sequencing library Search Results


sp 100 robots  (Complete Genomics Inc)
96
Complete Genomics Inc sp 100 robots
Sp 100 Robots, supplied by Complete Genomics Inc, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/sp 100 robots/product/Complete Genomics Inc
Average 96 stars, based on 1 article reviews
sp 100 robots - by Bioz Stars, 2026-06
96/100 stars
  Buy from Supplier
mgieasy whole genome bisulfite library preparation kit  (Complete Genomics Inc)
97
Complete Genomics Inc mgieasy whole genome bisulfite library preparation kit
Genome‐wide DNA methylation analysis in WT and GM seeds before and after GO treatments. a) Circos plots show the methylation levels across different chromosomes for WT and GM seeds before and after GO exposure. The colored sections on the outer ring represent different chromosomes. The concentric rings from outer to inner illustrate untreated samples, 0.75 mg‐C/L GO‐treated samples, and 1.5 mg‐C/L GO‐treated <t>samples.</t> <t>Whole‐genome</t> methylation levels were calculated as mean values within 100 kb windows for each chromosome. The color gradient from cyan to red indicates the methylation percentages, whereas the innermost ring represents gene density. b) Whole‐genome methylation levels in CG, CHG, and CHH contexts for WT and GM seeds after various GO exposures (sample size n = 3). Data are presented as means ± SD, with gray and red dots depicting individual data points in the WT and GM groups. Three biological replicates were included for each treatment. Independent sample two‐sided t ‐tests were performed: * indicates significant differences within the same genotype relative to the condition without GO, and # indicates significant differences between GM and WT under the same treatment. Significant differences are marked with p values. c) Differential methylation regions at promoter regions and gene bodies of key genes (Figure ) are represented by a color gradient showing Log 2 FC in methylation levels. Triangles and circles indicate CG and CHH methylation, respectively. No differential methylation was observed in the CHG context. Regions without differential methylation are blank. d) Dot plots of differential methylation for ALA metabolism‐related genes compare promoter and gene body methylation across conditions. Blue and red dots denote different comparisons, as indicated in the legend. Dots with circles indicate methylation levels with |Log 2 FC| >10.
Mgieasy Whole Genome Bisulfite Library Preparation Kit, supplied by Complete Genomics Inc, used in various techniques. Bioz Stars score: 97/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/mgieasy whole genome bisulfite library preparation kit/product/Complete Genomics Inc
Average 97 stars, based on 1 article reviews
mgieasy whole genome bisulfite library preparation kit - by Bioz Stars, 2026-06
97/100 stars
  Buy from Supplier
miseq sequencers  (fluidigm)
92
fluidigm miseq sequencers
Genome‐wide DNA methylation analysis in WT and GM seeds before and after GO treatments. a) Circos plots show the methylation levels across different chromosomes for WT and GM seeds before and after GO exposure. The colored sections on the outer ring represent different chromosomes. The concentric rings from outer to inner illustrate untreated samples, 0.75 mg‐C/L GO‐treated samples, and 1.5 mg‐C/L GO‐treated <t>samples.</t> <t>Whole‐genome</t> methylation levels were calculated as mean values within 100 kb windows for each chromosome. The color gradient from cyan to red indicates the methylation percentages, whereas the innermost ring represents gene density. b) Whole‐genome methylation levels in CG, CHG, and CHH contexts for WT and GM seeds after various GO exposures (sample size n = 3). Data are presented as means ± SD, with gray and red dots depicting individual data points in the WT and GM groups. Three biological replicates were included for each treatment. Independent sample two‐sided t ‐tests were performed: * indicates significant differences within the same genotype relative to the condition without GO, and # indicates significant differences between GM and WT under the same treatment. Significant differences are marked with p values. c) Differential methylation regions at promoter regions and gene bodies of key genes (Figure ) are represented by a color gradient showing Log 2 FC in methylation levels. Triangles and circles indicate CG and CHH methylation, respectively. No differential methylation was observed in the CHG context. Regions without differential methylation are blank. d) Dot plots of differential methylation for ALA metabolism‐related genes compare promoter and gene body methylation across conditions. Blue and red dots denote different comparisons, as indicated in the legend. Dots with circles indicate methylation levels with |Log 2 FC| >10.
Miseq Sequencers, supplied by fluidigm, used in various techniques. Bioz Stars score: 92/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/miseq sequencers/product/fluidigm
Average 92 stars, based on 1 article reviews
miseq sequencers - by Bioz Stars, 2026-06
92/100 stars
  Buy from Supplier
access array barcode library for illumina  (fluidigm)
95
fluidigm access array barcode library for illumina
Genome‐wide DNA methylation analysis in WT and GM seeds before and after GO treatments. a) Circos plots show the methylation levels across different chromosomes for WT and GM seeds before and after GO exposure. The colored sections on the outer ring represent different chromosomes. The concentric rings from outer to inner illustrate untreated samples, 0.75 mg‐C/L GO‐treated samples, and 1.5 mg‐C/L GO‐treated <t>samples.</t> <t>Whole‐genome</t> methylation levels were calculated as mean values within 100 kb windows for each chromosome. The color gradient from cyan to red indicates the methylation percentages, whereas the innermost ring represents gene density. b) Whole‐genome methylation levels in CG, CHG, and CHH contexts for WT and GM seeds after various GO exposures (sample size n = 3). Data are presented as means ± SD, with gray and red dots depicting individual data points in the WT and GM groups. Three biological replicates were included for each treatment. Independent sample two‐sided t ‐tests were performed: * indicates significant differences within the same genotype relative to the condition without GO, and # indicates significant differences between GM and WT under the same treatment. Significant differences are marked with p values. c) Differential methylation regions at promoter regions and gene bodies of key genes (Figure ) are represented by a color gradient showing Log 2 FC in methylation levels. Triangles and circles indicate CG and CHH methylation, respectively. No differential methylation was observed in the CHG context. Regions without differential methylation are blank. d) Dot plots of differential methylation for ALA metabolism‐related genes compare promoter and gene body methylation across conditions. Blue and red dots denote different comparisons, as indicated in the legend. Dots with circles indicate methylation levels with |Log 2 FC| >10.
Access Array Barcode Library For Illumina, supplied by fluidigm, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/access array barcode library for illumina/product/fluidigm
Average 95 stars, based on 1 article reviews
access array barcode library for illumina - by Bioz Stars, 2026-06
95/100 stars
  Buy from Supplier
fragments 10 kbp and a library was constructed using a ligation sequencing kit  (Oxford Nanopore)
97
Oxford Nanopore fragments 10 kbp and a library was constructed using a ligation sequencing kit
Genome‐wide DNA methylation analysis in WT and GM seeds before and after GO treatments. a) Circos plots show the methylation levels across different chromosomes for WT and GM seeds before and after GO exposure. The colored sections on the outer ring represent different chromosomes. The concentric rings from outer to inner illustrate untreated samples, 0.75 mg‐C/L GO‐treated samples, and 1.5 mg‐C/L GO‐treated <t>samples.</t> <t>Whole‐genome</t> methylation levels were calculated as mean values within 100 kb windows for each chromosome. The color gradient from cyan to red indicates the methylation percentages, whereas the innermost ring represents gene density. b) Whole‐genome methylation levels in CG, CHG, and CHH contexts for WT and GM seeds after various GO exposures (sample size n = 3). Data are presented as means ± SD, with gray and red dots depicting individual data points in the WT and GM groups. Three biological replicates were included for each treatment. Independent sample two‐sided t ‐tests were performed: * indicates significant differences within the same genotype relative to the condition without GO, and # indicates significant differences between GM and WT under the same treatment. Significant differences are marked with p values. c) Differential methylation regions at promoter regions and gene bodies of key genes (Figure ) are represented by a color gradient showing Log 2 FC in methylation levels. Triangles and circles indicate CG and CHH methylation, respectively. No differential methylation was observed in the CHG context. Regions without differential methylation are blank. d) Dot plots of differential methylation for ALA metabolism‐related genes compare promoter and gene body methylation across conditions. Blue and red dots denote different comparisons, as indicated in the legend. Dots with circles indicate methylation levels with |Log 2 FC| >10.
Fragments 10 Kbp And A Library Was Constructed Using A Ligation Sequencing Kit, supplied by Oxford Nanopore, used in various techniques. Bioz Stars score: 97/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/fragments 10 kbp and a library was constructed using a ligation sequencing kit/product/Oxford Nanopore
Average 97 stars, based on 1 article reviews
fragments 10 kbp and a library was constructed using a ligation sequencing kit - by Bioz Stars, 2026-06
97/100 stars
  Buy from Supplier
nanopore libraries  (Oxford Nanopore)
96
Oxford Nanopore nanopore libraries
Genome‐wide DNA methylation analysis in WT and GM seeds before and after GO treatments. a) Circos plots show the methylation levels across different chromosomes for WT and GM seeds before and after GO exposure. The colored sections on the outer ring represent different chromosomes. The concentric rings from outer to inner illustrate untreated samples, 0.75 mg‐C/L GO‐treated samples, and 1.5 mg‐C/L GO‐treated <t>samples.</t> <t>Whole‐genome</t> methylation levels were calculated as mean values within 100 kb windows for each chromosome. The color gradient from cyan to red indicates the methylation percentages, whereas the innermost ring represents gene density. b) Whole‐genome methylation levels in CG, CHG, and CHH contexts for WT and GM seeds after various GO exposures (sample size n = 3). Data are presented as means ± SD, with gray and red dots depicting individual data points in the WT and GM groups. Three biological replicates were included for each treatment. Independent sample two‐sided t ‐tests were performed: * indicates significant differences within the same genotype relative to the condition without GO, and # indicates significant differences between GM and WT under the same treatment. Significant differences are marked with p values. c) Differential methylation regions at promoter regions and gene bodies of key genes (Figure ) are represented by a color gradient showing Log 2 FC in methylation levels. Triangles and circles indicate CG and CHH methylation, respectively. No differential methylation was observed in the CHG context. Regions without differential methylation are blank. d) Dot plots of differential methylation for ALA metabolism‐related genes compare promoter and gene body methylation across conditions. Blue and red dots denote different comparisons, as indicated in the legend. Dots with circles indicate methylation levels with |Log 2 FC| >10.
Nanopore Libraries, supplied by Oxford Nanopore, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/nanopore libraries/product/Oxford Nanopore
Average 96 stars, based on 1 article reviews
nanopore libraries - by Bioz Stars, 2026-06
96/100 stars
  Buy from Supplier
cloud sequencing technology  (10X Genomics)
86
10X Genomics cloud sequencing technology
The five different enzyme concentrations/ng DNA using stLFR <t>sequencing</t> of D. wulumuqiensis R12 (A) The barcode frequency distribution of five conditions. (B) The Supernova-assembled statistics of five conditions.
Cloud Sequencing Technology, supplied by 10X Genomics, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/cloud sequencing technology/product/10X Genomics
Average 86 stars, based on 1 article reviews
cloud sequencing technology - by Bioz Stars, 2026-06
86/100 stars
  Buy from Supplier
library preparation rapid sequencing  (Oxford Nanopore)
96
Oxford Nanopore library preparation rapid sequencing
The five different enzyme concentrations/ng DNA using stLFR <t>sequencing</t> of D. wulumuqiensis R12 (A) The barcode frequency distribution of five conditions. (B) The Supernova-assembled statistics of five conditions.
Library Preparation Rapid Sequencing, supplied by Oxford Nanopore, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/library preparation rapid sequencing/product/Oxford Nanopore
Average 96 stars, based on 1 article reviews
library preparation rapid sequencing - by Bioz Stars, 2026-06
96/100 stars
  Buy from Supplier
library preparation and metagenomic sequencing  (LGC Genomics GmbH)
90
LGC Genomics GmbH library preparation and metagenomic sequencing
The five different enzyme concentrations/ng DNA using stLFR <t>sequencing</t> of D. wulumuqiensis R12 (A) The barcode frequency distribution of five conditions. (B) The Supernova-assembled statistics of five conditions.
Library Preparation And Metagenomic Sequencing, supplied by LGC Genomics GmbH, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/library preparation and metagenomic sequencing/product/LGC Genomics GmbH
Average 90 stars, based on 1 article reviews
library preparation and metagenomic sequencing - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
library preparation and sequencing  (Admera Health LLC)
90
Admera Health LLC library preparation and sequencing
The five different enzyme concentrations/ng DNA using stLFR <t>sequencing</t> of D. wulumuqiensis R12 (A) The barcode frequency distribution of five conditions. (B) The Supernova-assembled statistics of five conditions.
Library Preparation And Sequencing, supplied by Admera Health LLC, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/library preparation and sequencing/product/Admera Health LLC
Average 90 stars, based on 1 article reviews
library preparation and sequencing - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
a sequence-perfect library of 40 ecnagk variants  (Neochromosome Inc)
90
Neochromosome Inc a sequence-perfect library of 40 ecnagk variants
The five different enzyme concentrations/ng DNA using stLFR <t>sequencing</t> of D. wulumuqiensis R12 (A) The barcode frequency distribution of five conditions. (B) The Supernova-assembled statistics of five conditions.
A Sequence Perfect Library Of 40 Ecnagk Variants, supplied by Neochromosome Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/a sequence-perfect library of 40 ecnagk variants/product/Neochromosome Inc
Average 90 stars, based on 1 article reviews
a sequence-perfect library of 40 ecnagk variants - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
rna purification, reverse transcription, library preparation, and sequencing  (Biopharm GmbH)
90
Biopharm GmbH rna purification, reverse transcription, library preparation, and sequencing
The five different enzyme concentrations/ng DNA using stLFR <t>sequencing</t> of D. wulumuqiensis R12 (A) The barcode frequency distribution of five conditions. (B) The Supernova-assembled statistics of five conditions.
Rna Purification, Reverse Transcription, Library Preparation, And Sequencing, supplied by Biopharm GmbH, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/rna purification, reverse transcription, library preparation, and sequencing/product/Biopharm GmbH
Average 90 stars, based on 1 article reviews
rna purification, reverse transcription, library preparation, and sequencing - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier

Image Search Results


Genome‐wide DNA methylation analysis in WT and GM seeds before and after GO treatments. a) Circos plots show the methylation levels across different chromosomes for WT and GM seeds before and after GO exposure. The colored sections on the outer ring represent different chromosomes. The concentric rings from outer to inner illustrate untreated samples, 0.75 mg‐C/L GO‐treated samples, and 1.5 mg‐C/L GO‐treated samples. Whole‐genome methylation levels were calculated as mean values within 100 kb windows for each chromosome. The color gradient from cyan to red indicates the methylation percentages, whereas the innermost ring represents gene density. b) Whole‐genome methylation levels in CG, CHG, and CHH contexts for WT and GM seeds after various GO exposures (sample size n = 3). Data are presented as means ± SD, with gray and red dots depicting individual data points in the WT and GM groups. Three biological replicates were included for each treatment. Independent sample two‐sided t ‐tests were performed: * indicates significant differences within the same genotype relative to the condition without GO, and # indicates significant differences between GM and WT under the same treatment. Significant differences are marked with p values. c) Differential methylation regions at promoter regions and gene bodies of key genes (Figure ) are represented by a color gradient showing Log 2 FC in methylation levels. Triangles and circles indicate CG and CHH methylation, respectively. No differential methylation was observed in the CHG context. Regions without differential methylation are blank. d) Dot plots of differential methylation for ALA metabolism‐related genes compare promoter and gene body methylation across conditions. Blue and red dots denote different comparisons, as indicated in the legend. Dots with circles indicate methylation levels with |Log 2 FC| >10.

Journal: Advanced Science

Article Title: Accounting for ALA Natural Mutations Enhances the Efficiency of Graphene Oxide Nanopriming in Bar ‐Modified Arabidopsis

doi: 10.1002/advs.202500058

Figure Lengend Snippet: Genome‐wide DNA methylation analysis in WT and GM seeds before and after GO treatments. a) Circos plots show the methylation levels across different chromosomes for WT and GM seeds before and after GO exposure. The colored sections on the outer ring represent different chromosomes. The concentric rings from outer to inner illustrate untreated samples, 0.75 mg‐C/L GO‐treated samples, and 1.5 mg‐C/L GO‐treated samples. Whole‐genome methylation levels were calculated as mean values within 100 kb windows for each chromosome. The color gradient from cyan to red indicates the methylation percentages, whereas the innermost ring represents gene density. b) Whole‐genome methylation levels in CG, CHG, and CHH contexts for WT and GM seeds after various GO exposures (sample size n = 3). Data are presented as means ± SD, with gray and red dots depicting individual data points in the WT and GM groups. Three biological replicates were included for each treatment. Independent sample two‐sided t ‐tests were performed: * indicates significant differences within the same genotype relative to the condition without GO, and # indicates significant differences between GM and WT under the same treatment. Significant differences are marked with p values. c) Differential methylation regions at promoter regions and gene bodies of key genes (Figure ) are represented by a color gradient showing Log 2 FC in methylation levels. Triangles and circles indicate CG and CHH methylation, respectively. No differential methylation was observed in the CHG context. Regions without differential methylation are blank. d) Dot plots of differential methylation for ALA metabolism‐related genes compare promoter and gene body methylation across conditions. Blue and red dots denote different comparisons, as indicated in the legend. Dots with circles indicate methylation levels with |Log 2 FC| >10.

Article Snippet: Library construction was performed using an MGIEasy whole‐genome bisulfite library preparation kit (MGI).

Techniques: Genome Wide, DNA Methylation Assay, Methylation

The five different enzyme concentrations/ng DNA using stLFR sequencing of D. wulumuqiensis R12 (A) The barcode frequency distribution of five conditions. (B) The Supernova-assembled statistics of five conditions.

Journal: iScience

Article Title: Comparison of different sequencing strategies for assembling chromosome-level genomes of extremophiles with variable GC content

doi: 10.1016/j.isci.2021.102219

Figure Lengend Snippet: The five different enzyme concentrations/ng DNA using stLFR sequencing of D. wulumuqiensis R12 (A) The barcode frequency distribution of five conditions. (B) The Supernova-assembled statistics of five conditions.

Article Snippet: Different from previous studies, in which stLFR was applied for animal or plant genomics, our method allowed the pooling and parallel sequencing of a large number of samples, which cannot be achieved by 10X Genomics read cloud sequencing technology ( ).

Techniques: Sequencing

Statistics of three sequencing strategies assembly genomes

Journal: iScience

Article Title: Comparison of different sequencing strategies for assembling chromosome-level genomes of extremophiles with variable GC content

doi: 10.1016/j.isci.2021.102219

Figure Lengend Snippet: Statistics of three sequencing strategies assembly genomes

Article Snippet: Different from previous studies, in which stLFR was applied for animal or plant genomics, our method allowed the pooling and parallel sequencing of a large number of samples, which cannot be achieved by 10X Genomics read cloud sequencing technology ( ).

Techniques: Sequencing

The three sequencing strategies-assembled genome statistics of the six bacterial strains The total assembly genome length (bottom), N50 length (middle), and maximum scaffold length (top) by using different algorithms are shown. The assembly algorithms of each sample from left to right are NGS draft genome, stLFR chromosome scaffolds, stLFR + ONT complete genome, ONT complete genome assembled by Canu, and Hybrid complete genome assembled by Unicycler using ONT reads and NGS reads.

Journal: iScience

Article Title: Comparison of different sequencing strategies for assembling chromosome-level genomes of extremophiles with variable GC content

doi: 10.1016/j.isci.2021.102219

Figure Lengend Snippet: The three sequencing strategies-assembled genome statistics of the six bacterial strains The total assembly genome length (bottom), N50 length (middle), and maximum scaffold length (top) by using different algorithms are shown. The assembly algorithms of each sample from left to right are NGS draft genome, stLFR chromosome scaffolds, stLFR + ONT complete genome, ONT complete genome assembled by Canu, and Hybrid complete genome assembled by Unicycler using ONT reads and NGS reads.

Article Snippet: Different from previous studies, in which stLFR was applied for animal or plant genomics, our method allowed the pooling and parallel sequencing of a large number of samples, which cannot be achieved by 10X Genomics read cloud sequencing technology ( ).

Techniques: Sequencing

The longest chromosome sequence comparisons for strains (A–D) (A) E. coli K-12 using stLFR-assembled genome and the third-generation sequencing-assembled genome, (B) Rufibacter sp. LB8, (C) D. wulumuqiensis R12, and (D) J. melonis M714 using stLFR-assembled genomes, stLFR + ONT-assembled genomes, ONT + NGS Unicycler-assembled genomes, and ONT Canu-assembled genomes. The outermost circle is GC heatmap, the next circle is the histogram of GC (red: G > C; blue: G < (C), and the middle circle is gene density in chromosomes. The last two circles are the COG positive/negative annotation heatmaps, and the legend is shown at the bottom.

Journal: iScience

Article Title: Comparison of different sequencing strategies for assembling chromosome-level genomes of extremophiles with variable GC content

doi: 10.1016/j.isci.2021.102219

Figure Lengend Snippet: The longest chromosome sequence comparisons for strains (A–D) (A) E. coli K-12 using stLFR-assembled genome and the third-generation sequencing-assembled genome, (B) Rufibacter sp. LB8, (C) D. wulumuqiensis R12, and (D) J. melonis M714 using stLFR-assembled genomes, stLFR + ONT-assembled genomes, ONT + NGS Unicycler-assembled genomes, and ONT Canu-assembled genomes. The outermost circle is GC heatmap, the next circle is the histogram of GC (red: G > C; blue: G < (C), and the middle circle is gene density in chromosomes. The last two circles are the COG positive/negative annotation heatmaps, and the legend is shown at the bottom.

Article Snippet: Different from previous studies, in which stLFR was applied for animal or plant genomics, our method allowed the pooling and parallel sequencing of a large number of samples, which cannot be achieved by 10X Genomics read cloud sequencing technology ( ).

Techniques: Sequencing

The longest chromosome sequence comparison (A and B) (A) Sequences alignment viewer and (B) accuracy evaluation of stLFR genomes, stLFR + ONT genomes, Canu-assembled genomes, and NGS genomes when compared with the complete genomes assembled by Unicycler using NGS and ONT reads for the strains E. coli K-12, Rufibacter sp. LB8, D. wulumuqiensis R12, and J. melonis M714.

Journal: iScience

Article Title: Comparison of different sequencing strategies for assembling chromosome-level genomes of extremophiles with variable GC content

doi: 10.1016/j.isci.2021.102219

Figure Lengend Snippet: The longest chromosome sequence comparison (A and B) (A) Sequences alignment viewer and (B) accuracy evaluation of stLFR genomes, stLFR + ONT genomes, Canu-assembled genomes, and NGS genomes when compared with the complete genomes assembled by Unicycler using NGS and ONT reads for the strains E. coli K-12, Rufibacter sp. LB8, D. wulumuqiensis R12, and J. melonis M714.

Article Snippet: Different from previous studies, in which stLFR was applied for animal or plant genomics, our method allowed the pooling and parallel sequencing of a large number of samples, which cannot be achieved by 10X Genomics read cloud sequencing technology ( ).

Techniques: Sequencing, Comparison