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首页> 外文期刊>FEMS Microbiology Ecology >Primer set 2.0 for highly parallel qPCR array targeting antibiotic resistance genes and mobile genetic elements
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Primer set 2.0 for highly parallel qPCR array targeting antibiotic resistance genes and mobile genetic elements

机译:用于高度平行的QPCR阵列的引物组2.0靶向抗生素抗性基因和移动遗传元件

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摘要

The high-throughput antibiotic resistance gene (ARG) qPCR array, initially published in 2012, is increasingly used to quantify resistance and mobile determinants in environmental matrices. Continued utility of the array; however, necessitates improvements such as removing or redesigning questionable primer sets, updating targeted genes and coverage of available sequences. Towards this goal, a new primer design tool (EcoFunPrimer) was used to aid in identification of conserved regions of diverse genes. The total number of assays used for diverse genes was reduced from 91 old primer sets to 52 new primer sets, with only a 10% loss in sequence coverage. While the old and new array both contain 384 primer sets, a reduction in old primer sets permitted 147 additional ARGs and mobile genetic elements to be targeted. Results of validating the updated array with a mock community of strains resulted in over 98% of tested instances incurring true positive/negative calls. Common queries related to sensitivity, quantification and conventional data analysis (e.g. Ct cutoff value, and estimated genomic copies without standard curves) were also explored. A combined list of new and previously used primer sets is provided with a recommended set based on redesign of primer sets and results of validation.
机译:最初在2012年最初公布的高通量抗生素抗性基因(ARG)QPCR阵列越来越多地用于量化环境基质中的抗性和移动决定因素。阵列的持续效用;然而,需要改进,例如去除或重新设计可疑的引物集,更新有针对性的基因和可用序列的覆盖范围。为了实现这一目标,用于帮助识别不同基因的保守区域的新底漆设计工具。用于各种基因的测定总数从91次旧底漆组降低至52个新底漆集,序列覆盖率的损耗仅为10%。虽然旧和新阵列都包含384个引物集,但允许旧底漆组的减少147个额外的args和移动遗传元素。验证更新的阵列的结果验证了菌株的模拟群落,导致超过98%的测试实例,这是真正的正/负呼叫。还探讨了与灵敏度,量化和传统数据分析相关的常见查询(例如,CT截止值和没有标准曲线的估计基因组拷贝)。新的和先前使用的底漆集的组合列表具有基于引物集的重新设计和验证结果的推荐集。

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