Fluorescence-based Kits – VectorLabs https://staging.vectorlabs.com From linker design and synthesis, bioconjugated design and manufacturing, biomolecule labeling and functionalization, and detection system and solutions, our team is here to help you move forward, with impact. Wed, 22 Oct 2025 17:08:41 +0000 en-US hourly 1 https://wordpress.org/?v=6.8.3 https://staging.vectorlabs.com/wp-content/uploads/2024/11/V-favicon-02-100x100.png Fluorescence-based Kits – VectorLabs https://staging.vectorlabs.com 32 32 Click-&-Go® Plus 647 OPP https://staging.vectorlabs.com/products/click-go-plus-647-opp/ Tue, 19 Sep 2023 19:54:20 +0000 https://staging.vectorlabs.com/?post_type=product&p=22256 Description

Synthesis of many proteins is tightly controlled at the level of translation, and plays an essential role in fundamental processes such as cell growth and proliferation, signaling, differentiation, or death. Methods that allow imaging and identification of nascent proteins are critical for dissecting regulation of translation, both spatially and temporally, particularly in whole organisms. Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging.

The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with far-red-fluorescent AZDye 647 Azide Plus (Alexa Fluor® 647 equivalent), and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

[caption id="attachment_25905" align="alignnone" width="1000"] Abs/Em Spectra[/caption]

Specifications

Unit Size 1 kit
Label AZDye 647 Azide Plus
Abs/Em Maxima 648/671 nm
Number of Reactions 25
Storage Conditions 4C
Shipping Conditions Ambient temperature

The post Click-&-Go® Plus 647 OPP appeared first on VectorLabs.

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Click-&-Go® Plus 647 OPP Protein Synthesis Assay Kit is a non-radioactive method for measuring protein synthesis that employs the cell-permeable, alkyne-containing, puromycin analog O-Propargyl-puromycin (OPP). OPP (O-propargyl-puromycin) is an analog of puromycin that contains a terminal alkyne group, enters the acceptor site of ribosomes and incorporates into the C-terminus of translating polypeptide chains, thereby stopping translation. These truncated C-terminal alkyne-labeled proteins are then subsequently detected via copper-catalyzed click reaction using far-red fluorescent AZDye 647 Azide Plus. Unlike HPG or AHA labeling reagents OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. The kit contains all of the components needed to label and detect the incorporated OPP in newly translated proteins in samples of adherent cells. The kit includes sufficient reagents for the labeling of 25 18 mm × 18 mm coverslips using 1 mL of reaction buffer per test.

Description

Synthesis of many proteins is tightly controlled at the level of translation, and plays an essential role in fundamental processes such as cell growth and proliferation, signaling, differentiation, or death. Methods that allow imaging and identification of nascent proteins are critical for dissecting regulation of translation, both spatially and temporally, particularly in whole organisms. Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging.

The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with far-red-fluorescent AZDye 647 Azide Plus (Alexa Fluor® 647 equivalent), and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

Specifications

Unit Size1 kit
LabelAZDye 647 Azide Plus
Abs/Em Maxima648/671 nm
Number of Reactions25
Storage Conditions4C
Shipping ConditionsAmbient temperature

Abs/Em Spectra

AF647

Documents

The post Click-&-Go® Plus 647 OPP appeared first on VectorLabs.

]]> Click-&-Go® Plus 594 OPP https://staging.vectorlabs.com/products/click-go-plus-594-opp/ Tue, 19 Sep 2023 19:54:19 +0000 https://staging.vectorlabs.com/?post_type=product&p=22255 Description

Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging. Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging.

The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with red-fluorescent AZDye 594 Azide Plus, and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

[caption id="attachment_25875" align="alignnone" width="1000"] Abs/Em Spectra[/caption]

Specifications

Unit Size 1 kit
Label AZDye 594 Azide Plus
Abs/Em Maxima 590/615 nm
Number of Reactions 25
Storage Conditions 4C
Shipping Conditions Ambient temperature

The post Click-&-Go® Plus 594 OPP appeared first on VectorLabs.

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Click-&-Go® Plus 594 OPP Protein Synthesis Assay Kit enables fast and sensitive imaging of nascent proteins in complete, methionine-containing media. OPP (O-propargyl-puromycin) is an analog of puromycin that contains a terminal alkyne group, enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike HPG or AHA labeling reagents OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. In the next step, OPP-labeled nascent proteins are imaged through a chemoselective ligation, or “click” reaction, between the red fluorescent AZDye 594 Azide Plus (Alexa Fluor 594 ® equivalent) and the OPP-alkyne allowing the modified proteins to be detected by imaged-based analysis. The kit contains all of the components needed to label and detect the incorporated OPP in newly translated proteins in samples of adherent cells. The kit includes sufficient reagents for the labeling of 25 18 mm × 18 mm coverslips using 1 mL of reaction buffer per test.

Description

Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging.

The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with red-fluorescent AZDye 594 Azide Plus (Alexa Fluor® 594 equivalent), and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

Specifications

Unit Size1 kit
LabelAZDye 594 Azide Plus
Abs/Em Maxima590/615 nm
Number of Reactions25
Storage Conditions4C
Shipping ConditionsAmbient temperature

Abs/Em Spectra

AF594

Documents

The post Click-&-Go® Plus 594 OPP appeared first on VectorLabs.

]]> Click-&-Go® Plus 405 OPP https://staging.vectorlabs.com/products/click-go-plus-405-opp/ Tue, 19 Sep 2023 19:54:18 +0000 https://staging.vectorlabs.com/?post_type=product&p=22251 Description

Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging.

The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with blue-fluorescent AZDye 405 Azide Plus (Alexa Fluor® 405 equivalent), and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

Abs/Em Spectra

Specifications

Unit Size 1 kit
Label AZDye 405 Azide Plus
Abs/Em Maxima 402/421 nm
Number of Reactions 25
Storage Conditions 4C
Shipping Conditions Ambient temperature

The post Click-&-Go® Plus 405 OPP appeared first on VectorLabs.

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Click-&-Go® Plus 405 OPP Protein Synthesis Assay Kit enables fast, sensitive, and non-radioactive detection of protein synthesis using fluorescence microscopy or high-content imaging. O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. OPP that is incorporated into newly translated proteins is detected with fluorescent azides though a fast, highly-specific, and mild click reaction.

Description

Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging.

The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with blue-fluorescent AZDye 405 Azide Plus (Alexa Fluor® 405 equivalent), and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

Specifications

Unit Size1 kit
LabelAZDye 405 Azide Plus
Abs/Em Maxima402/421 nm
Number of Reactions25
Storage Conditions4C
Shipping ConditionsAmbient temperature

Abs/Em Spectra

AF405

Documents

The post Click-&-Go® Plus 405 OPP appeared first on VectorLabs.

]]> Click-&-Go® Plus 555 OPP https://staging.vectorlabs.com/products/click-go-plus-555-opp/ Tue, 19 Sep 2023 19:54:18 +0000 https://staging.vectorlabs.com/?post_type=product&p=22252 Description

Synthesis of many proteins is tightly controlled at the level of translation, and plays an essential role in fundamental processes such as cell growth and proliferation, signaling, differentiation, or death. Methods that allow imaging and identification of nascent proteins are critical for dissecting regulation of translation, both spatially and temporally, particularly in whole organisms. Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines.

The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with orange-fluorescent AZDye 555 Azide Plus, and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

[caption id="attachment_25595" align="alignnone" width="1000"] Abs/Em Spectra[/caption]

Specifications

Unit Size 1 kit
Label AZDye 555 Azide Plus
Abs/Em Maxima 556/572 nm
Number of Reactions 25
Storage Conditions 4C
Shipping Conditions Ambient temperature

The post Click-&-Go® Plus 555 OPP appeared first on VectorLabs.

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Click-&-Go® Plus 555 OPP Protein Synthesis Assay Kit enables sensitive, and non-radioactive chemical method to image and affinity-purify nascent proteins in cells and in animals, based on an alkyne analog of puromycin, O-propargyl-puromycin (OPP). OPP is an analog of puromycin that contains a terminal alkyne group, enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. OPP forms covalent conjugates with nascent polypeptide chains, which are rapidly turned over by the proteasome and can be visualized through copper(I)-catalyzed azide-alkyne cycloaddition. Unlike methionine analogs, OPP does not require methionine-free conditions and, uniquely, can be used to label and assay nascent proteins in whole organisms. This strategy should have broad applicability for imaging protein synthesis and for identifying proteins synthesized under various physiological and pathological conditions in vivo.

Description

Synthesis of many proteins is tightly controlled at the level of translation, and plays an essential role in fundamental processes such as cell growth and proliferation, signaling, differentiation, or death. Methods that allow imaging and identification of nascent proteins are critical for dissecting regulation of translation, both spatially and temporally, particularly in whole organisms. Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging.

The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with orange-fluorescent AZDye 555 Azide Plus (Alexa Fluor® 555 equivalent), and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

Specifications

Unit Size1 kit
LabelAZDye 555 Azide Plus
Abs/Em Maxima556/572 nm
Number of Reactions25
Storage Conditions4C
Shipping ConditionsAmbient temperature

Abs/Em Spectra

AF555

Documents

The post Click-&-Go® Plus 555 OPP appeared first on VectorLabs.

]]> Click-&-Go® Plus 488 OPP https://staging.vectorlabs.com/products/click-go-plus-488-opp/ Tue, 19 Sep 2023 19:54:16 +0000 https://staging.vectorlabs.com/?post_type=product&p=22248 Description

Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging. The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with green-fluorescent AZDye 488 Azide Plus (Alexa Fluor® 488 equivalent), and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

[caption id="attachment_25358" align="alignnone" width="1000"] Abs/Em Spectra[/caption]

Specifications

Unit Size 1 kit
Label AZDye 488 Azide Plus
Abs/Em Maxima 494/517 nm
Number of Reactions 25
Storage Conditions 4C
Shipping Conditions Ambient temperature

The post Click-&-Go® Plus 488 OPP appeared first on VectorLabs.

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Click-&-Go® Plus 488 OPP Protein Synthesis Assay Kit enables fast, sensitive, and non-radioactive detection of protein synthesis using fluorescence microscopy or high-content imaging. O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. In the next step, OPP-labeled nascent proteins are imaged through a chemoselective ligation, or “click” reaction, between the green fluorescent AZDye 488 Azide Plus (Alexa Fluor 488® equivalent) and the OPP-alkyne allowing the modified proteins to be detected by imaged-based analysis.

Description

Although protein synthesis is a conserved and essential cellular function, it is often regulated in a cell-type-specific manner to influence cell fate, growth and homeostasis. Most methods used to measure protein synthesis depend on metabolically labeling large numbers of cells with radiolabeled amino acids, stable isotope-labeled amino acids, bioorthogonal noncanonical amino acid tagging (L-azidohomoalanine or homopropargylglycine or their combination). Because these methods typically depend on specialized growth conditions, they have been largely restricted to yeast, bacteria and cell lines. Application of these techniques for investigating protein synthesis within mammalian systems in vivo has been challenging. The use of O-propargyl-puromycin (OPP), an analog of puromycin that contains a terminal alkyne group, has facilitated the quantification of protein synthesis within individual cells in vivo. OPP enters the acceptor site of ribosomes and incorporates into nascent polypeptide chains. Unlike traditional methods mentioned above, OPP is not an amino acid analog; thus, OPP can be added directly to cells in complete media (i.e., methionine-containing) or used to detect in vivo protein synthesis. It also can be used with cell lines that are sensitive to media exchanges or incubation in methionine-free media. The combination of high cell permeability and signal-to-noise ratio makes OPP an ideal candidate compound to study nascent proteomes across a wide array of cellular types and conditions. The kit contains all of the components needed to detect incorporated OPP with green-fluorescent AZDye 488 Azide Plus (Alexa Fluor® 488 equivalent), and blue-fluorescent Hoechst 33342 dye for nuclear staining. A sufficient amount of reagents is provided for imaging 25 coverslips or 250 wells using 96-well plates.

Specifications

Unit Size1 kit
LabelAZDye 488 Azide Plus
Abs/Em Maxima494/517 nm
Number of Reactions25
Storage Conditions4C
Shipping ConditionsAmbient temperature

Abs/Em Spectra

AF488

Documents

The post Click-&-Go® Plus 488 OPP appeared first on VectorLabs.

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