Abstract
The cDNA of human ribosomal protein S16 was cloned into the expression vector pET-15b. Large-scale production of the recombinant protein was carried out in E. coli cells and highly purified protein was isolated. A method for refolding the protein from inclusion bodies was optimized. The secondary structure content of the refolded protein was analyzed by CD spectroscopy. It was found that 21 +/- 4% of the amino acid sequence of the protein forms alpha-helices and 24 +/- 3% is in beta-strands. The protein structure stability was studied at various pH values and urea concentrations. The protein is quickly denatured at pH above 8.0, whereas increasing of urea concentration causes slow unfolding of the protein.
Publication types
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Comparative Study
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Research Support, Non-U.S. Gov't
MeSH terms
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Amino Acid Sequence
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Cloning, Molecular
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DNA, Complementary / genetics
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Gene Expression Regulation
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Humans
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Hydrogen-Ion Concentration
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Molecular Sequence Data
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Placenta / chemistry
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Protein Folding*
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Protein Structure, Secondary / drug effects
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Recombinant Proteins / chemistry
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Recombinant Proteins / genetics
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Recombinant Proteins / isolation & purification
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Reference Values
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Ribosomal Protein S9
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Ribosomal Proteins* / chemistry
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Ribosomal Proteins* / genetics
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Ribosomal Proteins* / isolation & purification
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Thermus thermophilus / chemistry
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Urea / pharmacology
Substances
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DNA, Complementary
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Recombinant Proteins
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Ribosomal Protein S9
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Ribosomal Proteins
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ribosomal protein S16
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Urea