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Quality Control of Biotechnological Inputs DetectingMycoplasma

机译:检测支原体的生物技术投入的质量控制

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The aim of this work was to study the Polymerase Chain Reaction (PCR) as a tool of quality control of bovine sera and cellular cultures used in the biotechnological industry. A total of 46 samples of bovine sera derived from two slaughterhouses and 33 samples of BHK21 cells derived from two biotechnological industries were evaluated using the primers GPO-3 (sense) and MGSO (antisense). The PCR technique sensibility analysis showed that 280 bp were amplified for the quantities of 50 ng to 0.006 ng of Micoplasma DNA. The primers specificity was confirmed in the test using Staphylococcus aureus, Escherichia coli, Bacillus subtilisand Candida albicans; except by the positive control, none of the samples showed amplification. The presence of Mycoplasma in bovine sera and in the cultures of BHK21 cells showed that 56.5 and 15.2%, respectively, were contaminated. Thus, it was possible to conclude that PCR was a fast and confident technique to detect mycoplasma and that it could be used to control the quality of immunobiological products and inputs, such as sera and cultures of BHK21 cells.
机译:这项工作的目的是研究聚合酶链反应(PCR),作为生物技术工业中使用的牛血清和细胞培养物质量控制的工具。使用引物GPO-3(有义)和MGSO(反义)对来自两个屠宰场的46份牛血清和来自两个生物技术行业的BHK21细胞的33份样本进行了评估。 PCR技术的敏感性分析表明,扩增了280 bp的量为50 ng至0.006 ng的Micoplasma DNA。使用金黄色葡萄球菌,大肠杆菌,枯草芽孢杆菌和白色念珠菌验证了引物的特异性。除了阳性对照外,没有样品显示扩增。牛血清和BHK21细胞培养物中支原体的存在表明分别污染了56.5%和15.2%。因此,有可能得出结论,PCR是检测支原体的一种快速而可靠的技术,它可用于控制免疫生物学产品和输入的质量,例如血清和BHK21细胞的培养。

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