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牛精子高效RNA提取方法的建立与优化

Development and optimization of an efficient RNA isolation protocol from bovine () spermatozoa.

作者信息

Umar Sofi Imran Ul, Prasad Sushil, Naskar Soumen, Chowdhury Pooja, Rana Anju, Das Pranab Jyoti

机构信息

ICAR-Indian Institute of Agricultural Biotechnology, Garhkhatanga, Ranchi, 834003, India.

Birsa Agricultural University, Kanke, Ranchi, 834006, India.

出版信息

Biochem Biophys Rep. 2024 Nov 2;40:101862. doi: 10.1016/j.bbrep.2024.101862. eCollection 2024 Dec.

Abstract

Achieving the optimum extraction of RNA from spermatozoal cells is crucial for carrying out effective high-throughput analysis regarding its role in fertility and other reproduction processes in . Nevertheless, semen comprises spermatozoa and several other secretions from the male reproductive system, which as well consist of diverse somatic cell types. Therefore, the elimination of somatic cells guarantees the purity of the sperm RNA. In the present study, we tested five different RNA isolation protocols and evaluated them for their yield and purity using spectrophotometer and polymerase chain reaction. Among the five RNA isolation protocols, the Triazol + RNAeasy plus Kit + TCEP method revealed optimum performance. We successfully achieved isolation of spermatozoal RNA without any spermatozoal DNA contamination from spermatozoa that contains approx. 1000 to 10,000 times less RNA as compared to other mammalian somatic cells. RNA quality was assessed using primers (spermatozoal RNA and spermatozoal DNA), (epithelial cell), (germ cell) and (leukocytes) designed using primer BLAST where there was no product amplified except whose product size was specific for spermatozoal RNA. The results of our investigation on RNA isolation procedures indicate that the inclusion of a disulphide reducing agent (TCEP) is crucial for the process of sperm cell lysis.

摘要

从精子细胞中实现RNA的最佳提取对于开展关于其在生育及其他生殖过程中作用的有效高通量分析至关重要。然而,精液包含精子以及男性生殖系统的其他几种分泌物,其中也包括多种体细胞类型。因此,去除体细胞可确保精子RNA的纯度。在本研究中,我们测试了五种不同的RNA分离方案,并使用分光光度计和聚合酶链反应评估了它们的产量和纯度。在这五种RNA分离方案中,Triazol + RNAeasy plus试剂盒+ TCEP方法表现出最佳性能。我们成功地从精子中分离出了精子RNA,且没有任何精子DNA污染,这些精子含有的RNA比其他哺乳动物体细胞少约1000至10000倍。使用通过引物BLAST设计的引物(精子RNA和精子DNA)、(上皮细胞)、(生殖细胞)和(白细胞)评估RNA质量,除了其产物大小对精子RNA具有特异性的引物外,没有扩增出任何产物。我们对RNA分离程序的研究结果表明,加入二硫键还原剂(TCEP)对于精子细胞裂解过程至关重要。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fd47/11566313/909699f5af2a/gr1.jpg

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