促性腺激素释放激素(GnRH)脉冲的产生和同步:GT1-1 GnRH神经元细胞系的内在特性。

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摘要

The immortalized neuronal cell line GT1-1 was used to investigate the endogenous pattern of GnRH release. The GT1-1 cell line was derived from a GnRH-secreting tumor in a transgenic mouse induced by genetically targeted expression of the potent simian virus 40 oncogene encoding tumor antigen. Cells attached to coverslips were superfused in Sykes-Moore chambers with Locke's medium, Ca(2+)-free Locke's medium, or Opti-MEM (another defined medium) for 2 hr, and samples were collected at 4-min intervals. Release of GnRH in 17 of 18 superfusion chambers was seen to be pulsatile when data were analyzed by cluster analysis. No significant differences were observed whether only one or both of the coverslips forming the chamber were coated with cells. Pulses exhibited a mean interpulse interval of 25.8 +/- 1.5 min, a mean duration of 18.8 +/- 1.4 min, and a mean amplitude of 150.5 +/- 6.0% above preceding nadir. The removal of Ca2+ from the Locke's medium resulted in the progressive reduction of the amplitude and eventually in the absence of identifiable pulses. Pulses reappeared after the return of Ca2+ to the medium. It is concluded that the GT1-1 cell line secretes GnRH in a rhythmic pattern. These findings suggest that the pulsatile release of GnRH (GnRH pulse generator) may be an intrinsic characteristic of the GnRH neurons. Synchronization of pulsatile release from individual neurons could be mediated via numerous cell-to-cell contacts observed in the cultured cells on coverslips. Synchronization of GnRH release from cells on two physically separated coverslips forming a chamber would appear to be accomplished by a diffusible mediator.
机译:使用永生化的神经元细胞系GT1-1研究GnRH释放的内源性模式。 GT1-1细胞系衍生自转基因小鼠中分泌GnRH的肿瘤,该转基因小鼠通过有效靶向猿猴病毒40编码肿瘤抗原的癌基因的基因靶向表达而诱导。将附着在盖玻片上的细胞在Sykes-Moore室中与Locke培养基,无Ca(2+)的Locke培养基或Opti-MEM(另一种定义的培养基)融合2小时,并以4分钟的间隔收集样品。当通过聚类分析对数据进行分析时,可以看出在18个灌注室中的17个中,GnRH的释放是脉动的。无论是仅形成腔室的两个盖玻片中的一个还是两个都盖有细胞,均未观察到显着差异。脉冲表现出平均脉冲间隔为25.8 +/- 1.5分钟,平均持续时间为18.8 +/- 1.4分钟,平均振幅比先前最低点高150.5 +/- 6.0%。从Locke介质中去除Ca2 +会导致振幅逐渐减小,并最终导致没有可识别的脉冲。 Ca2 +返回介质后,脉冲再次出现。结论是,GT1-1细胞系以有节奏的方式分泌GnRH。这些发现表明,GnRH(GnRH脉冲发生器)的脉冲释放可能是GnRH神经元的固有特征。通过盖玻片上培养的细胞中观察到的大量细胞间接触,可以介导单个神经元的搏动释放同步。 GnRH从两个物理分离的盖玻片上形成腔室的细胞释放的同步似乎是由可扩散介体完成的。

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