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mouse anti-shh (5e1  (Thermo Fisher)


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    Structured Review

    Thermo Fisher mouse anti-shh (5e1
    (A) Purified <t>SCUBE2-SHH</t> or SHH-N was added to HEK293T cells expressing EGFP-tagged PTCH1, and bound ligand was quantified by anti-SHH <t>(5E1)</t> immunofluorescence. SCUBE2 reduces SHH affinity for PTCH1. Data are normalized between background signal (untreated cells) and maximum SHH-N binding (defined as 100%), and are fit with a three-parameter curve. Points represent average binding for four replicates, and error bars represent SEM. At least 200 cells were measured per replicate.
    Mouse Anti Shh (5e1, supplied by Thermo Fisher, 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/mouse anti-shh (5e1/product/Thermo Fisher
    Average 90 stars, based on 1 article reviews
    mouse anti-shh (5e1 - by Bioz Stars, 2026-02
    90/100 stars

    Images

    1) Product Images from "Hedgehog Pathway Activation Requires Coreceptor-Catalyzed, Lipid-Dependent Relay of the Sonic Hedgehog Ligand"

    Article Title: Hedgehog Pathway Activation Requires Coreceptor-Catalyzed, Lipid-Dependent Relay of the Sonic Hedgehog Ligand

    Journal: Developmental cell

    doi: 10.1016/j.devcel.2020.09.017

    (A) Purified SCUBE2-SHH or SHH-N was added to HEK293T cells expressing EGFP-tagged PTCH1, and bound ligand was quantified by anti-SHH (5E1) immunofluorescence. SCUBE2 reduces SHH affinity for PTCH1. Data are normalized between background signal (untreated cells) and maximum SHH-N binding (defined as 100%), and are fit with a three-parameter curve. Points represent average binding for four replicates, and error bars represent SEM. At least 200 cells were measured per replicate.
    Figure Legend Snippet: (A) Purified SCUBE2-SHH or SHH-N was added to HEK293T cells expressing EGFP-tagged PTCH1, and bound ligand was quantified by anti-SHH (5E1) immunofluorescence. SCUBE2 reduces SHH affinity for PTCH1. Data are normalized between background signal (untreated cells) and maximum SHH-N binding (defined as 100%), and are fit with a three-parameter curve. Points represent average binding for four replicates, and error bars represent SEM. At least 200 cells were measured per replicate.

    Techniques Used: Purification, Expressing, Immunofluorescence, Binding Assay

    (A) Fluorescently labeled SCUBE2 (300 nM) was incubated with cells expressing EGFP-tagged SHH-binding proteins, and bound ligand was quantified by fluorescence microscopy. SCUBE2 binds to CDON/BOC, but not to other SHH interactors. Data are normalized between binding to EGFP-tagged SMO (negative control) and the highest bound signal (100%). Box plots represent median and the first and third quartiles of binding. At least 400 cells were measured per condition.
    Figure Legend Snippet: (A) Fluorescently labeled SCUBE2 (300 nM) was incubated with cells expressing EGFP-tagged SHH-binding proteins, and bound ligand was quantified by fluorescence microscopy. SCUBE2 binds to CDON/BOC, but not to other SHH interactors. Data are normalized between binding to EGFP-tagged SMO (negative control) and the highest bound signal (100%). Box plots represent median and the first and third quartiles of binding. At least 400 cells were measured per condition.

    Techniques Used: Labeling, Incubation, Expressing, Binding Assay, Fluorescence, Microscopy, Negative Control

    (A) Fluorescently labeled SCUBE2 (600 nM), alone or in complex with SHH(HPC7) (300 nM), was incubated with cells expressing EGFP-tagged GAS1, scFv5E1::TM (positive control), or SMO (negative control), and bound SCUBE2 was measured by fluorescence microscopy. Even when complexed with SHH(HPC), SCUBE2 is not recruited to GAS1, in contrast to scFv5E1::TM. Data are normalized between binding of SCUBE2-SHH(HPC) to the negative and positive controls. At least 600 cells were measured per condition.
    Figure Legend Snippet: (A) Fluorescently labeled SCUBE2 (600 nM), alone or in complex with SHH(HPC7) (300 nM), was incubated with cells expressing EGFP-tagged GAS1, scFv5E1::TM (positive control), or SMO (negative control), and bound SCUBE2 was measured by fluorescence microscopy. Even when complexed with SHH(HPC), SCUBE2 is not recruited to GAS1, in contrast to scFv5E1::TM. Data are normalized between binding of SCUBE2-SHH(HPC) to the negative and positive controls. At least 600 cells were measured per condition.

    Techniques Used: Labeling, Incubation, Expressing, Positive Control, Negative Control, Fluorescence, Microscopy, Binding Assay

    KEY RESOURCES TABLE
    Figure Legend Snippet: KEY RESOURCES TABLE

    Techniques Used: Recombinant, SYBR Green Assay, Purification, Luciferase, CRISPR, Sequencing, Blocking Assay, Software, Microscopy



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    (A) Purified <t>SCUBE2-SHH</t> or SHH-N was added to HEK293T cells expressing EGFP-tagged PTCH1, and bound ligand was quantified by anti-SHH <t>(5E1)</t> immunofluorescence. SCUBE2 reduces SHH affinity for PTCH1. Data are normalized between background signal (untreated cells) and maximum SHH-N binding (defined as 100%), and are fit with a three-parameter curve. Points represent average binding for four replicates, and error bars represent SEM. At least 200 cells were measured per replicate.
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    Image Search Results


    (A) Purified SCUBE2-SHH or SHH-N was added to HEK293T cells expressing EGFP-tagged PTCH1, and bound ligand was quantified by anti-SHH (5E1) immunofluorescence. SCUBE2 reduces SHH affinity for PTCH1. Data are normalized between background signal (untreated cells) and maximum SHH-N binding (defined as 100%), and are fit with a three-parameter curve. Points represent average binding for four replicates, and error bars represent SEM. At least 200 cells were measured per replicate.

    Journal: Developmental cell

    Article Title: Hedgehog Pathway Activation Requires Coreceptor-Catalyzed, Lipid-Dependent Relay of the Sonic Hedgehog Ligand

    doi: 10.1016/j.devcel.2020.09.017

    Figure Lengend Snippet: (A) Purified SCUBE2-SHH or SHH-N was added to HEK293T cells expressing EGFP-tagged PTCH1, and bound ligand was quantified by anti-SHH (5E1) immunofluorescence. SCUBE2 reduces SHH affinity for PTCH1. Data are normalized between background signal (untreated cells) and maximum SHH-N binding (defined as 100%), and are fit with a three-parameter curve. Points represent average binding for four replicates, and error bars represent SEM. At least 200 cells were measured per replicate.

    Article Snippet: Purified mouse anti-SHH (5E1), anti-FLAG-M1 and anti-HPC monoclonal antibodies were fluorescently labeled using Alexa Fluor 568 NHS ester or Alexa Fluor 647 NHS ester (Thermo), according to the manufacturer’s instructions.

    Techniques: Purification, Expressing, Immunofluorescence, Binding Assay

    (A) Fluorescently labeled SCUBE2 (300 nM) was incubated with cells expressing EGFP-tagged SHH-binding proteins, and bound ligand was quantified by fluorescence microscopy. SCUBE2 binds to CDON/BOC, but not to other SHH interactors. Data are normalized between binding to EGFP-tagged SMO (negative control) and the highest bound signal (100%). Box plots represent median and the first and third quartiles of binding. At least 400 cells were measured per condition.

    Journal: Developmental cell

    Article Title: Hedgehog Pathway Activation Requires Coreceptor-Catalyzed, Lipid-Dependent Relay of the Sonic Hedgehog Ligand

    doi: 10.1016/j.devcel.2020.09.017

    Figure Lengend Snippet: (A) Fluorescently labeled SCUBE2 (300 nM) was incubated with cells expressing EGFP-tagged SHH-binding proteins, and bound ligand was quantified by fluorescence microscopy. SCUBE2 binds to CDON/BOC, but not to other SHH interactors. Data are normalized between binding to EGFP-tagged SMO (negative control) and the highest bound signal (100%). Box plots represent median and the first and third quartiles of binding. At least 400 cells were measured per condition.

    Article Snippet: Purified mouse anti-SHH (5E1), anti-FLAG-M1 and anti-HPC monoclonal antibodies were fluorescently labeled using Alexa Fluor 568 NHS ester or Alexa Fluor 647 NHS ester (Thermo), according to the manufacturer’s instructions.

    Techniques: Labeling, Incubation, Expressing, Binding Assay, Fluorescence, Microscopy, Negative Control

    (A) Fluorescently labeled SCUBE2 (600 nM), alone or in complex with SHH(HPC7) (300 nM), was incubated with cells expressing EGFP-tagged GAS1, scFv5E1::TM (positive control), or SMO (negative control), and bound SCUBE2 was measured by fluorescence microscopy. Even when complexed with SHH(HPC), SCUBE2 is not recruited to GAS1, in contrast to scFv5E1::TM. Data are normalized between binding of SCUBE2-SHH(HPC) to the negative and positive controls. At least 600 cells were measured per condition.

    Journal: Developmental cell

    Article Title: Hedgehog Pathway Activation Requires Coreceptor-Catalyzed, Lipid-Dependent Relay of the Sonic Hedgehog Ligand

    doi: 10.1016/j.devcel.2020.09.017

    Figure Lengend Snippet: (A) Fluorescently labeled SCUBE2 (600 nM), alone or in complex with SHH(HPC7) (300 nM), was incubated with cells expressing EGFP-tagged GAS1, scFv5E1::TM (positive control), or SMO (negative control), and bound SCUBE2 was measured by fluorescence microscopy. Even when complexed with SHH(HPC), SCUBE2 is not recruited to GAS1, in contrast to scFv5E1::TM. Data are normalized between binding of SCUBE2-SHH(HPC) to the negative and positive controls. At least 600 cells were measured per condition.

    Article Snippet: Purified mouse anti-SHH (5E1), anti-FLAG-M1 and anti-HPC monoclonal antibodies were fluorescently labeled using Alexa Fluor 568 NHS ester or Alexa Fluor 647 NHS ester (Thermo), according to the manufacturer’s instructions.

    Techniques: Labeling, Incubation, Expressing, Positive Control, Negative Control, Fluorescence, Microscopy, Binding Assay

    KEY RESOURCES TABLE

    Journal: Developmental cell

    Article Title: Hedgehog Pathway Activation Requires Coreceptor-Catalyzed, Lipid-Dependent Relay of the Sonic Hedgehog Ligand

    doi: 10.1016/j.devcel.2020.09.017

    Figure Lengend Snippet: KEY RESOURCES TABLE

    Article Snippet: Purified mouse anti-SHH (5E1), anti-FLAG-M1 and anti-HPC monoclonal antibodies were fluorescently labeled using Alexa Fluor 568 NHS ester or Alexa Fluor 647 NHS ester (Thermo), according to the manufacturer’s instructions.

    Techniques: Recombinant, SYBR Green Assay, Purification, Luciferase, CRISPR, Sequencing, Blocking Assay, Software, Microscopy