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通过分析线粒体细胞色素b靶点,对九种潜在粪便污染来源进行实时PCR检测和定量分析。

Real-time PCR detection and quantification of nine potential sources of fecal contamination by analysis of mitochondrial cytochrome b targets.

作者信息

Schill William B, Mathes Melvin V

机构信息

U.S. Geological Survey Leetown Science Center, 11649 Leetown Road, Kearneysville, West Virginia 25430, USA.

出版信息

Environ Sci Technol. 2008 Jul 15;42(14):5229-34. doi: 10.1021/es800051z.

Abstract

We designed and tested real-time PCR probe/primer sets to detect and quantify Cytochrome b sequences of mitochondrial DNA (mtDNA) from nine vertebrate species of pet (dog), farm (cow, chicken, sheep, horse, pig), wildlife (Canada goose, white-tailed deer), and human. Linear ranges of the assays were from 10(1) to 10(8) copies/microl. To formally test the performance of the assays, twenty blinded fecal suspension samples were analyzed by real-time PCR to identify the source of the feces. Sixteen of the twenty samples were correctly and unambiguously identified. Average sensitivity was calculated to be 0.850, while average specificity was found to be 0.994. One beef cow sample was not detected, but mtDNA from 11 other beef cattle of both sexes and varying physiological states was found in concentrations similar (3.45 x 10(7) copies/g) to thatfound in human feces (1.1 x 10(7) copies/g). Thus, environmental conditions and sample handling are probably important factors for successful detection of fecal mtDNA. When sewage samples were analyzed, only human mtDNA (7.2 x 10(4) copies/ 100 mL) was detected. With a detection threshold of 250 copies/reaction, an efficient concentration and purification method resulted in a final detection limit for human feces of 1.8 mg/ 100 mL water.

摘要

我们设计并测试了实时荧光定量PCR探针/引物组,用于检测和定量来自宠物(狗)、农场动物(牛、鸡、绵羊、马、猪)、野生动物(加拿大鹅、白尾鹿)和人类这9种脊椎动物的线粒体DNA(mtDNA)细胞色素b序列。这些检测方法的线性范围为10(1)至10(8)拷贝/微升。为了正式测试这些检测方法的性能,通过实时荧光定量PCR对20个盲法粪便悬液样本进行分析,以确定粪便来源。20个样本中有16个被正确且明确地鉴定出来。计算得出平均灵敏度为0.850,而平均特异性为0.994。有一个肉牛样本未被检测到,但在其他11头不同性别和生理状态的肉牛粪便中发现的mtDNA浓度(3.45×10(7)拷贝/克)与人类粪便中发现的浓度(1.1×10(7)拷贝/克)相似。因此,环境条件和样本处理可能是成功检测粪便mtDNA的重要因素。在分析污水样本时,仅检测到人类mtDNA(7.2×10(4)拷贝/100毫升)。以250拷贝/反应的检测阈值,一种有效的浓缩和纯化方法使得人类粪便的最终检测限达到1.8毫克/100毫升水。

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