Luminex 200™ Performance Verification Kit
Luminex 200™ Performance Verification Kit
Invitrogen™

Luminex 200™ Performance Verification Kit

Le kit de vérification des performances Luminex 200 est destiné au système Luminex 200 et contient des contrôles xMAP utilisésAfficher plus
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RéférenceQuantité
LX2RPVERK2525 utilisations
Référence LX2RPVERK25
Prix (EUR)
624,00
Each
Ajouter au panier
Quantité:
25 utilisations
Prix (EUR)
624,00
Each
Ajouter au panier
Le kit de vérification des performances Luminex 200 est destiné au système Luminex 200 et contient des contrôles xMAP utilisés pour vérifier l’étalonnage des canaux de classification MagPlex et MicroPlex et du canal rapporteur. Les contrôles fluidiques sont inclus pour la détection précoce, ainsi qu’un CD spécifique au lot pour l’importation des valeurs cibles. Le kit est conçu pour être utilisé avec la plaque de maintenance automatisée (AMP). Les barrettes pour l’AMP sont fournies avec chaque kit. Chaque kit fournit 25 vérifications.
Usage exclusivement réservé à la recherche. Ne pas utiliser pour des procédures de diagnostic.
Spécifications
Gamme de produitsLuminex
Quantité25 utilisations
Conditions d’expéditionGlace humide
TypeKit de vérification des performances
Unit SizeEach
Contenu et stockage
• Barrettes à 28 puits
• CD de kit de vérification des performances L x 100/200
• Microsphères de contrôle de classification Luminex
• Microsphères de contrôle de classification MagPlex
• Microsphères de contrôle de rapporteur Luminex
• Microsphères fluidiques 1 xMAP
• Microsphères fluidiques 2 xMAP

Conserver (entre 2° et 8°C)

Foire aux questions (FAQ)

During my ProcartaPlex assay data analysis, I am getting a warning message that there is high bead aggregation. What should I do?

Here are possible causes and solutions for this issue:

- Check the protocol settings (make sure you select the correct DD settings).
- Check the level of sheath fluid and empty the waste.
- Before acquiring the plate, run calibration and verification beads on the Luminex instrument.

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

During my ProcartaPlex assay data analysis, the beads fall below or to the lower left of their bead region on the bead map. Why is this?

Here are possible causes and solutions for this issue:

This usually indicates that the beads have been photobleached. This problem can also be caused by exposing the beads to organic solvents. Unfortunately, the assay will have to be repeated because the beads cannot be restored. The beads must be protected from light and organic solvents.
Alternatively, the instrument may be off in its measurements or you may have a calibration issue. Call the manufacturer for a service appointment.

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

During my ProcartaPlex assay data analysis, beads do not appear in the region gated. What happened?

This indicates that an incorrect buffer was used for the final step. The Wash Solution provided in the kit must be used for washing the beads and the Reading Buffer should be used for resuspending the beads before loading them into the Luminex instrument. The osmolarity of the solution will impact the size of the bead, and any change in the bead size will alter detection by the instrument.

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

The bead counts for all of my ProcartaPlex assay wells are erratic. What went wrong?

Here are some suggestions:

- Before acquiring the plate, run calibration and verification beads on the Luminex instrument.
- Review the instrument settings and make sure they are appropriate for the assay being run (adjustment of needle height, make sure you select the correct bead gates and the correct DD settings).
- Shake the plate before acquisition on the instrument to resuspend the beads.
- Vortex the beads for 30 sec before adding them into the plate.
- Washing: Do not forget to keep the plate for about 2 mins on the Hand-Held Magnetic Plate Washer before emptying the plate.

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

The bead count for my ProcartaPlex assay standard curve is correct and regular. The bead count for my samples is erratic and I get a warning message saying "The acquisition had at least one region that did not reach the maximum count". What should I do?

This pattern is indicative of a sample matrix effect. Here are some suggestions:

- Confirm that the sample has been clarified and is free of debris and free of lipids (5-10 min centrifugation recommended).
- Confirm that there is at least a 1:1 ratio of sample to assay diluent for serum, plasma samples. For cell lysates or tissue homogenates, confirm that the sample has been diluted appropriately in assay buffer to reduce the concentration of detergent in the lysis buffer to ⋜0.01%. For other sample types, further sample optimization may be required.

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

View all Luminex 200™ Performance Verification Kit FAQs