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Ichthyoplankton metabarcoding: an efficient tool for early detection of invasive species establishment

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DataONE2025-08-25 更新2025-08-30 收录
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Detection of invasive species is critical for management but is often limited by challenges associated with capture, processing, and identification of early life stages. DNA metabarcoding facilitates large-scale monitoring projects to detect establishment early. Here, we test the use of DNA metabarcoding to monitor invasive species by sequencing over 5000 fishes in bulk ichthyoplankton samples (larvae and eggs) from four rivers of ecological and cultural importance in southern Canada. We were successful in detecting species known from each river, and three invasive species in two of the four rivers. This includes the first detection of early life-stage rudd in the Credit River. We evaluated whether sampling gear affected detection of invasive species and estimates of species richness and found that light traps outperform bongo nets in both cases. We also found that the primers used for amplification of target sequences and the number of sequencing reads generated per sample, affect the ..., DNA extracted from homogenized bulk ichthyoplankton samples using salt extraction protocol, 1st PCR amplification using MiFish 12S or modified PS1 Teleost Primers with heterogeneity spacers and Nextera adaptor sequences, 2nd PCR using combinatorial Nextera i5/i7 indices, purified using Ampure XP magnetic beads and quantification via QuBit broad range kit, Illumina MiSeq using the V2 (150bp x 2).  Sequencing data were processed using the Qiime2 software package, utilizing the following algorithms (cudadapt / DADA2 / Vsearch). Processed sequencing data were analyzed using custom scripts in R and software packages VEGAN, MUSCLE, APE, and DECIPHER. Plots were generated using ggplot2. , Qiime2 R Mesquite, , # Ichthyoplankton metabarcoding: an efficient tool for early detection of invasive species establishment --- In this study, we used DNA metabarcoding of bulk samples of early life-stage fishes to analyze species composition and monitor invasive fishes in four major rivers in southern Ontario, Canada. Samples were collected using two different gear types, and we analyzed each sample by amplifying and sequencing two different barcode sequence markers in the COI and 12S mitochondrial genes, allowing comparison of how differences in methodology affect our results. DNA was extracted from homogenized bulk ichthyoplankton samples using salt extraction protocol. 1st PCR amplification using MiFish 12S or modified PS1 Teleost Primers with heterogeneity spacers and Nextera adaptor sequences. 2nd PCR using combinatorial Nextera i5/i7 indices, purified using Ampure XP magnetic beads and quantification via QuBit broad range kit. Sequenced using an Illumina MiSeq using the V2 (150bp x 2). We compa...
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2025-08-26
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