Techniques in Protein Biochemistry Stryer Short Course Chapter 5.

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Presentation transcript:

Techniques in Protein Biochemistry Stryer Short Course Chapter 5

Protein Analysis Isolation Purification Anaylsis of purity Activity Assay Sequencing

Isolation Homogenate Fractions Differential centrifugation Crude extract

Purification Solubility Chromatography – Size – Charge – Affinity HPLC

Separation by Solubility Salting-in and salting- out Competition for water of hydration dialysis

Gel Filtration Chromatography Size exclusion Porous polyacrylamide or agarose beads

Ion-Exchange Chromatography Choose charge of beads based on net charge of protein of interest Elute using more concentrated ion buffer

Affinity Chromatography Most specific Most selective Most difficult Once developed, can be a highly effective purification technique

Affinity Chromatography Immunoglobins Poly-His tail Bound inhibitors – Serine proteases Biotin/streptavidin Calmodulin binding proteins And many others

Qualitative Purity Analysis Electrophoresis and staining Approximate size (kDa) Relative purity Denature protein – Charge it evenly with SDS

SDS-PAGE

Isoelectric Focusing Based on isoelectric point Buffer gradient Electrophoresis with no SDS

Two-Dimensional Electrophoresis Separate based on pI and on size First, isoelectric focusing Second, gel laid horizontally on SDS- PAGE Separation of hudreds of proteins

Application Find relative increase in protein concentration in disease state or physiological response

Quantitative Analysis Activity assay – Enzymatic or binding – Colorimetric, radiolabel – Continuous/discontinuous Total protein (Bradford, Lowry)

Binding Assay Example: estrogen receptor Binds tightly to radiolabeled estradiol Ultracentifugation

Quantitation

Traditional Sequencing Full hydrolysis Amino acid composition

Edman Degradation

Sequencing Longer Polypeptides Edman limited to about 50 residues Can cleave longer peptides into shorter ones with specific hydrolysis Then overlap

Modern Techniques: MS MALDI-TOF

Identify Known Proteins Fast Reliable Automated Technician-level

Sequencing Unknown Proteins Tandem Mass Spectroscopy After precursor ion analyzed, can be bombarded and fragmented Analysis of fragments by second mass analyzer