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cAMP Binding Protein Assay for Widespread Use in Cell Signaling Studies
Author(s) -
Hen-Li Chen,
Laurie K. McCauley,
Nisha J. D’Silva
Publication year - 2002
Publication title -
biotechniques
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.617
H-Index - 131
eISSN - 1940-9818
pISSN - 0736-6205
DOI - 10.2144/02331st03
Subject(s) - protein kinase a , protein purification , binding protein , signal transduction , creb1 , ligand binding assay , biology , plasma protein binding , microbiology and biotechnology , receptor , biochemistry , phosphorylation , chemistry , transcription factor , creb , gene
cAMP plays a critical role in intracellular signaling pathways that regulate proliferation or differentiation. The cAMP binding protein assay, using a naturally derived cAMP binding protein, is one of the most widely used methods for cAMP determination. The major steps of this binding assay include purification of the binding protein, cAMP extraction from samples, and quantification of the cAMP. Most purification methods of the cAMP binding protein were published before 1975, and many of the materials and methods are outdated. Here we describe an updated method of purification of cAMP binding protein from bovine skeletal muscle with the advantages of simplicity, low cost, and high yield. The isolation procedures can be completed in two days using commercially available materials and equipment. The cAMP binding properties of the isolated protein can be utilized for more than two years. Binding protein isolated from 1 kg bovine muscle is sufficient for at least 3×10 4 assay tubes. Furthermore, we describe the techniques of cAMP extraction and quantification that have been used successfully in studying parathyroid hormone signaling as an example of a G protein-linked seven transmembrane domain receptor that signals through the protein kinase A pathway.

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