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TOPICS IN (NANO) BIOTECHNOLOGY Lecture 5

PhD Course. TOPICS IN (NANO) BIOTECHNOLOGY Lecture 5. 19th April, 200 6. An important set of proteins: Enzymes. Enzymes. Thousands of biochemical reactions proceed at any given instant within living cells. These reactions are catalyzed by enzymes;

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TOPICS IN (NANO) BIOTECHNOLOGY Lecture 5

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  1. PhD Course TOPICS IN (NANO) BIOTECHNOLOGY Lecture 5 19th April, 2006

  2. An important set of proteins: Enzymes

  3. Enzymes • Thousands of biochemical reactions proceed at any given instant within living cells. These reactions are catalyzed by enzymes; • Enzymes are mostly proteins. But two important enzymes are most certainly to be RNA (ribozymes). One is the ribosome (peptidyl transfer) and the other is the spliceosome (splicing of intron); • Enzymes are the agents of metabolic function. Enzymes play key functions in controlling rate of reaction, coupling reactions, and sensing the momentary metabolic needs of the cell.

  4. Enzymatic Catalysis Suited to Biological systems • Higher reactions rates • Milder reaction conditions • Greater reaction specificity • Capacity for regulation

  5. Enzymatic Catalysis Suited to Biological systems • All chemical reactions require some amount of energy to get them started. This energy is called activation energy. • The way enzymes operate is by effectively lowering the amount of activation energy required for a chemical reaction to start.  • Sometimes this happens because enzymes might weaken a covalent bond within a substrate molecule. In other cases this lowering of activation energy seems to happen because the enzyme holds the substrate molecules in a particular position that increases the likely that the molecules are going to react. http://www.chem.uwec.edu/Chem150_S06/Pages/Lecture-slides/C150_lect07_enzyme.html

  6. Enzyme-substrate interactions-a prerequisite for catalysis • Forces Important for substrate recognition • Active Site Characteristics

  7. Models for Enzyme Substrate Interactions Example: Carboxypeptidase

  8. Enzyme Cofactors ATP NAD(P) CoASH

  9. Enzyme Cofactors This is an oxidation reaction and results in the removal of two hydrogen ions and two electrons which are added to the NAD+, converting it to NADH and H+. This is the first reaction in the metabolism of alcohol. CH3CH2OH + NAD+ ---> CH3CH=O + NADH + H+ The active site of ADH has two binding regions. The coenzyme binding site, where NAD+ binds, and the substrate binding site, where the alcohol binds. Most of the binding site for the NAD+ is hydrophobic as represented in green.

  10. Enzyme Classifications

  11. Enzyme Classifications Oxido-reductases Transferases

  12. Enzyme Classifications Hydrolases Lyases

  13. Enzyme Classifications Isomerases Ligases

  14. Enzymatic Reactions with Stereochemical Specificity

  15. An important set of proteins: Antibodies

  16. So, what is an antibody?

  17. What is an antigen? Any substance capable of producing a specific immune response

  18. So, what is an antibody? http://www.cat.cc.md.us/courses/bio141/lecguide/unit3/viruses/opsonvir.html http://www.cat.cc.md.us/courses/bio141/lecguide/unit3/viruses/adcc.html http://www.learner.org/channel/courses/biology/archive/animations/hires/a_hiv1_h.html

  19. B cells and T cells The two major classes of lymphocytes are B cells, which grow to maturity in the bone marrow, and T cells, which mature in the thymus, high in the chest behind the breastbone. B cells produce antibodies that circulate in the blood and lymph streams and attach to foreign antigens to mark them for destruction by other immune cells. B cells are part of what is known as antibody-mediated or humoral immunity, so called because the antibodies circulate in blood and lymph, which the ancient Greeks called, the body's "humors."

  20. B cells and T cells B cells become plasma cells, which produce antibodies when a foreign antigen triggers the immune response.

  21. B cells and T cells Certain T cells, which also patrol the blood and lymph for foreign invaders, can do more than mark the antigens; they attack and destroy diseased cells they recognize as foreign. T lymphocytes are responsible for cell-mediated immunity (or cellular immunity). T cells also orchestrate, regulate and coordinate the overall immune response. T cells depend on unique cell surface molecules called the major histocompatibility complex (MHC) to help them recognize antigen fragments. http://www.bio.davidson.edu/courses/Immunology/Bio307.html

  22. Recognition of antigen by B and T-cells • B-cells can recognise an epitope alone • T-cells can recognise antigen only when it is associated with an MHC molecule • There are four cell membrane molecules that are involved in recognition: • membrane bound antibody (B-cells) • T-cell receptor or TCR (T-cells) • MHC class I • MHC class II

  23. What is an antibody? • Antigen-specific products of B-cells • Present on the B-cell surface • Secreted by plasma cells • Effectors of the humoral immune response, searching and neutralising/eliminate antigens • Two functions: • to bind specifically to molecules from the pathogen • to recruit other cells and molecules to destroy the pathogen once the antibody is bound to it

  24. Structure of the antibody molecule • The antigen-binding region of the antibody molecule is called the variable region or V region • The region of the antibody molecule that engages the effector functions of the immune system is known as the constant region or C region. • They are joined by a polypeptide chain that is known as the hinge region

  25. Structure of the antibody molecule • X-ray crystallography has revealed that the overall shape is roughly that of a Y • Each arm of the Y is formed by the association of a light chain with a heavy chain • The leg of the Y is formed by the pairing of the carboxyl-terminal halves of two heavy chains

  26. Light Chain • There are two types of light chain • kappa (k) chains • lambda (l) chains • No functional difference has been found between antibodies having l or k light chains • In humans 60% of the light chains are k, and 40% are l

  27. Heavy chain • There are five heavy chain classes or isotypes • IgM (m chain) • IgD (d chain) • IgG (g chain) • IgA (a chain) • IgE (e chain) • These determine the functional activity of an antibody molecule

  28. IgG • IgG • most abundant immunoglobulin in the blood • provides the bulk of immunity to most blood-borne infections

  29. IgD • IgD • present in low quantities in circulation • primary function is that of antigen receptor on B-cells

  30. IgE • IgE • present in the serum at very low levels • plays a role in acute inflammation and infection by parasites

  31. IgA • IgA • present in external secretions, such as tears, milk, saliva • first line of defense against microbial invaders at mucosal surfaces

  32. IgM • IgM • first antibody produced and expressed on the surface of B-cells, also secreted • 10 combining binding sites per molecule make it very effective in removal of microbes

  33. Enzyme Linked ImmunoSorbent Assay (ELISA)

  34. ELISA • An analytical method based on the exploitation of the highly specific and selective nature of antibodies • Radioimmunoassay developed in mid-sixties and the first report of enzyme immunoassay was in 1976 (Rubenstein et al.)

  35. How do we produce polyclonal and monoclonal antibodies? Polyclonal antibodies - larger quantities may be produced at a time - sometimes better selectivity and sensitivity due to recogintion of multiple epitopes - no guarantee of batch to batch reproducibility Monoclonal antibodies - long and expensive process - sometimes lower selectivity and sensitivity in comparison to Pabs observed - once cell line established constant reproducible supply of antibodies …. forever

  36. Enzyme Labels ENZYME SUBSTRATE  (nm) Horseradish peroxidase o-phenylenediamine dihydrochloride (OPD) 492* tetramethylbenzidine (TMB) 450* 2,2’-azino-di-(3-ethyl)benzthiazoline 414* sulphonic acid (ABTS) 5-aminosalicyclic acid (ASA) 450* [* H2O2 added and reaction stopped with sulphuric acid] Alkaline phosphatase p-nitrophenyl phosphate 405 -D-galactosidase o-nitrophenyl -D-galactosidase 405 Glucose oxidase Glucose (H2O2 produced and HRP and substrate used) • Enzymes are protein catalysts present in all living cells. • They catalyse all essential reactions to supply the energy and/or chemical chnages necessary for vital activities. • Enzymes bind their corresponding substrates with high specificity. E + S  ES  E + P • Release of this product may be monitored by measuring, for example, colour change. • With the substrate in excess, the signal observed is proportional to the amount of enzyme present. • Following enzymatic action, the products of the reaction are released and the enzyme is free to bind another substrate molecule. • The speed with which this occurs is known as the turnover rate. • Enzymes are conjugated to antibodies to provide a means of measuring the mount of antibody present. • Enzymes commonly used are horse radish peroxidase, alkaline phosphatase, -galactosidase and glucose oxidase.

  37. TMB/OPD/APTS (no colour) p-nitrophenylphosphate (no colour) p-nitrophenylgalacto-pyronasidase (no colour) HRP ALP -GAL Oxidised product p-nitrophenol p-nitrophenol Measurement principle Note: Can also label antigen with enzyme!

  38. 1 2 3 4 5 6 7 8 9 10 11 12 A B C D E F G H Microtitre plates 96-well ELISA plate Surface of polystyrene is activated with amine groups for enhanced binding of antibody NUNC plates - best well to well reproducibility in binding (also very useful web site www.nunc.com) With the exception of checkerboard titrations, avoid using column 1 and 12 and rows A and H, due to uneven heating effects

  39. substrate substrate substrate Sandwich assay product product product Response Concentration Useful for large molecules Robust assay - all reagents in excess Use with Pabs or different MAbs

  40. substrate substrate Competition assay product product Useful for small molecules Reportedly less sensitive Concentrations of reagents critical Response Concentration

  41. substrate substrate product product Response Concentration Displacement assay One step assay In practise difficulties to achieve - effect of non specific displacement Sub-optimum haptens met with some success

  42. http://www.biology.arizona.edu/immunology/activities/elisa/technique.html?http://www.biology.arizona.edu/immunology/activities/elisa/technique.html?

  43. APTAMER DEFINITION Artificial nucleic acid ligands that can be generated against amino acids, drugs, proteins and even cells. They bind their target with selectivity, specificity and affinity equal and often superior to those of antibodies. Aptamers are isolated from combinatorial libraries of synthetic nucleic acid by exponential enrichment via an in vitro iterative process of adsorption, recovery and reamplification, known as SELEX (systematic evolution of ligands by exponential enrichment).

  44. SELEX

  45. SELEX

  46. APTAMERS VS. ANTIBODIES  can be selected against toxins/molecules that do not elicit good immune response  selection is in vitro process - does not need animals  kinetic parameters (kon/koff) can be controlled  can be regenerated in minutes, stable for long term storage, can be transported at ambient temperature  can be used in non-physiological conditions  produced by chemical synthesis no ‘batch to batch’ variation  negative selection against structures similar to target structure can improve specificity BUT low stability = short life Can be solved by chemical modification, spiegelmers, mixed LNA/DNA structures

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