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96
Thermo Fisher alexa fluor 488 goat anti mouse antibody
Alexa Fluor 488 Goat Anti Mouse Antibody, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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New England Biolabs snap surface alexa fluor 488
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
Snap Surface Alexa Fluor 488, supplied by New England Biolabs, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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99
Thermo Fisher streptavidin alexa fluor 405 conjugate
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
Streptavidin Alexa Fluor 405 Conjugate, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Thermo Fisher alexa fluor 555 conjugated streptavidin
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
Alexa Fluor 555 Conjugated Streptavidin, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Thermo Fisher alexa fluor 647 labelled dna thermo fisher scientific
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
Alexa Fluor 647 Labelled Dna Thermo Fisher Scientific, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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96
New England Biolabs o6 benzylguanine bg coupled alexa fluor 647
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
O6 Benzylguanine Bg Coupled Alexa Fluor 647, supplied by New England Biolabs, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 96 stars, based on 1 article reviews
o6 benzylguanine bg coupled alexa fluor 647 - by Bioz Stars, 2026-02
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96
Thermo Fisher goat anti mouse alexa fluor 488
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
Goat Anti Mouse Alexa Fluor 488, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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goat anti mouse alexa fluor 488 - by Bioz Stars, 2026-02
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Thermo Fisher goat anti rabbit igg alexa fluor 647
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
Goat Anti Rabbit Igg Alexa Fluor 647, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Thermo Fisher alexa fluor 647 labeled dextran conjugate
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
Alexa Fluor 647 Labeled Dextran Conjugate, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 97/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Thermo Fisher alexa fluor 488 streptavidin conjugate s32354
Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa <t>Fluor</t> <t>488</t> and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.
Alexa Fluor 488 Streptavidin Conjugate S32354, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Image Search Results


Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa Fluor 488 and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.

Journal: iScience

Article Title: Synthetic zipper mediated pre-targeting system for near-infrared photoimmunotherapy

doi: 10.1016/j.isci.2025.114558

Figure Lengend Snippet: Specific interaction of scFv-Zip2 and Zip1-SNAP and their binding specificity in ovarian cancer cells (A) IR700 fluorescence was visualized using an Odyssey DLx Imager after incubation of scFv-Zip2 fusion proteins (scFv-Farletuzumab-Zip2, scFv-Sacituzumab-Zip2, and scFv-Tisotumab-SNAP-Zip2) with Zip1-SNAP-IR700. The scFv-Farletuzumab-SNAP was used as a control to assess the specificity of synthetic zipper interactions. (B) Flow cytometry analysis confirmed the antigen-specific binding of the pre-targeting complex in ovarian cancer cell lines. Histograms show the binding of scFv-Farletuzumab-Zip2 + Zip1-SNAP-IR700, scFv-Sacituzumab-Zip2 + Zip1-SNAP-IR700 and scFv-Tisotumab-Zip2 + Zip1-SNAP-IR700 to FOLR1 + , TROP2 + , and TF + ovarian cancer cells. (C) scFv-Zip2 and Zip1-SNAP were conjugated with 488 and IR700 respectively. We showed only IR700 channel to visualize only the Zip1-SNAP-IR700 florescence signal and finally merged to 488 and DAPI to visualize the internalization. Fluorescence microscopy images showing co-localization of scFv-Farletuzumab-Zip2 labeled with Alexa Fluor 488 and Zip1-SNAP-IR700 on ovarian cancer cells at 4°C, confirming the specific cell surface interaction of the pre-targeting complex. Scale bars, 25 μm.

Article Snippet: After incubation with SNAP-Surface® Alexa Fluor® 488 (New England Biolabs, Ipswich, MA, USA) for 20 min at room temperature in the dark, the fractions were subjected to 10% SDS-PAGE to verify SNAP-tag activity and protein presence, followed by Coomassie Brilliant Blue staining.

Techniques: Binding Assay, Fluorescence, Incubation, Control, Flow Cytometry, Microscopy, Labeling

Specific binding and co-localization of pre-targeting complex (A) Cells were incubated with Alexa Fluor 488-labeled (A) scFv-Sacituzumab-Zip2 and (B) scFv-Tisotumab-Zip2, followed by treatment with Zip1-SNAP-IR700. Fluorescence microscopy at 4°C revealed specific binding and co-localization of the scFv-Zip2 constructs with Zip1-SNAP-IR700, confirming zipper-mediated interaction and spatial overlap of the pre-targeting components. Scale bars, 25 μm.

Journal: iScience

Article Title: Synthetic zipper mediated pre-targeting system for near-infrared photoimmunotherapy

doi: 10.1016/j.isci.2025.114558

Figure Lengend Snippet: Specific binding and co-localization of pre-targeting complex (A) Cells were incubated with Alexa Fluor 488-labeled (A) scFv-Sacituzumab-Zip2 and (B) scFv-Tisotumab-Zip2, followed by treatment with Zip1-SNAP-IR700. Fluorescence microscopy at 4°C revealed specific binding and co-localization of the scFv-Zip2 constructs with Zip1-SNAP-IR700, confirming zipper-mediated interaction and spatial overlap of the pre-targeting components. Scale bars, 25 μm.

Article Snippet: After incubation with SNAP-Surface® Alexa Fluor® 488 (New England Biolabs, Ipswich, MA, USA) for 20 min at room temperature in the dark, the fractions were subjected to 10% SDS-PAGE to verify SNAP-tag activity and protein presence, followed by Coomassie Brilliant Blue staining.

Techniques: Binding Assay, Incubation, Labeling, Fluorescence, Microscopy, Construct