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nextera- tagmented reductivelyamplified dna genotyping- by- sequencing (nextrad) libraries  (Nextera AS)

 
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    Nextera AS nextera- tagmented reductivelyamplified dna genotyping- by- sequencing (nextrad) libraries
    Nextera Tagmented Reductivelyamplified Dna Genotyping By Sequencing (Nextrad) Libraries, supplied by Nextera AS, 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/nextera- tagmented reductivelyamplified dna genotyping- by- sequencing (nextrad) libraries/product/Nextera AS
    Average 90 stars, based on 1 article reviews
    nextera- tagmented reductivelyamplified dna genotyping- by- sequencing (nextrad) libraries - by Bioz Stars, 2026-04
    90/100 stars

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    Nextera AS sequencing libraries by tagmentation
    ( a ) Experimental workflow starts with the isolation, sectioning and micro-dissection of the primary visual cortex from a transgenic mouse. The tissue samples are converted into a single-cell suspension, single cells are isolated by FACS, poly(A)-RNA from each cell is reverse transcribed (RT), <t>cDNA</t> <t>is</t> <t>amplified</t> and fragmented, and sequenced on a next-generation sequencing (NGS) platform. ( b ) Analysis workflow starts with the definition of high variance genes and iterative clustering based on two different methods, PCA (shown here) and WGCNA, and cluster membership validation using a random forest classifier. Cells that are classified consistently into one cluster are called ‘core’ cells (N = 1424), while cells that are mapped to more than one cluster are labeled ‘intermediate cells’ (N = 255). After the termination criteria are met, clusters from the two methods are intersected, and iteratively validated until all core clusters contain at least 4 cells. ( , ). ( c ) The final 49 clusters were assigned an identity based on cell location and marker genes . Each type is represented by a color bar with the name and number of core cells representing that type. The violin plots represent distribution of mRNA expression on a linear scale, adjusted for each gene (max. RPKM on the right), for major known marker genes: Snap25 (pan-neuronal); Gad1 (pan-GABAergic); Vip, Sst and Pvalb (GABAergic); Slc17a7 (pan-glutamatergic); Rorb (mostly L4 and L5a); Foxp2 (L6); Aqp4 (astrocytes); Pdgfra (oligodendrocyte precursor cells, OPCs); Mog (oligodendrocytes); Itgam (microglia); Flt1 (endothelial cells) and Bgn (smooth muscle cells, SMC).
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    ( a ) Experimental workflow starts with the isolation, sectioning and micro-dissection of the primary visual cortex from a transgenic mouse. The tissue samples are converted into a single-cell suspension, single cells are isolated by FACS, poly(A)-RNA from each cell is reverse transcribed (RT), cDNA is amplified and fragmented, and sequenced on a next-generation sequencing (NGS) platform. ( b ) Analysis workflow starts with the definition of high variance genes and iterative clustering based on two different methods, PCA (shown here) and WGCNA, and cluster membership validation using a random forest classifier. Cells that are classified consistently into one cluster are called ‘core’ cells (N = 1424), while cells that are mapped to more than one cluster are labeled ‘intermediate cells’ (N = 255). After the termination criteria are met, clusters from the two methods are intersected, and iteratively validated until all core clusters contain at least 4 cells. ( , ). ( c ) The final 49 clusters were assigned an identity based on cell location and marker genes . Each type is represented by a color bar with the name and number of core cells representing that type. The violin plots represent distribution of mRNA expression on a linear scale, adjusted for each gene (max. RPKM on the right), for major known marker genes: Snap25 (pan-neuronal); Gad1 (pan-GABAergic); Vip, Sst and Pvalb (GABAergic); Slc17a7 (pan-glutamatergic); Rorb (mostly L4 and L5a); Foxp2 (L6); Aqp4 (astrocytes); Pdgfra (oligodendrocyte precursor cells, OPCs); Mog (oligodendrocytes); Itgam (microglia); Flt1 (endothelial cells) and Bgn (smooth muscle cells, SMC).

    Journal: Nature neuroscience

    Article Title: Adult Mouse Cortical Cell Taxonomy by Single Cell Transcriptomics

    doi: 10.1038/nn.4216

    Figure Lengend Snippet: ( a ) Experimental workflow starts with the isolation, sectioning and micro-dissection of the primary visual cortex from a transgenic mouse. The tissue samples are converted into a single-cell suspension, single cells are isolated by FACS, poly(A)-RNA from each cell is reverse transcribed (RT), cDNA is amplified and fragmented, and sequenced on a next-generation sequencing (NGS) platform. ( b ) Analysis workflow starts with the definition of high variance genes and iterative clustering based on two different methods, PCA (shown here) and WGCNA, and cluster membership validation using a random forest classifier. Cells that are classified consistently into one cluster are called ‘core’ cells (N = 1424), while cells that are mapped to more than one cluster are labeled ‘intermediate cells’ (N = 255). After the termination criteria are met, clusters from the two methods are intersected, and iteratively validated until all core clusters contain at least 4 cells. ( , ). ( c ) The final 49 clusters were assigned an identity based on cell location and marker genes . Each type is represented by a color bar with the name and number of core cells representing that type. The violin plots represent distribution of mRNA expression on a linear scale, adjusted for each gene (max. RPKM on the right), for major known marker genes: Snap25 (pan-neuronal); Gad1 (pan-GABAergic); Vip, Sst and Pvalb (GABAergic); Slc17a7 (pan-glutamatergic); Rorb (mostly L4 and L5a); Foxp2 (L6); Aqp4 (astrocytes); Pdgfra (oligodendrocyte precursor cells, OPCs); Mog (oligodendrocytes); Itgam (microglia); Flt1 (endothelial cells) and Bgn (smooth muscle cells, SMC).

    Article Snippet: We developed a robust procedure for isolating individual adult live cells from the suspension by fluorescence activated cell sorting (FACS), reverse transcribed and amplified full-length poly(A)-RNA with the SMARTer protocol, converted the cDNA into sequencing libraries by tagmentation (Nextera XT), and sequenced them by next generation sequencing ( , , ).

    Techniques: Isolation, Dissection, Transgenic Assay, Suspension, Reverse Transcription, Amplification, Next-Generation Sequencing, Biomarker Discovery, Labeling, Marker, Expressing