Tampón de muestras NuPAGE™ LDS (4X)
Tampón de muestras NuPAGE™ LDS (4X)
Citas y referencias (9)
Invitrogen™

Tampón de muestras NuPAGE™ LDS (4X)

El tampón de muestra de LDS NuPAGE (4X) se utiliza para preparar muestras de proteínas para desnaturalizar la electroforesis enMás información
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Número de catálogoCantidad
NP000710 ml
NP0008250 ml
Número de catálogo NP0007
Precio (MXN)
-
Cantidad:
10 ml
El tampón de muestra de LDS NuPAGE (4X) se utiliza para preparar muestras de proteínas para desnaturalizar la electroforesis en gel con geles Bis-Tris o Tris-acetato. Contiene dodecil sulfato de litio, pH 8,4, que permite la actividad máxima del agente reductor.

Consulte todos los tampones y reactivos disponibles para SDS-PAGE

El tampón de muestra de LDS NuPAGE contiene Coomassie G250 y rojo de fenol como tintes de seguimiento en lugar de azul de bromofenol. Coomassie G250 proporciona nitidez a la parte delantera del colorante con tampones de desplazamiento tanto de MES como de MOPS SDS y migra mucho más cerca del frente de iones en movimiento que el azul de bromofenol. El azul de bromofenol funciona más lentamente que algunos péptidos con el tampón de desplazamiento MES SDS. Esto garantiza que los péptidos pequeños no se deshagan en los geles.

Uso: Caliente la muestra en una dilución 1X (reducida o no reducida) a 70 °C durante 10 minutos para obtener unos resultados óptimos.

Nota: El tampón de muestra de LDS NuPAGE debe estar a temperatura ambiente (25 °C) antes de su uso. Se trata de una solución muy viscosa y concentrada que contiene el doble de LDS en comparación con la cantidad de SDS en los tampones de muestra habituales. El tampón de muestra de LDS NuPAGE también contiene una mayor concentración de glicerol.
Para uso exclusivo en investigación. No apto para uso en procedimientos diagnósticos.
Especificaciones
TampónTampones de carga de muestras
Concentración4 X
Compatibilidad del gelGeles NuPAGE™
Línea de productosNuPAGE
Tipo de productoTampón de muestras LDS
Cantidad10 ml
Condiciones de envíoAprobado para su envío a temperatura ambiente o en hielo húmedo
Tipo de gelGel NuPAGE
Unit SizeEach
Contenido y almacenamiento
Tampón de muestra (4X) que contiene sulfato de dodecilo de litio (LDS) a pH 8,5 con SERVA Blue G250 y rojo de fenol.

Almacenar en 4° C a 25° C.

Preguntas frecuentes

Can I prepare my protein sample with the reducing agent and store it for future use?

DTT is not stable, so it must be added and the reduction performed just prior to loading your samples.

Find additional tips, troubleshooting help, and resources within our Protein Gel 1D Electrophoresis Support Center.

My LDS or SDS sample buffer precipitates when stored at 4 degrees C. Can I warm it up? Can I store it at room temperature?

Precipitation of the LDS or SDS at 4 degrees C is normal. Bring the buffer to room temperature and mix until the LDS/SDS goes into solution. If you do not want to wait for it to dissolve, you can store the sample buffer at room temperature.

Find additional tips, troubleshooting help, and resources within our Protein Gel 1D Electrophoresis Support Center.

How are Bolt gels different than NuPAGE gels?

While they are both Bis-Tris based gels, the chemistries are very different since Bolt gels are optimized for western blotting. Another key difference is the wedge well design of the Bolt gels, which allows larger sample volumes to be loaded.

Find additional tips, troubleshooting help, and resources within our Protein Gel 1D Electrophoresis Support Center.

What is the advantage of NuPAGE Gels over regular Tris-Glycine gels?

The neutral operating pH of the NuPAGE Gels and buffers provides following advantages over the Laemmli system:
-Longer shelf life of 8-12 months due to improved gel stability
-Improved protein stability during electrophoresis at neutral pH resulting in sharper band resolution and accurate results (Moos et al, 1998)
-Complete reduction of disulfides under mild heating conditions (70 degrees C for 10 min) and absence of cleavage of asp-pro bonds using the NuPAGE LDS Sample buffer (pH > 7.0 at 70 degrees C)
-Reduced state of the proteins maintained during electrophoresis and blotting of the proteins by the NuPAGE Antioxidant
Please refer to the following paper: Moos M Jr, Nguyen NY, Liu TY (1988) Reproducible High Yield Sequencing of Proteins Electrophoretically Separated and Transferred to an Inert Support. J Biol Chem 263:6005-6008.

Find additional tips, troubleshooting help, and resources within our Protein Gel 1D Electrophoresis Support Center.

What is the composition of the NuPAGE LDS Sample Buffer and what is the recipe for the 4X formulation?

The composition of the 1X NuPAGE LDS Sample Buffer is as follows:

141 mM Tris base
106 mM Tris HCl
2% LDS
10% Glycerol
0.51 mM EDTA
0.22 mM SERVA Blue G
0.175 mM Phenol Red
pH 8.5


To prepare 10 mL of 4 X NuPAGE LDS Sample Buffer, dissolve the following reagents to 8 mL ultrapure water:

Tris HCl 0.666 g
Tris Base 0.682 g
LDS 0.800 g
EDTA 0.006 g
Glycerol 4 g
SERVA Blue G (1 solution) 0.75 mL
Phenol Red (1 solution) 0.25 mL

Mix well and adjust the volume to 10 mL with ultrapure water. Store at +4. The buffer is stable for 6 months when stored at +4°C.

Find additional tips, troubleshooting help, and resources within our Protein Gel 1D Electrophoresis Support Center.

View all Tampón de muestras NuPAGE™ LDS (4X) FAQs

Citations & References (9)

Citations & References
Abstract
Characterization of four murine homologs of the human ov-serpin monocyte neutrophil elastase inhibitor MNEI (SERPINB1).
Authors: Benarafa Charaf; Cooley Jessica; Zeng Weilan; Bird Phillip I; Remold-O'Donnell Eileen;
Journal:J Biol Chem
PubMed ID:12189154
'The human ov-serpin monocyte neutrophil elastase inhibitor (MNEI) is encoded by a single gene SERPINB1. It is a highly efficient inhibitor of neutrophil granule proteases. Four murine genes with high sequence identity with MNEI were identified and fully sequenced, and these were named EIA, EIB, EIC, and EID. EIA, EIB ... More
Novel Modulation of Neuronal Nicotinic Acetylcholine Receptors by Association with the Endogenous Prototoxin lynx1.
Authors: Ibañez-Tallon Inés; Miwa Julie M; Wang Hai Long; Adams Niels C; Crabtree Gregg W; Sine Steven M; Heintz Nathaniel;
Journal:Neuron
PubMed ID:11906696
We previously identified lynx1 as a neuronal membrane molecule related to snake alpha-neurotoxins able to modulate nAChRs. Here, we show that lynx1 colocalizes with nAChRs on CNS neurons and physically associates with nAChRs. Single-channel recordings show that lynx1 promotes the largest of three current amplitudes elicited by ACh through alpha(4)beta(2) ... More
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
In vivo functional assay of a recombinant aquaporin in Pichia pastoris.
Authors:Daniels MJ, Wood MR, Yeager M,
Journal:Appl Environ Microbiol
PubMed ID:16461705
The water channel protein PvTIP3;1 (alpha-TIP) is a member of the major intrinsic protein (MIP) membrane channel family. We overexpressed this eukaryotic aquaporin in the methylotrophic yeast Pichia pastoris, and immunogold labeling of cellular cryosections showed that the protein accumulated in the plasma membrane, as well as vacuolar and other ... More
Spermidine but not spermine is essential for hypusine biosynthesis and growth in Saccharomyces cerevisiae: Spermine is converted to spermidine in vivo by the FMS1-amine oxidase.
Authors:Chattopadhyay MK, Tabor CW, Tabor H,
Journal:Proc Natl Acad Sci U S A
PubMed ID:14617780
In our earlier work we showed that either spermidine or spermine could support the growth of spe2Delta or spe3Delta polyamine-requiring mutants, but it was unclear whether the cells had a specific requirement for either of these amines. In the current work, we demonstrate that spermidine is specifically required for the ... More
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