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egfp mcherry mcitrine mtagbfp2  (Addgene inc)


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    Structured Review

    Addgene inc egfp mcherry mcitrine mtagbfp2
    Cytometry set up with an example of sample at inoculation. A: YL2 (600DLP-620/15)/BL1 (495DLP-530/30) dot plot is used to separate GFP positive and mCherry positive cells. B: VL2 (495DLP-512/25)/SSC dot plot derived from the GFPPos gate on A, is used to separate <t>mCitrine</t> (-) from eGFP signal (+). C: VL1 (417LP-440/50)/SSC dot plot derived from the GFPNeg gate on A, is used to separate non-fluorescent cells from BFP positive cells. D: Hierarchy of gating and percentage of each population. % Total indicates the % of the total population of events in the corresponding gate.
    Egfp Mcherry Mcitrine Mtagbfp2, supplied by Addgene inc, used in various techniques. Bioz Stars score: 93/100, based on 11 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/egfp mcherry mcitrine mtagbfp2/product/Addgene inc
    Average 93 stars, based on 11 article reviews
    egfp mcherry mcitrine mtagbfp2 - by Bioz Stars, 2026-03
    93/100 stars

    Images

    1) Product Images from "Design of a new model yeast consortium for ecological studies of enological fermentation"

    Article Title: Design of a new model yeast consortium for ecological studies of enological fermentation

    Journal: bioRxiv

    doi: 10.1101/2024.05.06.592697

    Cytometry set up with an example of sample at inoculation. A: YL2 (600DLP-620/15)/BL1 (495DLP-530/30) dot plot is used to separate GFP positive and mCherry positive cells. B: VL2 (495DLP-512/25)/SSC dot plot derived from the GFPPos gate on A, is used to separate mCitrine (-) from eGFP signal (+). C: VL1 (417LP-440/50)/SSC dot plot derived from the GFPNeg gate on A, is used to separate non-fluorescent cells from BFP positive cells. D: Hierarchy of gating and percentage of each population. % Total indicates the % of the total population of events in the corresponding gate.
    Figure Legend Snippet: Cytometry set up with an example of sample at inoculation. A: YL2 (600DLP-620/15)/BL1 (495DLP-530/30) dot plot is used to separate GFP positive and mCherry positive cells. B: VL2 (495DLP-512/25)/SSC dot plot derived from the GFPPos gate on A, is used to separate mCitrine (-) from eGFP signal (+). C: VL1 (417LP-440/50)/SSC dot plot derived from the GFPNeg gate on A, is used to separate non-fluorescent cells from BFP positive cells. D: Hierarchy of gating and percentage of each population. % Total indicates the % of the total population of events in the corresponding gate.

    Techniques Used: Cytometry, Derivative Assay



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    93
    Addgene inc egfp mcherry mcitrine mtagbfp2
    Cytometry set up with an example of sample at inoculation. A: YL2 (600DLP-620/15)/BL1 (495DLP-530/30) dot plot is used to separate GFP positive and mCherry positive cells. B: VL2 (495DLP-512/25)/SSC dot plot derived from the GFPPos gate on A, is used to separate <t>mCitrine</t> (-) from eGFP signal (+). C: VL1 (417LP-440/50)/SSC dot plot derived from the GFPNeg gate on A, is used to separate non-fluorescent cells from BFP positive cells. D: Hierarchy of gating and percentage of each population. % Total indicates the % of the total population of events in the corresponding gate.
    Egfp Mcherry Mcitrine Mtagbfp2, supplied by Addgene inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/egfp mcherry mcitrine mtagbfp2/product/Addgene inc
    Average 93 stars, based on 1 article reviews
    egfp mcherry mcitrine mtagbfp2 - by Bioz Stars, 2026-03
    93/100 stars
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    Cytometry set up with an example of sample at inoculation. A: YL2 (600DLP-620/15)/BL1 (495DLP-530/30) dot plot is used to separate GFP positive and mCherry positive cells. B: VL2 (495DLP-512/25)/SSC dot plot derived from the GFPPos gate on A, is used to separate mCitrine (-) from eGFP signal (+). C: VL1 (417LP-440/50)/SSC dot plot derived from the GFPNeg gate on A, is used to separate non-fluorescent cells from BFP positive cells. D: Hierarchy of gating and percentage of each population. % Total indicates the % of the total population of events in the corresponding gate.

    Journal: bioRxiv

    Article Title: Design of a new model yeast consortium for ecological studies of enological fermentation

    doi: 10.1101/2024.05.06.592697

    Figure Lengend Snippet: Cytometry set up with an example of sample at inoculation. A: YL2 (600DLP-620/15)/BL1 (495DLP-530/30) dot plot is used to separate GFP positive and mCherry positive cells. B: VL2 (495DLP-512/25)/SSC dot plot derived from the GFPPos gate on A, is used to separate mCitrine (-) from eGFP signal (+). C: VL1 (417LP-440/50)/SSC dot plot derived from the GFPNeg gate on A, is used to separate non-fluorescent cells from BFP positive cells. D: Hierarchy of gating and percentage of each population. % Total indicates the % of the total population of events in the corresponding gate.

    Article Snippet: The following plasmids were constructed by Gibson assembly (Gibson et al., 2009): pFA6a-link-yEmCitrine-NATMX, pFA6a-link-yomCherry-NATMX, pFA6-TDH3.1kb.Td-mCitrine-NATMX, pFA6-Hu1kb-BFP2-KAN. Gibson assembly were done using the NEB Builder HiFi DNA Assembly Master Mix (New England Biolabs) and transformed into E. coli DH5ɑ (New England Biolabs) following the manufacturer instructions. pFA6 plasmid backbone, antibiotic resistance cassettes ( KanMX, hphMX ) and fluorescent protein genes (EGFP, mCherry, mCitrine, mTagBFP2) were obtained from plasmids ordered from AddGene (#44900, #44899, #44645, #44903, Supplementary Table 1 , ; ).

    Techniques: Cytometry, Derivative Assay