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首页> 外文期刊>Veterinarni Medicina >Methods of mycobacterial DNA isolation from different biological material: a review
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Methods of mycobacterial DNA isolation from different biological material: a review

机译:从不同生物材料中分离出分枝杆菌DNA的方法:综述

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摘要

Mycobacteria cause serious infections in animals and human beings. Huge economic losses on farms are caused by selected species of this wide family. A high risk of transmission of infection from animal to human exists. The knowledge of exact pathogencharacteristics is an important factor which can improve quick and adequate healing. Cultivation and determination of phenotype is still the "gold standard", but has the disadvantage of taking a long time and also low detection limit. Biochemical characterisation of isolates is not exact, and it is expensive. A more popular method used is the amplification of specific loci by polymerase chain reaction (PCR). For this method, the isolation of sufficient amounts of purified DNA is necessary. In this paperthe most frequently used method for DNA isolation from live mycobacterial cells, body fluids, tissues, histological samples and forensic materials are outlined. This paper assists only as guide for these methods, so we describe them briefly.
机译:分枝杆菌在动物和人类中引起严重的感染。农场的巨大经济损失是由这个大家族的选定物种造成的。存在从动物向人类传播感染的高风险。确切的病原体特征知识是可以改善快速和充分愈合的重要因素。表型的培养和确定仍然是“金标准”,但是具有耗时长且检测限低的缺点。分离物的生化特性不精确,而且价格昂贵。使用的更流行的方法是通过聚合酶链反应(PCR)扩增特定基因座。对于此方法,必须分离足够量的纯化DNA。本文概述了从活的分枝杆菌细胞,体液,组织,组织学样本和法医材料中分离DNA的最常用方法。本文仅作为这些方法的指导,因此我们简要介绍它们。

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