![]() This paper also provides you with the latest publication guidelines, so you can meet standards and obtain publishable data. A more unified procedure among members of the scientific community can help mitigate variation and increase overall reproducibility. By helping to minimize error in Western blot methodology, it can guide you toward more precise data. “A systematic approach to quantitative Western blot analysis” is a step-by-step workflow and the ideal resource for your lab. ![]() Paired with original data examples, these easy-to-follow steps can guide your Western blots for useful quantitative results. This guide also emphasizes that replicating your results is extremely important: it confirms that there is reproducibility or actual differences between samples-not experimental variability. This valuable resource explains the importance of validating primary antibodies and ILCs, post-translationally modified (PTM) proteins, and the linear range of detection. In addition to core concepts, you can follow the paper’s step-by-step systematic approach to help you get reliable data. Imager: Odyssey ® CLx resolution: 169 μm Intensity: auto mode. Blocking buffer: Intercept Blocking Buffer (TBS) Intercept T20 (TBS) Antibody Diluent Protein ladder: Chameleon duo ladder (LI-COR P/N 928-70000 Lot# C70803-03). CLR was identified at 4.5 micrograms for both cell types. Combined linear range for total protein extract and OCT-4 protein detection was plotted for both cell extract types (c, d). (a-a”) Individual linear range of detection for total protein and OCT-4 was determined for control cell extracts (a - a”) as well as for experimental cell extracts (b – b”). Subsequently, the blots were incubated in Intercept Blocking Buffer for one hour at room temperature and thereafter in Anti-Oct-4 antibody (CST #2750 Lot #4) and IRDye 800CW Goat anti-Rabbit IgG (H + L). All the blots were incubated with Revert 700 Total Protein Stain (LI-COR P/N 926-11010) to visualize total protein extract in each lane. 4-fold dilution of cell extracts from HEK293T untreated control (a’-a”) as well as knockdown HEK293T (experimental) (b-b”) category were loaded onto 10% Bis-Tris gel (NP0303BOX) and run under the MOPS buffer system. Consequently, this guide can help enhance your data reproducibility and increase the likelihood of publication.Ĭombined Linear Range (CLR) detection of Total protein extract and OCT-4 in HEK293T cells. By establishing a solid foundation and deep comprehension of these concepts, sources of error in your experimentation become minimal. ![]() Additionally, learn how to use normalization techniques to correct for unavoidable and small variations, such as sample concentration or cell number. This makes sure that you have no variability in HKP expression that can introduce error into your analysis. You can also use an HKP, or single endogenous reference protein, as an internal loading control (ILC) but must first validate it. ![]() Empirical calculations of the amount of protein to load onto a gel are highly important: ensuring that this amount is within the linear range can help ensure that your quantitation is accurate. Take an in-depth look at the core concepts of Western blots - including linear range, housekeeping proteins (HKPs), and proper normalization techniques. This systematic guide helps you understand the most critical aspects in getting accurate, precise results. Not only will you have more confidence in your data, but it will help ensure that you are in alignment with best practices. Refer to this guide as you work through your experimental design and analysis. Original data examples and publication guidelines for each step are also provided and explained, ensuring that you are fully prepared before submitting your research. It carefully walks you through each core concept of a Western blot then thoroughly describes a systematic approach for achieving quantitative data in your own lab. The recent paper “A systematic approach to quantitative Western blot analysis” by Lakshmi Pillai-Kastoori, Amy Schutz-Geschwender, and Jeff Harford is the ideal resource for researchers who use Western blotting techniques in their research and want reliable, robust data.
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