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A comparison of Lyse-It to other cellular sample preparation, bacterial lysing, and DNA fragmentation technologies

机译:Lyse-It与其他细胞样品制备,细菌裂解和DNA片段化技术的比较

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摘要

The ability for safe and rapid pathogenic sample transportation and subsequent detection is an increasing challenge throughout the world. Herein, we describe and use bead-beating, vortex, sonication, 903 protein saver cards, and Lyse-It methods, aiming to inactivate Gram-positive and -negative bacteria with subsequent genome DNA (quantitative Polymerase Chain Reaction) qPCR detection. The basic concepts behind the four chosen technologies is their versatility, cost, and ease of use in developed and underdeveloped countries. The four methods target the testing of bacterial resilience, cellular extraction from general and complex media and subsequent DNA extraction for qPCR detection and amplification. These results demonstrate that conventional high temperature heating, 903 protein saver cards, and Lyse-It are all viable options for inactivating bacterial growth for safe shipping. Additionally, Lyse-It was found to be particularly useful as this technology can inactivate bacteria, extract cells from 903 protein saver cards, lyse bacterial cells, and additionally keep genomic DNA viable for qPCR detection.
机译:安全和快速的病原体样品运输以及随后的检测能力在世界范围内日益成为挑战。在本文中,我们描述并使用磁珠敲打,涡旋,超声处理,903蛋白保存卡和Lyse-It方法,旨在通过随后的基因组DNA(定量聚合酶链反应)qPCR检测灭活革兰氏阳性和阴性细菌。所选择的四种技术背后的基本概念是它们的多功能性,成本以及在发达国家和欠发达国家中的易用性。四种方法的目标是测试细菌的弹性,从普通和复杂培养基中提取细胞以及随后的DNA提取以进行qPCR检测和扩增。这些结果表明,常规的高温加热,903蛋白保存卡和Lyse-It都是灭活细菌生长以安全运输的可行选择。另外,发现Lyse-It特别有用,因为该技术可以灭活细菌,从903蛋白保存卡中提取细胞,裂解细菌细胞,并保持基因组DNA在qPCR检测中的可行性。

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