A-431 Whole Cell Lysate: sc-2201

The A-431 Whole Cell Lysate is produced from the A-431 cell line, which originates from an epidermoid carcinoma of the skin from an 85-year-old female. This lysate is a comprehensive preparation containing all the cellular components extracted from A-431 cells, thus providing a rich source of cellular material for research. It includes proteins, nucleic acids, lipids, and other small molecules, making it extremely useful for a wide range of biochemical and molecular biology investigations. Researchers utilize this lysate to study protein expression profiles, investigate enzyme activities, and analyze cellular structures and functions under various experimental conditions. The A-431 cell line itself is particularly noted for its high expression of the epidermal growth factor receptor (EGFR), making the lysate ideal for studying EGFR signaling pathways without the complexity of isolating specific proteins or complexes. This allows scientists to explore cellular responses in a system that closely mimics the natural state of the cells. The A-431 Whole Cell Lysate has been instrumental in advancing our understanding of cellular mechanisms and protein interactions, facilitating explorations into how cells communicate, respond to environmental stimuli, and regulate various metabolic and signal transduction pathways. This lysate serves as a crucial tool in basic research, particularly in fields such as cell biology and proteomics.

A-431 Whole Cell Lysate References:

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2. Assembly of alpha-hemolysin on A431 cells leads to clustering of Caveolin-1.  |  Vijayvargia, R., et al. 2004. Biochem Biophys Res Commun. 324: 1124-9. PMID: 15485671
3. Stress-induced phosphorylation of caveolin-1 and p38, and down-regulation of EGFr and ERK by the dietary lectin jacalin in two human carcinoma cell lines.  |  Sahasrabuddhe, AA., et al. 2006. Cell Stress Chaperones. 11: 135-47. PMID: 16817319
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5. Three-dimensional culture using a radial flow bioreactor induces matrix metalloprotease 7-mediated EMT-like process in tumor cells via TGFbeta1/Smad pathway.  |  Shibata, S., et al. 2009. Int J Oncol. 34: 1433-48. PMID: 19360357
6. Modulation of PP2A activity by Jacalin: is it through caveolae and ER chaperones?  |  Ahmed, N., et al. 2010. Glycoconj J. 27: 723-34. PMID: 19823931
7. Low ascorbate levels are associated with increased hypoxia-inducible factor-1 activity and an aggressive tumor phenotype in endometrial cancer.  |  Kuiper, C., et al. 2010. Cancer Res. 70: 5749-58. PMID: 20570889
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10. Separation of novel phosphoproteins of Porphyromonas gingivalis using phosphate-affinity chromatography.  |  Izumigawa, M., et al. 2016. Microbiol Immunol. 60: 702-707. PMID: 27663267
11. Microfluidic communicating vessel chip for expedited and automated immunomagnetic assays.  |  Yang, Y. and Zeng, Y. 2018. Lab Chip. 18: 3830-3839. PMID: 30394473
12. Selective and reversible modification of kinase cysteines with chlorofluoroacetamides.  |  Shindo, N., et al. 2019. Nat Chem Biol. 15: 250-258. PMID: 30643284
13. Monoclonal antibodies specific for peptide epitopes of the epidermal growth factor receptor′s extracellular domain.  |  Baron, AT., et al. 1997. Hybridoma. 16: 259-71. PMID: 9219036
14. A sandwich type acridinium-linked immunosorbent assay (ALISA) detects soluble ErbB1 (sErbB1) in normal human sera.  |  Baron, AT., et al. 1998. J Immunol Methods. 219: 23-43. PMID: 9831386