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               <h2><a href="https://www.litmetric.com/detail/32760558/Compared-with-conventional-PCR-assay-qPCR-assay-greatly-improves-the-detection-efficiency-of-predati" >Compared with conventional PCR assay, qPCR assay greatly improves the detection efficiency of predation.</a></h2>
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                <div class="publication-auther"><a href="https://www.litmetric.com/author/Ting-Bang+Yang" class="tag" style="margin-bottom: 5px;">Ting-Bang Yang</a> <a href="https://www.litmetric.com/author/Jie+Liu" class="tag" style="margin-bottom: 5px;">Jie Liu</a> <a href="https://www.litmetric.com/author/Jian+Chen" class="tag" style="margin-bottom: 5px;">Jian Chen</a></div>                   
                    <p class="mb-0 dark-color fz15 fw500 list-inline-item ml15 mb5-sm ml0-xs"><i class="flaticon-contract vam fz20 me-2"></i> Ecol Evol</p>
              
                   <p class="mb-0 dark-color fz15 fw500 list-inline-item mr15  mb5-sm ml0-xs"><i class="flaticon-place text-thm2 vam fz20 me-2"></i>  <a href='https://www.litmetric.com/search/The+State+Key+Laboratory+of+Biocatalysis+and+Enzyme+Engineering+of+China+School+of+Life+Sciences+Hubei+University+Wuhan+China.%5BAffiliation%5D' style='text-decoration: underline'>The State Key Laboratory of Biocatalysis and Enzyme Engineering of China School of Life Sciences Hubei University Wuhan China.</a></p>
                    
                     
                   <p class="mb-0 dark-color fz15 fw500 list-inline-item ml15 mb5-sm ml0-xs"><i class="flaticon-calendar vam fz20 me-2"></i> Published: July 2020</p>
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                   <p class="text mb30"><p class="text mt10">Studies of predation can contribute greatly to understanding predator-prey relationships and can also provide integral knowledge concerning food webs and multi-trophic level interactions. Both conventional polymerase chain reaction (cPCR) and quantitative PCR (qPCR) have been employed to detect predation in the field because of their sensitivity and reproducibility. However, to date, few studies have been used to comprehensively demonstrate which method is more sensitive and reproducible in studies of predation. We used a specific DNA fragment (99 bp) to construct a tenfold gradient dilution of standards. Additionally, we obtained DNA samples from  individuals that fed on  at various time since feeding. Finally, we compared the sensitivity and reproducibility between cPCR and qPCR assays for detecting DNA samples from feeding trials and standards. The results showed that the cPCR and qPCR assays could detect as few as 1.62 × 10 and 1.62 × 10 copies of the target DNA fragment, respectively. The cPCR assay could detect as few as 48 hr post-feeding of the target DNA fragment. But the qPCR assay showed that all spiders were positive after consuming prey at various time intervals (0, 24, 48, 72, and 96 hr). A smaller proportion of the technical replicates were positive using cPCR, and some bands on the agarose gel were absent or gray, while some were white and bright for the same DNA samples after amplification by cPCR. By contrast, a larger proportion of the technical replicates were positive using qPCR and the coefficients of variation of the  value for the three technical replicates of each DNA sample were less than 5%. These data showed that qPCR was more sensitive and highly reproducible in detecting such degraded DNA from predator's gut. The present study provides an example of the use of cPCR and qPCR to detect the target DNA fragment of prey remains in predator's gut.</p><table class="table table-bordered table-striped downloadTable" >
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