期刊
ELECTROPHORESIS
卷 29, 期 7, 页码 1467-1472出版社
WILEY
DOI: 10.1002/elps.200700699
关键词
DNA quantification; humic acid; humic acid intercalation; PCR inhibition mechanisms; quantitative real-time PCR
Human DNA quantification by quantitative real-time PCR (QRT-PCR) has gained great importance in forensic DNA and ancient DNA studies. However, in such samples, DNA quantification is impaired by the frequently present humic acid (HA). We have previously shown that the addition of synthetic HA inhibits QRT-PCR. In this study we investigated the possible mechanisms of HA interaction with human DNA, and kinetics of QRT-PCR inhibition. In QRT-PCR with pure human DNA and no HA added, V-MAX was 40. With DNA sample containing 4 mu g/mL of HA, V-MAX was 30.30 while the addition of extra Taq polymerase to the same sample changed V-MAX into 38.91, amplifying between 80 and 90% of input DNA. The K-M/V-MAX ratio in all the samples remained constant, indicating that the mechanism of HA inhibition of QRT-PCR is uncompetitive by nature. Moreover, HA shifts the human DNA melting temperature point (T-m) from 75 to 87 degrees C and inhibits DNase I-mediated DNA cleavage, most probably affecting the enzyme's activity.
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