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Data from: “Direct PCR” optimization yields a rapid, cost-effective, non-destructive, and efficient method for obtaining DNA barcodes without DNA extraction

负责人：

关键词：: ecosystem services;Chironomidae;DNA Barcoding;insects;Invertebrates

DOI：: doi:10.5061/dryad.4q4kf

摘要：: PCR method that skips DNA extraction (“direct PCR”) and that can be used for a broad range of invertebrate taxa. We demonstrate how direct PCR can be optimized

Data from: An examination of the accuracy of a sequential PCR and sequencing test used to detect the incursion of an invasive species: the cas

负责人：

关键词：: scats;predator faeces;specificity;sensitivity;sequential testing;trace DNA;Vulpes vulpes

DOI：: doi:10.5061/dryad.7652s

摘要：: 1. Polymerase Chain Reaction (PCR) diagnostic tests are increasingly applied to the identification of wildlife. Yet rigorous verification is rare

Data from: Microfluidic PCR-based target enrichment: a case study in two rapid radiations of Commiphora (Burseraceae) from Madagascar

负责人：

关键词：: Illumina MiSeq;microfluidic PCR;genome-tagged amplification;Miocene;Burseraceae;targeted amplicon sequencing;Commiphora;phylogenomics;Bursera

DOI：: doi:10.5061/dryad.591q3

摘要：: . Here we describe the development and validation of a novel set of 91 nuclear markers for PCR-based target enrichment. Using microfluidic PCR

Data from: Estimating and mitigating amplification bias in qualitative and quantitative arthropod metabarcoding

负责人：

关键词：: Arthropoda;Arthropods

DOI：: doi:10.5061/dryad.fs728

摘要：: can be derived from metabarcoding due to taxon specific PCR amplification biases. PCR-free approaches have been suggested to mitigate this problem

Data from: Optimizing methods for PCR-based analysis of predation

负责人：

关键词：: replicability;Pardosa;Oreonebria castanea;molecular gut content analysis;visualisation methods;annealing temperature;Nebria germari

DOI：: doi:10.5061/dryad.8947

摘要：: alpine carabid beetles and lycosid spiders, we investigated how PCR annealing temperature affects prey DNA detection success and how post-PCR visualization

Data from: Improving PCR detection of prey in molecular diet studies: importance of group-specific primer set selection and extraction protocol

负责人：: Zarzoso-Lacoste, Diane

关键词：: Invasive rats Diet Analysis PCR-based method Extraction protocol performances A260/A280 absorbance ratio Group-specific primer pairs

DOI：: doi:10.5061/dryad.8c134

摘要：: itical step, as PCR inhibitors may be co-extracted. Another critical step consist in carefully select suitable group-specific primer sets that should

Data from: PCR-based isolation of multigene families: lessons from the avian MHC class IIB

负责人：

关键词：: Musophagiformes;multi-gene families;Coraciiformes;Birds;Charadriiformes;Strigiformes;Major histocompatibility complex;Procellariformes;Ciconiformes;PCR-bias;Passeriformes;Columbiformes;Struthioniformes;Apodiformes;Piciformes;Accipitridae;Gruiformes

DOI：: doi:10.5061/dryad.1mn40

摘要：: r a range of species are readily obtained by aligning conserved gene regions, and laborious gene isolation procedures can often be replaced by quicker PCR

Data from: Residual eDNA detection sensitivity assessed by quantitative real-time PCR in a river ecosystem

负责人：

关键词：: Environmental DNA;qRT-PCR;river;Residual;DNA persistence

DOI：: doi:10.5061/dryad.5rf92

摘要：: eDNA detection sensitivity using quantitative real-time polymerase chain reaction (qRT-PCR), in a flowing, uncontrolled river after the eDNA source

Data from: Development of a PCR-RFLP assay to identify Drosophila melanogaster among field-collected larvae

负责人：: Raquin Vincent

关键词：: Fruit fly larvae field samples PCR-RFLP taxonomic identification

DOI：: doi:10.5061/dryad.pm71k02

摘要：: ecially field-derived samples. Here, we developed a Polymerase Chain Reaction-Restriction Fragment Length Polymorphism (PCR-RFLP) assay that discr

Data from: Blood-stage parasitaemia and age determine Plasmodium falciparum and P. vivax gametocytaemia in Papua New Guinea

负责人：

关键词：: asymptomatic infection;Plasmodium vivax;Plasmodium falciparum;age trend;malaria transmission;cross-sectional;gametocyte;submicroscopic infection

DOI：: doi:10.5061/dryad.550p3

摘要：: and gametocytes by detection of pfs25 and pvs25 mRNA transcripts by reverse-transcriptase PCR (qRT-PCR). The parasite prevalence by PCR was 18

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