Marqueurs d’ARN Millennium™
Marqueurs d’ARN Millennium™
Invitrogen™

Marqueurs d’ARN Millennium™

Les marqueurs d’ARN Ambion® Millenium™ ont été conçus pour une détermination précise de la taille des transcripts d’ARN à simpleAfficher plus
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RéférenceQuantité
AM7150Promo Image50 μl
Référence AM7150
Prix (EUR)
266,50
Special offer
Online exclusive
termine: 15-Aug-2025
410,00
Économisez 143,50 (35%)
Each
En stock
Ajouter au panier
Quantité:
50 μl
Recurring order eligible. Learn more »
Grand volume ou format personnalisé
Prix (EUR)
266,50
Special offer
Online exclusive
termine: 15-Aug-2025
410,00
Économisez 143,50 (35%)
Each
Ajouter au panier
Ask our AI about this Product
Les marqueurs d’ARN Ambion® Millenium™ ont été conçus pour une détermination précise de la taille des transcripts d’ARN à simple brin de 0,5 à 9 kb et peuvent être utilisés dans n’importe quel protocole Northern. Suffisamment de marqueurs sont fournis pour 25 voies de gel Northern. Il s’agit d’un mélange de 10 transcripts d’ARN distincts avec des dimensions faciles à retenir : 0,5, 1, 1,5, 2, 2,5, 3, 4, 5, 6 et 9 kilobases. Les marqueurs peuvent être colorés avec du bromure d’éthidium pendant ou après l’électrophorèse. En raison de leur quantité et de leur espacement uniforme, ces marqueurs sont parfaits pour élaborer des courbes d’étalonnage très précises pour la détermination de la taille de l’ARNm. Ils fournissent également une échelle de référence facilitant la vérification et la comparaison des bandes connues. Les marqueurs d’ARN de 1 à 2 µg (1 à 2 µg) Millenium™ produiront 10 bandes distinctes sur un gel d’agarose dénaturant à 1 % avec une coloration au bromure d’éthidium. Tous les lots de marqueurs subissent des tests de nucléase rigoureux et sont stables pendant la nuit à 37°C.
Usage exclusivement réservé à la recherche. Ne pas utiliser pour des procédures de diagnostic.
Spécifications
Concentration1 μg/μl
Compatibilité du gelGels contenant du formaldéhyde, gels d’agarose dénaturant
Gamme de produitsAmbion™, Millennium Markers™
Type de produitMarqueur d’ARN
Quantité50 μl
Prêt à chargerNon
Conditions d’expéditionGlace carbonique
Plage de dimensions0,5 à 9 kb
Unit SizeEach
Contenu et stockage
Conserver en dessous de –70°C.
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Foire aux questions (FAQ)

Why are my RNA bands not sharp?

(1) RNA was not completely denatured. Electrophorese RNA under denaturing conditions. Use urea, formamide or formaldehyde gels, or glyoxal-treated RNA.

(2) For glyoxal-treated RNA, a buffer gradient formed during electrophoresis. Recirculate buffer during electrophoresis to prevent gradient formation.

What is the cause of extra bands when using an RNA ladder?

Extra bands appear in RNA Ladders for a few reasons:

(1) RNA was not completely denatured. Electrophorese RNA under denaturing conditions. Use urea, formamide or formaldehyde gels, or glyoxal-treated RNA.

(2) Extra bands may be a result of using formaldehyde that is not fresh; the pH becomes acidic in older formaldehyde. In our hands, when fresh formaldehyde with neutral pH was used, the extra bands disappeared.

(3) Alternatively, if the extra bands appear after hybridization, it could be that the gel purified probe contains contaminating vector DNA (pUC or pBR) that hybridizes to RNA Ladder template DNA.

Why are some of the RNA marker bands not visible?

Missing RNA bands may be due to:

(1) A small amount of RNA diffused out of gel during extended destaining. Minimize destaining time. Destaining for 2 hours is sufficient for most applications.

(2) RNA bands of similar molecular size were not resolved. Use the correct gel type and denaturing conditions.

Why are the RNA bands disappearing when looking and photographing a gel on a UV box?

RNA was exposed to UV light for extended periods of time. Minimize exposure to UV light. Stain and destain gels in the dark and photograph the gel immediately.

Why are the RNA marker bands so faint?

Many factors could affect the intensity of the bands as summarized below.

(1) Insufficient RNA was loaded on the gel. Increase the amount of RNA loaded.

(2) RNA was degraded. Avoid nuclease contamination of the RNA standards. Store RNA at -70 degrees C in formamide. Deionize formamide and glyoxal, store aliquots at -20 degrees C.

(3) RNA was electrophoresed off the gel. Electrophorese the gel for less time, at a lower voltage, or in a higher percentage gel.

(4) For ethidium bromide-stained RNA, improper UV light source was used. Use short-wavelength (254 nm) UV light. For ethidium bromide-stained RNA, improper staining and destaining conditions were used. Stain in the dark with 5 mg/mL ethidium bromide. For thin (3.2 mm) formaldehyde gels, stain 5 min and destain 1 h. For thicker gels, stain 30 min and destain 2 hr. To reduce background staining, use 0.66 M formaldehyde instead of 2.2 M formaldehyde in gels. For glyoxal RNA gels, stain and destain in 0.5 M ammonium acetate to help reduce background staining.

(5) For radiolabeled RNA, an improper labeling method was used.

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Certificats

Numéro de lotCertificate TypeDateCatalog Number(s)
3257560Certificate of Analysis21 juil. 2025AM7150
3244944Certificate of Analysis10 juin 2025AM7150
3205504Certificate of Analysis26 mai 2025AM7150
3196865Certificate of Analysis08 avr. 2025AM7150
3173886Certificate of Analysis26 mars 2025AM7150
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