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Citations & References (80)
Invitrogen™
Antibody Labeling Kits for 1 mg
Form stable dye–protein conjugates across the spectrum with any of our 16 available protein labeling kits for use in various fluorescence microscopy applications including flow cytometry, IHC/IF/ICC, FISH, and high content analysis.
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| Catalog Number | Label or Dye |
|---|---|
| A10235 | Alexa Fluor 488 |
| A10170 | Alexa Fluor 350 |
| A10236 | Alexa Fluor 532 |
| A10237 | Alexa Fluor 546 |
| A20174 | Alexa Fluor 555 |
| A10238 | Alexa Fluor 568 |
| A10239 | Alexa Fluor 594 |
| A20170 | Alexa Fluor 633 |
| A20173 | Alexa Fluor 647 |
| A20171 | Alexa Fluor 660 |
| A20172 also known as A-20172 | Alexa Fluor 680 |
| F10240 | FITC (Fluorescein) |
| O10241 also known as O-10241 | Oregon Green 488 |
| P30012 | Pacific Blue |
| D20655 | Biotin (DSB-X) |
Catalog number A10235
Price (EUR)
876,00
Each
Label or Dye:
Alexa Fluor 488
Price (EUR)
876,00
Each
Ready to use in just 90 minutes, our protein labeling kits include an easy-to-use, pre-packed spin column for rapid dye removal and typical recovery greater than 85%. Each kit contains enough reagent for 3–5 protein conjugation reactions. Our kits provide better results due to lower background fluorescence, less nonspecific binding, and easier workflows for protein conjugation with 16 different fluorophores.
- Fluorescently label up to 1 mg of protein per reaction (three reactions per kit)
- Label 0.5–3 mg per reaction with DSB-X Biotin Protein Labeling Kit (five reactions per kit)
- Labeled proteins ready to use in 90 min. (∼15 min. hands-on time)
- Rapidly purify proteins by quickly removing unbound dye using pre-packed Zeba Dye and Biotin Removal Spin Columns (7K MWCO, Cat. No. A44299) for >85% recovery
- Includes detailed instructions for determining degree of labeling (DOL)
Each protein labeling kit contains everything you need to perform 3-5 separate labeling reactions and purify the resulting conjugates. The reactive dye has either a succinimidyl ester (SE) or a tetrafluorophenyl (TFP) ester moiety that reacts efficiently with primary amines of proteins to form stable dye–protein conjugates. Each of the vials of reactive dye provided in the kit is sufficient for labeling 1 mg of a variety of purified proteins, including growth factors, cytokines, nanobodies, enzymes, cell-adhesion molecules, and antibodies.
Direct labeling with fluorophores allows multiple primary antibodies of the same isotype (derived from the same species) to be used in the same experiment. Stabilizing proteins such as BSA should be removed from the sample before labeling.
The different protein labeling kits
- Blue-fluorescent Alexa Fluor 350 —excitation and emission maxima of 346/442 nm
- Green-fluorescent Alexa Fluor 488 – excitation and emission maxima of 494/519 nm; excited using a 488 nm argon laser line and detected under standard FITC/Cy2 filters
- Yellow-fluorescent Alexa Fluor 532 – excitation and emission maxima of 530/554 nm; excited using a 532 nm Nd:YAG laser line and detected under standard Rhodamine 6G filters
- Orange-fluorescent Alexa Fluor 546 – excitation and emission maxima of 554/570 nm; excited using a 543 nm He-Ne laser line and detected under standard TRITC/Cy3 filters
- Orange-fluorescent Alexa Fluor 555 – excitation and emission maxima of 555/565 nm; excited using a 543 nm He-Ne laser line and detected under standard TRITC/Cy3 filters
- Orange-red-fluorescent Alexa Fluor 568 – excitation and emission maxima of 577/603 nm; excited using a 568 nm Kr laser line and detected under standard Rhodamine Red/Cy3.5 filters
- Red-fluorescent Alexa Fluor 594 – excitation and emission maxima of 590/617 nm; excited using a 594 nm Kr or He-Ne laser line and detected under standard Texas Red filters
- Far-red-fluorescent Alexa Fluor 633 – excitation and emission maxima of 632/647 nm
- Far-red-fluorescent Alexa Fluor 647 – excitation and emission maxima of 650/668 nm; excited using a 633 or 635 nm Kr or He-Ne laser line and detected under standard APC/Cy5 filters.
- Far-red-fluorescent Alexa Fluor 660 – excitation and emission maxima of 663/690 nm
- Near-IR-fluorescent Alexa Fluor 680 – excitation and emission maxima of 680/700 nm
- Green-fluorescent Fluorescein-EX – excitation and emission maxima of 494/518 nm
- Oregon Green 488 – excitation and emission maxima of 496/524 nm
- Pacific Blue – a violet light excitable dye with an excitation and emission maxima of 410/455 nm
- Texas Red-X – excitation and emission maxima of 595/615 nm
- DSB-X Biotin – Conjugates can be reversibly bound to biotin-binding proteins such as streptavidin or avidin. The concentration (mg/mL) of the DSB-X Biotin-labeled antibody preparation can be determined by measuring the absorbance of the dialyzed sample at 280 nm and dividing this value by 1.3 or 1.4 when measured in solution in a cuvette with a 1-cm pathlength. DSB-X Biotin does not absorb significantly at 280 nm.
For labeling smaller amounts of antibodies (∼100 μg), we recommend our antibody labeling kits. Please review the protein labeling kit user manual for more in depth information, protocols, molecular weights, and degree of labeling for each dye.
For Research Use Only. Not for use in diagnostic procedures.
Specifications
ColorGreen
Detection MethodFluorescence
Excitation/Emission494/519
Label TypeAlexa Fluor Dyes
Labeling MethodConjugation-Based
Labeling Scale1 mg
Product LineAlexa Fluor
Product TypeProtein Labeling Kit
Quantity1 kit
Shipping ConditionRoom Temperature
Chemical ReactivityAmine
Labeling TargetAntibodies, Proteins
Label or DyeAlexa Fluor 488
SolubilityDMSO (Dimethylsulfoxide)
Unit SizeEach
Contents & Storage
Store in refrigerator 2°C to 8°C and protect from light.
Frequently asked questions (FAQs)
Can I use 50 μg of protein with Fluorescent Protein Labeling Kits?
What formulation of antibody should I use for conjugation for small animal in vivo imaging?
What is degree of labeling (DOL)?
Citations & References (80)
Citations & References
Abstract
Golgi apparatus immunolocalization of endomannosidase suggests post-endoplasmic reticulum glucose trimming: implications for quality control.
Journal:Mol Biol Cell
PubMed ID:11102520
'Trimming of N-linked oligosaccharides by endoplasmic reticulum (ER) glucosidase II is implicated in quality control of protein folding. An alternate glucosidase II-independent deglucosylation pathway exists, in which endo-alpha-mannosidase cleaves internally the glucose-substituted mannose residue of oligosaccharides. By immunogold labeling, we detected most endomannosidase in cis/medial Golgi cisternae (83.8% of immunogold
Glycosylation influences the lectin activities of the macrophage mannose receptor.
Journal:J Biol Chem
PubMed ID:15983039
'The mannose receptor (MR) is a heavily glycosylated endocytic receptor that recognizes both mannosylated and sulfated ligands through its C-type lectin domains and cysteine-rich (CR) domain, respectively. Differential binding properties have been described for MR isolated from different sources, and we hypothesized that this could be due to altered glycosylation.
An endocytosed TGN38 chimeric protein is delivered to the TGN after trafficking through the endocytic recycling compartment in CHO cells.
Journal:J Cell Biol
PubMed ID:9722606
'To examine TGN38 trafficking from the cell surface to the TGN, CHO cells were stably transfected with a chimeric transmembrane protein, TacTGN38. We used fluorescent and 125I-labeled anti-Tac IgG and Fab fragments to follow TacTGN38''s postendocytic trafficking. At steady-state, anti-Tac was mainly in the TGN, but shortly after endocytosis it
Alexa dyes, a series of new fluorescent dyes that yield exceptionally bright, photostable conjugates.
Journal:J Histochem Cytochem
PubMed ID:10449539
'Alexa 350, Alexa 430, Alexa 488, Alexa 532, Alexa 546, Alexa 568, and Alexa 594 dyes are a new series of fluorescent dyes with emission/excitation spectra similar to those of AMCA, Lucifer Yellow, fluorescein, rhodamine 6G, tetramethylrhodamine or Cy3, lissamine rhodamine B, and Texas Red, respectively (the numbers in the
Removal of the membrane-anchoring domain of epidermal growth factor leads to intracrine signaling and disruption of mammary epithelial cell organization.
Journal:J Cell Biol
PubMed ID:9832559
'Autocrine EGF-receptor (EGFR) ligands are normally made as membrane-anchored precursors that are proteolytically processed to yield mature, soluble peptides. To explore the function of the membrane-anchoring domain of EGF, we expressed artificial EGF genes either with or without this structure in human mammary epithelial cells (HMEC). These cells require activation