ELK Biotechnology Optional Related loading controls. For example, PCNA, an loading control protein in the nucleus, is expressed in the S phase of DNA and is therefore not recommended for non-proliferating cells. Commonly used loading control proteins are those that are highly expressed by housekeeping genes and are required for cell development and maintenance of cell viability. The loading control protein selected needs to be highly expressed in the sample to be tested. For example, if the molecular weight of the target protein is 40 KD, it is not appropriate to choose β-actin or GAPDH as the loading control, but rather α-Tubulin or β-tubulin. When selecting a loading control antibody, the molecular weight of the target protein should be taken into account, generally ensuring that the difference between the molecular weight of the target protein and the loading control protein is more than 5 KD. There are fewer studies of samples from other sources, so it is appropriate to refer to journal literature data and select appropriate proteins as loading control s. Western blot processing is a well-established procedure that includes. For experimental samples of plant origin, plantactin, Rubisco, etc. Image Lab features simplified lane loading normalization and automated detection. Mammalian tissue or cell samples, usually β-actin, β-tubulin, GAPDH, Lamin B, Histone H3, Na,Katpase etc. The first thing to consider is what species the experimental sample comes from.ġ. This article will briefly describe five principles that should be followed in the selection of loading control antibodies. The selection of different loading control antibodies for different samples is also the key to the success of WB experiments. There are many types of loading control antibodies, such as β-actin, β-tubunlin, GAPDH, Vinculin, LaminB, PCNA, etc. Loading control antibodies are divided into unlabelled and labelled types, and markers include biotin, HRP, FITC, PE, Cy dyes and Alexa Fluor dyes. Loading control antibodies are also used as positive controls for co-staining in immunofluorescence studies of target proteins. (4) Evaluate whether the total amount of protein in each well is generally consistent (3) Comparison of relative changes in trace amounts of products (2) Testing for correct gene expression products (1) Check if the whole WB process is in order Key functions of loading control antibodies Such controls can help identify differences in expression levels between samples, whether due to actual protein levels in cell lysates or differences in loading. The loading control antibody can be used to evaluate the efficiency of Western Blot and compare the amount of protein loaded per well in the gel.
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