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Overview

“ Urease Purification by Filtration and Salting Out". Overview. Introduction Scheme of process Method of purification Quantity and quality. Introduction. Intracellular/exracellular protein Check the existence of protein by activity

kimberley-curry
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Overview

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  1. “Urease Purification by Filtration and Salting Out"

  2. Overview • Introduction • Scheme of process • Method of purification • Quantity and quality

  3. Introduction • Intracellular/exracellular protein • Check the existence of protein by activity • Cell distruption • Purification • Filtration • Salting out(Ammonium sulfate precipitation) • Other methods

  4. Quantity • Lowry method • Activity • Other methods • Quality • Chromatography • Electrophoresis • Summary

  5. Supernatant Crude cell Supernatant Precipitation Cell debris 1. Scheme of process • We have to confirm the existence of the protein • by activity at each step. Fig. 1. Checking the existence of the protein.

  6. 2. Activity • Correlation with purity and concentration. • Substrate and enzyme reaction. • Expressed in activity unit[U]or[U/mg]. • Check the activity with color change. When enzyme exists, the color changes from red to pink.

  7. 3. Protein Extraction Table. 1. Cell disruption methods for various tissues.

  8. Sonication • Disrupts tissue by creating vibrations which cause mechanical shearing of the cell wall. Fig. 2. Sonicator

  9. 4. Purification • Filtration • Protein solution through a membrane which retains the protein of interest. • This method is less likely to cause denaturation. Fig. 3. Concentration of a protein solution using the Amicon Concentration system.

  10. Salting out (Ammonium sulfate precipitation) • Proteins tend to aggregate and precipitate from solution. • Different proteins precipitate at different salt concentration. • Important factor : pH, temperature, protein purity. • Making to X% solution from Xo% solution. g = [515(X-Xo0]/[100-0.27x]

  11. Table. 2. Ammonium sulfate precipitation table.

  12. Other methods - Dialysis, polyethylene glycol precipitation, Ion exchange chromatography and so on.

  13. 5. Quantity • Lowry method • A combination of the copper reaction with peptide bond. • Folin-Ciocalteau reagent with phenol was found to give blue color with proteins. • There are many modified methods. • Obtain a value by spectrophotometer.

  14. Activity • The total activity(U) is in proportion to the total protein(mg or μg). • Using a spectrophotometer, we can check the activity.

  15. Other methods. - Bradford Assay, bicinchoninic acid assay, Kjeldahl method, Warburg-Christian method etc.

  16. 6. Quality • Chromatography -Accomplished by the physical and chemical properties such as size, charge, hydrophobicity and affinity.

  17. Gel filtration chromatography : separates proteins by size, column packed with porous polymeric bead. Fig. 4. Mechanism of gel filtration.

  18. Ion exchange chromatography : proteins bind to ion exchangers by electrostatic force between the protein’s surface and the charged group of exchangers Fig. 5. Schematic of cation exchange mechanism.

  19. Electrophoresis • separates proteins based on their size and charge. • SDS-PAGE – denaturing condition • Native gel electrophoresis - nondenaturing condition

  20. 7.Summary • Urease is a intracellular protein. • Most of enzyme’s size is greater than 300kDa. • Most of enzyme precipitate between 60% to 80% ammonium sulfate. • Activity is 0.86 APU. • Recovery is 30%.

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