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Qdot™ 605 Biotin Conjugate Kit
Citations et références (3)
Invitrogen™

Qdot™ 605 Biotin Conjugate Kit

Les nanocristaux Qdot™ 605 marqués à la biotine sont disponibles pour détecter les sondes de streptavidine ou pour créer desAfficher plus
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RéférenceQuantité
Q10301MP1 kit
Référence Q10301MP
Prix (EUR)
936,00
Each
Quantité:
1 kit
Prix (EUR)
936,00
Each
Les nanocristaux Qdot™ 605 marqués à la biotine sont disponibles pour détecter les sondes de streptavidine ou pour créer des conjugués non covalents avec des molécules marquées à la streptavidine ou avec d’autres molécules biotinylées à l’aide d’un pont de streptavidine. Le produit est fourni sous forme de 250 µl d’une solution de 2 µm et comprend 30 ml de tampon d’incubation Qdot™.
Usage exclusivement réservé à la recherche. Ne pas utiliser pour des procédures de diagnostic.
Spécifications
Type de produitKit de conjugaison de biotine Qdot
Quantité1 kit
Conditions d’expéditionTempérature ambiante
Gamme de produitsQdot
Unit SizeEach
Contenu et stockage
Conserver au réfrigérateur (2–8°C).

Foire aux questions (FAQ)

What is the best way to remove white precipitate from my ITK Qdot nanocrystals?

Spinning your ITK Qdot nanocrystals at approximately 3,000 rpm for 3-5 minutes should remove the white precipitate from the supernatant. Use the supernatant immediately.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

I see a white precipitate in my ITK Qdot nanocrystals; should I be concerned?

The precipitate in the organic ITK Qdot nanocrystals occurs with some frequency. The ITK Qdot nanocrystals sometimes include impurities that show as a white precipitate.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

Why do my Qdot nanocrystals appear to be blinking?

Blinking is an inherent property of quantum dots; in fact, all single-luminescent molecules blink, including organic dyes. The brightness and photostability of Qdot nanocrystals makes the blinking more visibly apparent. Under higher energy excitation, Qdot nanocrystals blink even faster.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

My Qdot nanocrystals were brightly fluorescent before I mounted my samples; now I'm seeing a loss of fluorescence. Why is this happening?

Appropriate mounting media selection is very important to retain the fluorescence of Qdot nanocrystals. In our studies, Qdot nanocrystals work best with the following mountants:

HistoMount medium (Cat No. 00-8030); best for long term archiving
Cytoseal 60 Mountant
Clarion Mountant
Most polyvinyl alcohol-based mountants (limited storage time, less than weeks)
Water-based mountants (limited storage time, less than week)
Up to 50% glycerol (limited storage time, less than week)
Note: We do not recommend using ProLong mounting media with Qdot nanocrystals as it will quench their fluorescence.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

Why can't I freeze my Qdot nanocrystal solution?

Freezing will cause the product to aggregate. The Qdot nanocrystals cannot be dispersed into solution after aggregation.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

View all Qdot™ 605 Biotin Conjugate Kit FAQs

Citations et références (3)

Citations et références
Abstract
Nanoparticles as fluorescence labels: is size all that matters?
Authors:Swift JL, Cramb DT,
Journal:Biophys J
PubMed ID:18390610
'Fluorescent labels are often used in bioassays as a means to detect and characterize ligand-receptor binding. This is due in part to the inherently high sensitivity of fluorescence-based technology and the relative accessibility of the technique. There is often little concern raised as to whether or not the fluorescent label ... More
Measuring an antibody affinity distribution molecule by molecule.
Authors:Temirov JP, Bradbury AR, Werner JH,
Journal:Anal Chem
PubMed ID:18847284
Single molecule fluorescence microscopy was used to observe the binding and unbinding of hapten decorated quantum dots to individual surface immobilized antibodies. The fluorescence time history from an individual antibody site can be used to calculate its binding affinity. While quantum dot blinking occurs during these measurements, we describe a ... More
A two-photon excitation fluorescence cross-correlation assay for a model ligand-receptor binding system using quantum dots.
Authors:Swift JL, Heuff R, Cramb DT
Journal:Biophys J
PubMed ID:16299079
Two-photon excitation fluorescence cross-correlation spectroscopy (TPE-XCS) is a very suitable method for studying interactions of two distinctly labeled fluorescent molecules. As such, it lends itself nicely to the study of ligand-receptor interactions. By labeling the ligand with one color of fluorescent dye and the receptor with another, it is possible ... More