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FOCUS™ Extraction Buffers, G-Biosciences

Supplier: G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™ Extraction Buffers, G-Biosciences
FOCUS™
786-233 786-223 786-221 786-219 786-234 786-223 786-220 786-234 786-222 786-222 786-233 786-221 786-220 786-219
82022-648EA 242.77 USD
CA82022-648 CA82022-656 CA82022-668 82022-648 82022-656 CA82022-654 82022-668 CA82022-666 CA82022-652 82022-654 82022-666 CA82022-650 82022-652 82022-650
FOCUS™ Extraction Buffers, G-Biosciences
Buffers Extraction Buffers
One of the most important considerations before running 2D gel electrophoresis is the choice of protein solubilization buffers

One way to minimize the risk of carbamylation is to prepare the urea based reagents fresh before each use. G-Biosciences has developed a series of dry urea based pre-mixed and ready-to-use solubilization buffers. Simply add an appropriate volume of the supplied rehydration buffer to the dry buffer and then use to solubilize proteins, saving time and improving the quality of IEF/2D gel electrophoresis. FOCUS™ Extraction Buffers are also designed to be used as rehydration buffers for IPG strips.
FOCUS™ Extraction Buffers are experimentally optimized concentrations of critical agents, buffering and stabilizing agents, including urea, thiourea, Nonidet® P-40, CHAPS, and sulfobetaines (SB). The FOCUS™ Extraction Buffers are designed to produce optimal protein extraction and improved spot resolution for 2D gel analysis.
A range of FOCUS™ Extraction Buffers have been developed (see table) and depending on the nature of the samples, one or more of the buffers suitable for your applications can be ordered. FOCUS™ Extraction Buffer-I is suitable for most applications, however for stronger solubilization effects, we recommend FOCUS™ Extraction Buffer-II, III, IV, V or VI. For analysis of a proteome, a single buffer may not be suitable and sequential solubilization using different FOCUS™ Extraction Buffers will help in identifying new proteins. For analysis of a proteome, a single buffer may not be suitable and sequential solubilization using different FOCUS™ Extraction Buffers will help in identifying new proteins.

The suitable buffer must solubilize proteins effectively, without disturbing the native charge of the proteins. Urea, a common chaotrope, is widely used for solubilization and denaturation of proteins. One of the disadvantages of using urea is carbamylation. Urea in water exists in equilibrium with ammonium cyanate, the level of which increases with increasing temperature and pH. Cyanate reacts with α-amino and ε-amino groups of proteins and induces a change in the isoelectric point of proteins. This leads to artifactual results and therefore carbamylation must be avoided.

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