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Quality Control Biochemistry

Quality Control Biochemistry. IEF (Isoelectric Focusing) HPLC (High Pressure Liquid Chromatography ) ELISA (Enzyme-Linked Immunosorbent Assay) SDS-PAGE (Sodium Dodecyl Sulfate- Polyacrylamide Gel Electrophoresis). Sampling. Sample Environment Sample Water Sample Equipment

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Quality Control Biochemistry

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  1. Quality Control Biochemistry IEF (Isoelectric Focusing) HPLC (High Pressure Liquid Chromatography) ELISA (Enzyme-Linked Immunosorbent Assay) SDS-PAGE (Sodium Dodecyl Sulfate-Polyacrylamide Gel Electrophoresis)

  2. Sampling • Sample Environment • Sample Water • Sample Equipment • Sample Process Samples processed in QC Microbiology (already covered in Lecture One) and QC Biochemistry

  3. Common Process Compounds and Methods of Removal or Purification*

  4. Test: Total Protein via Spectrophotemetric Absorption at 280nm Tryphophan Phenylalanine Tyrosine ALL ABSORB LIGHT AT 280 nm Crude, not necessarily quantitative Same amount of protein will show different A280 depending on amount of above amino acids

  5. Test: Total Protein Bradford Assay Coomassie Brilliant Blue G Dye and Spectrophotometry at 595 and 450nm

  6. ELISAs and PAGE • ELISAs: Use antibody reagents and a microtitre plate reader to determine the concentration and/or the activity of a protein of interest. • SDS-PAGE: Use acrylamide gel electrophoresis to separate proteins according to molecular weight (a single band indicates purity – if validated to do so). • IEF (Isoelectric Focusing): Use an SDS-PAGE gel box (or CE = capillary electrophoresis) to determine the pI or the pH at which the protein of interest is neutral.

  7. ELISAsAntibodies as Reagents ELISAS are Immunoassays which use an antibody (Ab) to detect and quantify substances Ab are extremely specific – ADVANTAGE Ab can not be detected, need a marker: Radioactive labels (RIA) Enzymes (EIA) – Horseradish Peroxidase or Alkaline Phosphatase Fluorescent Tag (FIA) Chemiluminescencent Tag

  8. ELISAs There are several types of ELISAs including direct (sandwich), indirect, competitive and activity ELISAs. ELISAs are read on a microtitre plate reader which is a mini-spectrophotometer that determines the absorption or transmission of a beam of light of a particular wave length passing through a solution of the protein of interest. Using standards to generate a standard curve, one can determine the concentration of the protein of interest in a sample.

  9. HSA Direct ELISA ResultsSpring 2009 Data

  10. ELISA Equipment Multi-Channel Pipettor Microtitre Plate Reader

  11. ELISA Process To make an ELISA, one must utilize antibodies to the protein of interest. The first antibody recognizes the protein of interest. The second antibody recognizes another epitope on the protein of interest and carries a signal (or enzyme) that will be used to quantify the protein of interest.

  12. Direct ELISA = Antibody Sandwich

  13. Direct and Indirect ELISA Animation usmlemd.wordpress.com/2007/06/12/elisa-test/

  14. Acrylamide Gel Electrophoresis • Sodium Dodecyl Sulfate-Polyacrylamide Gel Electrophoresis* • SDS-PAGE • demonstrates proteins in a sample • separates proteins based on molecular weight • quantify proteins by densitometry • step in Western blot used to identify protein • Isoelectric Focusing • IEF • identifies the pH at which a protein carries no net charge • used to develop chromatographic separation protocols/SOPs • *Developed by Laemmli in 1970

  15. SDS-PAGE SDS-PAGE Gel Box SDS-PAGE Overview SDS Polyacrylamide gels (SDS-PAGE) are called “denaturing gels” because they contain sodium dodecyl sulfate (SDS), an ionic detergent that binds to the amino acid residues in the proteins. Due to its ionic properties, SDS confers a net negative charge on all the proteins, overcoming any intrinsic charge; in this way the proteins uniformly migrate toward the positive electrode. SDS also disrupts the secondary and tertiary structure of the proteins, essentially destroying their globular configuration and making them into linear molecules that then migrate in the electric field on the basis of their size. PAGE is a very powerful technique because even small differences in molecular weights produce distinguishable bands on a gel.

  16. SDS-PAGE • detect proteins using Coomassie Blue Stain • characterize (MW) • quantify (densitometry) • determine other proteins in a sample (purity) • step in Western blot (used to identify)

  17. Molecular Weight DeterminationSDS-PAGE • Run SDS PAGE with known standards (MW markers) • Graph distance from wells to bands to make standard curve • Measure distance from well unknown protein traveled • Compare on standard curve to determine MW of unknown

  18. IdentificationImmunoblot (Western) from PAGE

  19. Identification and Quantification HPLC High Pressure Liquid Chromatography (HPLC) uses the same components and processes as LPLC; HPLC uses small samples injected with high pressure.

  20. QC Biochemistry: Additional Techniques to Determine Purity, Molecular Weight, Function and 1o, 2o, 3o, 4o Structure 2D Gel Electrophoresis Capillary Eletrophoresis Analytical Ultracentrifugation Mass Sepctrometry Fluorescence Spectroscopy Amino Acid Sequencing X-ray Crystallography Nuclear Magnetic Resonance PCR (used in QC Microbiology)

  21. Small QC Laboratory in Production Area of a Biomanufacturing Facility Biological Safety Cabinets (BSCs) Pass Through for Samples

  22. Small QC Laboratory in Production Area of a Biomanufacturing Facility Nova Analyate Analyzer Centrifuge

  23. Small QC Laboratory in Production Area of a Biomanufacturing Facility Micropipettor Set Compound Microscope

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