The preparation of human spermatozoal RNA for clinical analysis.

Robert Goodrich, Graham Johnson, Stephen A Krawetz
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引用次数: 116

Abstract

The recent identification of RNA as a component of mature spermatozoa necessitated the development of a reliable isolation protocol capable of yielding a high-quality substrate. In addition to the inherent difficulties associated with isolating RNA, the procedure as applied to sperm must overcome the resilient nature and reduced RNA content found within this cell type. Further, the protocol must be suited to the clinical setting. A reliable RNA isolation procedure optimized for this unique cell type is described. Ejaculate is collected, contaminating somatic cells lysed then spermatozoal RNA released by homogenization in a chaotrope. RNA is then purified from the homogenate by chromatography using a commercially available resin. The quality of isolated samples is assessed by PCR and RT-PCR. Once purity is established samples are suitable for numerous applications including amplification and probe synthesis. The reliable and consistent isolation of high-quality RNA from mature spermatozoa will aid in the development of new tools for the clinical assessment of male-factor fertility.

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用于临床分析的人精子RNA的制备。
最近鉴定的RNA作为成熟精子的一个组成部分,需要开发一种可靠的分离方案,能够产生高质量的底物。除了与分离RNA相关的固有困难外,应用于精子的过程必须克服这种细胞类型的弹性和减少的RNA含量。此外,该方案必须适合临床环境。可靠的RNA分离程序优化这种独特的细胞类型描述。收集精液,污染裂解的体细胞,然后在混沌中匀浆释放精子RNA。然后用市售树脂从匀浆中通过层析纯化RNA。采用PCR和RT-PCR对分离样品的质量进行评价。一旦纯度确定,样品适用于多种应用,包括扩增和探针合成。从成熟精子中可靠和一致地分离高质量RNA将有助于开发用于临床评估男性因素生育能力的新工具。
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