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一种从宫颈刮片中快速大量分离DNA以检测人乳头瘤病毒感染的简单方法。

A simple and rapid method of high quantity DNA isolation from cervical scrapes for detection of human papillomavirus infection.

作者信息

Gopalkrishna V, Francis A, Sharma J K, Das B C

机构信息

Division of Molecular Oncology, Institute of Cytology and Preventive Oncology (ICMR), New Delhi, India.

出版信息

J Virol Methods. 1992 Jan;36(1):63-72. doi: 10.1016/0166-0934(92)90157-9.

Abstract

Infection with human papillomavirus (HPV) is an important etiological factor in the development of cervical cancer, and detection of the viral genome is of prognostic importance, particularly for preneoplastic lesions. We developed a simple, easy and efficient non-organic method of DNA extraction from cervical scrapes for reliable detection of HPV DNA sequences. The method involves incubation of cell nuclei in higher concentration of proteinase K at 65 degrees C for 2.5 h. Following prolonged incubation at higher temperature, the enzyme is autoinactivated and the DNA isolated can be used directly for analysis without further purification. The recovery of DNA is more than 95% and it can be easily cleaved by restriction enzymes and is suitable for amplification by the polymerase chain reaction (PCR). The whole procedure is carried out in a single Eppendorf tube and a large number of specimens can be processed at a time without any error of handling. DNA extracted from a single smear sample is sufficient to conduct as many as four different molecular biology tests. This provides an opportunity for verification of sensitivity, specificity and reliability of each test for diagnosis of HPV infection without resorting to biopsy.

摘要

人乳头瘤病毒(HPV)感染是宫颈癌发生发展的重要病因,病毒基因组的检测具有预后重要性,尤其是对于癌前病变。我们开发了一种简单、便捷且高效的从宫颈刮片中提取DNA的非有机方法,用于可靠检测HPV DNA序列。该方法包括将细胞核在较高浓度的蛋白酶K中于65摄氏度孵育2.5小时。在较高温度下长时间孵育后,酶会自动失活,分离出的DNA无需进一步纯化即可直接用于分析。DNA回收率超过95%,可轻松被限制性内切酶切割,适用于聚合酶链反应(PCR)扩增。整个过程在单个艾本德管中进行,一次可处理大量标本且无任何操作误差。从单个涂片样本中提取的DNA足以进行多达四项不同的分子生物学检测。这为在不进行活检的情况下验证每项检测诊断HPV感染的敏感性、特异性和可靠性提供了机会。

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