ZOOM™ IPGRunner™ Combo Kit
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Invitrogen™

ZOOM™ IPGRunner™ Combo Kit

El sistema ZOOM™ IPGRunner™ es el primero que ofrece electroforesis 2D sin aceite en formato minigel. El isoelectroenfoque (IEF) deMás información
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Número de catálogoCantidad
ZM00021 kit
Número de catálogo ZM0002
Precio (MXN)
-
Cantidad:
1 kit
El sistema ZOOM™ IPGRunner™ es el primero que ofrece electroforesis 2D sin aceite en formato minigel. El isoelectroenfoque (IEF) de separación de primera dimensión suele completarse en menos de tres horas. El diseño de minigel del sistema es fácil de manejar, elimina las capas de aceite mineral y permite el procesamiento de hasta 12 muestras a la vez para un uso de alto rendimiento.

El kit combinado ZOOM™ IPGRunner™ incluye todo lo necesario para la separación de primera dimensión:
• Minicelda ZOOM™ IPGRunner™
• 10 casetes ZOOM™ IPGRunner™
• 12 tiras ZOOM™, pH 3-10 NL

Para la separación de segunda dimensión, se recomiendan los geles Novex™ ZOOM™ y la minicelda XCell SureLock™ (ambos están disponibles por separado).

Minicelda ZOOM™ IPGRunner™
La minicelda ZOOM™ IPGRunner™ consta de un núcleo Zoom™ IPGRunner, una cámara de minicelda y una tapa. El núcleo ZOOM™ IPGRunner™ se utiliza para el isoelectroenfoque de hasta 12 tiras IPG (tiras ZOOM™) cargadas en dos casetes ZOOM™ IPGRunner™.

Casete ZOOM™ IPGRunner™
El casete ZOOM™ IPGRunner™ se utiliza para la rehidratación sin aceite y el isoelectroenfoque de hasta seis tiras IPG de 7,0 cm (tiras ZOOM™) sin necesidad de unidades separadas para rehidratación e isoelectroenfoque. Los casetes ZOOM™ IPGRunner™ son desechables.

Tiras ZOOM™
Las tiras ZOOM™ miden 7 cm de largo y contienen una capa final de gel de poliacrilamida con un gradiente de pH fijo. Cada tira ZOOM™ está claramente etiquetada con un número de identificación único, un intervalo de pH y marcas de orientación (Gráfico 3). Las tiras ZOOM™ se suministran en una tarjeta de tres pliegues (Figura 4) para un fácil acceso y extracción.

Geles Novex™ ZOOM™ (disponibles por separado)
Los geles ZOOM™ son geles de poliacrilamida prefundidos diseñados para análisis 2D de proteínas tras el isoelectroenfoque con tiras ZOOM™. Se recomienda su uso con nuestra minicelda XCell SureLock™. Los geles ZOOM™ contienen un pocillo IPG y un pocillo de marcador de peso molecular. El pocillo IPG está diseñado para admitir tiras ZOOM™ de 7,0 cm. Hay dos tipos de geles ZOOM™ disponibles por separado:

Gel NuPAGE™ Novex™ ZOOM™ Bis-Tris al 4-12 %

Gel Novex™ ZOOM™ de Tri-glicina al 4-20 %
Para uso exclusivo en investigación. No apto para uso en procedimientos diagnósticos.
Especificaciones
Cantidad1 kit
Para utilizar con (equipo)Mini XCell SureLock™, Mini ZOOM™ IPGRunner™
Gel CompatibilityTiras IPG ZOOM™
Tamaño de gelTiras de 7 cm
Línea de productosIPGRunner, ZOOM
Unit Size1 kit
Contenido y almacenamiento
La minicelda ZOOM™ IPGRunner™ incluye la tapa y el núcleo de tampón ZOOM™ IPGRunner™, la cuña de tensión de gel, la barrera de tampón y la cámara de minicelda

El kit combinado ZOOM™ IPGRunner™ incluye la minicelda ZOOM™ IPGRunner™, las mechas de electrodos, la cinta de sellado, 10 casetes ZOOM™ IPGRunner™ y 12 tiras ZOOM™, pH de 3-10 NL

El kit de actualización ZOOM™ IPGRunner™ para la minicelda XCell SureLock™ incluye la tapa y el núcleo de tampón ZOOM™ IPGRunner™. Los casetes ZOOM™ IPGRunner™ incluyen mechas de electrodos y cinta de sellado

Preguntas frecuentes

What may cause streaking on the 2nd dimension gel after IEF?

There are several reasons why streaking may occur.

(1) Sample is not completely solubilized prior to application.

(2) Sample is poorly soluble in rehydration solution.

(3) Non-protein impurities in the sample can interfere with IEF, causing horizontal streaking in the final 2-D result, particularly toward the acidic side of the gel.

(4) Ionic impurities are present in sample.

(5) Ionic detergent is present in sample.

(6) Sample load is too high.

(7) Underfocusing. Focusing time was not long enough to achieve steady state focusing.

(8) Overfocusing. Extended focusing times (over 100,000 Vh) may result in electroendosmotic water and protein movement, which can produce horizontal smearing.

What should be done?

(1) Be sure that the sample is completely and stably solubilized. Note: Repeated precipitation-resolubilization cycles produce or increase horizontal streaking.

(2) Increase the concentration of the solubilizing components in the rehydration solution.

(3) Modify sample preparation to limit these contaminants or dialyze protein.

(4) Reduce salt concentration to below 10 mM by dilution or desalt the sample by dialysis. Precipitation with TCA and acetone and subsequent resuspension is another effective desalting technique that removes lipids, nucleotides and other small molecules.
Note: Specific and non-specific losses of proteins can occur with dialysis, gel chromatography, and precipitation/resuspension of samples. If the sample preparation cannot be modified, the effect of ionic impurities can be reduced by modifying the IEF protocol. Limit the voltage to 100-150 V for 2 hours, then resume a normal voltage step program. This pre-step allows the ions in the sample to move to the ends of the IPG strip.

(5) If the ionic detergent SDS is used in sample preparation, the final concentration must not exceed 0.25% after dilution into the rehydration solution. Additionally, the concentration of the non-ionic detergent present must be at least 8 times higher than the concentration of any ionic detergent to ensure complete removal of SDS from the proteins.

(6) Extend focusing time. Load less sample.

(7) Prolong focusing time.

(8) Reduce focusing time.

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

Will my proteins focus better on the ZOOM IPGRunner system if I use a voltage higher than 2000 V?

With the ZOOM system, it is not recommended to use a voltage higher than 2000 V. The ZOOM IPG Runner System is rated to 3500 VDC and 3.5 Watts, but for performing IEF, the results are optimal at maximum of 2000 V and 0.1 W per strip (~50 µA per strip).

Find additional tips, troubleshooting help, and resources within our Protein Electrophoresis and Western Blotting Support Center.

My sample is in Sample Rehydration Buffer containing urea. What would happen if it is heated?

To avoid modification of proteins, never heat a sample over 37 degrees C after adding urea. Elevated temperatures cause urea to hydrolyze to isocyanate, which modifies proteins by carbamylation.

Find additional tips, troubleshooting help, and resources within our Protein Electrophoresis and Western Blotting Support Center.

What is the maximum amount of SDS that can be in a sample for the ZOOM IPGRunner System?

We do not recommend using more than 0.2% SDS. If the percentage of SDS is too high, all the proteins will be negatively charged and will migrate to the positive electrode.

Find additional tips, troubleshooting help, and resources within our Protein Electrophoresis and Western Blotting Support Center.

What is the recommended amount of protein to load on the IPG strip?

A typical load amount is 5-10 µg for silver staining and 10-50 ug for Coomassie staining. We have determined that 400 µg of protein can be focused on our 7 cm strips with a mixture of purified standard proteins. To load this much protein, some cleaning up (like pre-fractionation) of crude lysate is required. Often this is because of the large dynamic range between "high abundance" proteins vs "low abundance" proteins, making the most abundant proteins the load-limiting factor. This is cell/tissue dependent. When testing sample preparation and run parameters, we recommend that the typical load recommended above for the stain of choice be used. After satisfactory results are obtained, higher loads can be run. Longer run times may be required when using higher loads.

Find additional tips, troubleshooting help, and resources within our Protein Electrophoresis and Western Blotting Support Center.

View all ZOOM™ IPGRunner™ Combo Kit FAQs

Citations & References (2)

Citations & References
Abstract
Apolipoprotein A-I is a selective target for myeloperoxidase-catalyzed oxidation and functional impairment in subjects with cardiovascular disease.
Authors:Zheng L, Nukuna B, Brennan ML, Sun M, Goormastic M, Settle M, Schmitt D, Fu X, Thomson L, Fox PL, Ischiropoulos H, Smith JD, Kinter M, Hazen SL,
Journal:J Clin Invest
PubMed ID:15314690
In recent studies we demonstrated that systemic levels of protein-bound nitrotyrosine (NO(2)Tyr) and myeloperoxidase (MPO), a protein that catalyzes generation of nitrating oxidants, serve as independent predictors of atherosclerotic risk, burden, and incident cardiac events. We now show both that apolipoprotein A-I (apoA-I), the primary protein constituent of HDL, is ... More
The 14-3-3 protein epsilon isoform expressed in reactive astrocytes in demyelinating lesions of multiple sclerosis binds to vimentin and glial fibrillary acidic protein in cultured human astrocytes.
Authors:Satoh J, Yamamura T, Arima K,
Journal:Am J Pathol
PubMed ID:15277231
The 14-3-3 protein family consists of acidic 30-kd proteins expressed at high levels in neurons of the central nervous system. Seven isoforms form a dimeric complex that acts as a molecular chaperone that interacts with key signaling components. Recent studies indicated that the 14-3-3 protein identified in the cerebrospinal fluid ... More