Presentation is loading. Please wait.

Presentation is loading. Please wait.

1 Mechanism Testing of the Drug (Modified Megestrol) Mr.Pasavi Ratchapongsirikul.

Published byDarnell Harman Modified over 9 years ago

Similar presentations

Presentation on theme: "1 Mechanism Testing of the Drug (Modified Megestrol) Mr.Pasavi Ratchapongsirikul."— Presentation transcript:

1 1 Mechanism Testing of the Drug (Modified Megestrol) Mr.Pasavi Ratchapongsirikul

2 2 Outline of the Presentation Introduction –Key function of the drug OBJECTIVES –Mechanism testing and the techniques used System of the experiments( In vitro and In vivo ) Methods used in the experiments Summary

3 3 KEY function of the drug “Able to covalently modify DNA, forming adducts that bind to the variant estrogen receptor (vER) ” Mechanism testing of the Drug

4 4 OBJECTIVES To determine binding affinity of the drug for the estrogen receptors Competitive Binding Assay To examine covalent modification of DNA by the drug DNA Covalent modification Test To examine the drug-modified DNA on the variant estrogen receptor binding Electrophoretic Mobility Shift Assay Mechanism testing of the Drug

5 5 In vitro In vitro (cell free extract) 1.Relative Affinity of the Drug to ERs 2.DNA Covalent modification test 3.The drug modified DNA binding to the variant estrogen receptor In vitro (cell line) 4.DNA Covalent modification test In vivo 5.DNA Covalent modification test (in mice)

6 6 1.Relative Affinity of the Drug to the ERs ( In Vitro, cell free extract) To determine binding affinity of the drug for the estrogen receptors Competitive Binding Assay Technique: Competitive Binding Assay

7 7 Method Varied concentrations of the drug or Estradiol(E2)* are combined with [3H]-E2 Incubate with wtER or vER Remove unbound radioactivity Measure the radioactivity of [3H]-E2 bound ER

8 8 Incubation of: [ 3 H]-E 2 Drug (increasing conc) ER ( wtER or vER ) Buffer Method Mixture : Bound ligand* + Free ligand* *Ligand =Drug or [3H]-E2 Ligand Bound ligand* Free ligand*

9 9 [3H]-E2(ER-[3H]-E2) (ER-Drug) (Drug),(E2) (ER-[3H]-E2) (ER-Drug) Free ligand separate “ bound ligand” from “free ligand” by HAP extract the [3H]-E2 from the HAP by ethanol Measure : radioactivity [3H]-E2 ER

10 10 Plot [3H]-E2 bound(%) against drug conc(M) In the presence of wtER or vER Plot [3H]-E2 bound(%) against E2 conc(M) estimate: IC 50 (50%inhibition of (3H]-E2 binding) of the drug “nonlinear curve fitting” Calculate: Relative Binding Affinity (RBA) Calculations RBA (%) = Data Obtained: ReceptorRBA(%) of the Drug wtER…?.... vER…?....

11 11 2. DNA Covalent modification test (In Vitro, cell free extract) To examine the DNA covalent adduct formation by the drug Method: DNA Covalent Modification Test

12 12 Methods 14 (C) labeled DrugSalmon testes DNA is incubated with 14 (C) labeled Drug Aliquot is removed at various time points Hydrolyze DNA covalent compound (Remove non-covalent DNA adduct) Determine the DNA concentration & measure the radioactivity

13 13 Measure Radioactivity Removed ! Adducts Reaction time (h) m/z Relative Abundance ESI-MSScintillation

14 14 3. The drug-modified DNA binding to the variant estrogen receptor (In Vitro, cell free extract) To examine drug-modified DNA binding to the variant estrogen receptor Method: Electrophoretic Mobility Shift Assay

15 15 Prepare: oligonucleotide 5’-d(AATATTGGCCAATATT)-3’ labeled with (  - 32 P) ATP at 5’ end = ( 32 P) DNA Incubate: –Untreated DNA (Control)+ vER (1) –warhead + DNA + vER (2) –The drug + DNA + vER (3) Method Electrophoretic Mobility Shift Assay

16 16 Control (1) Warhead (2) Drug (3) vER (16 mer) DNA

17 17 Gel electrophoresis Analyze gel by PhosphoImager DNA migrationretarded due tocomplex with ER-LBD Where; (1)Untreated DNA (2)Warhead modified DNA +vER (3)Drug modified DNA+ vER

18 18 4. DNA modification test (In vitro, Cell line) HepG2Incubate HepG2 cell line with the drug Isolate DNA from HepG2 cell Hydrolyze DNA covalent compounds Analyze the covalent products by electrospray ionization mass spectrometry (ESI-MS)

19 19 5. DNA modification test (In vivo, nude mice bearing of hepG2) a xenographmiceAdminister a single dose of the drug to a xenograph mice Isolate DNA from xenograph Hydrolyze DNA covalent compounds Analyze the covalent products by electrospray ionization mass spectrometry(ESI-MS)

20 20 Electrospray Ionization Mass Spectrometry (ESI-MS) m/z A B Analysis of the drug –DNA adducts formed in vitro and in vivo A, The drug reacted with the DNA B, The drug reacted with the DNA in HepG2 cell line C, The drug reacted with the DNA in xenograph mice Expected: “The Same Compound” Relative Abundance C

21 21 Binding Affinity of the drug to the estrogen receptor is determined by “Competitive Binding Assay” The drug covalent modification of DNA is examined by “DNA Covalent modification Test” The complex formation between vER and the drug- modified DNA is examined by “ Electrophoretic Mobility Shift Assay” SUMMARY The experiments are conducted in vitro and in vivo to test the drug’s mechanisms

Download ppt "1 Mechanism Testing of the Drug (Modified Megestrol) Mr.Pasavi Ratchapongsirikul."

Similar presentations

Antibodies Analytical Techniques Utilizing Antibodies: flow cytometry

Antibodies Analytical Techniques Utilizing Antibodies: flow cytometry
Preclinical Drug Development Miss Sirikan Nawapan.

Preclinical Drug Development Miss Sirikan Nawapan.
Supplementary Figure S1.

Supplementary Figure S1.
Vickie S. Wilson EDVMS Meeting December 10-12-2003 Vickie S. Wilson EDVMS Meeting December 10-12-2003 Androgen Receptor Binding Assay Update.

Vickie S. Wilson EDVMS Meeting December Vickie S. Wilson EDVMS Meeting December Androgen Receptor Binding Assay Update.
Mph1 (60 fmol) 1 234567 9 101112 8 1314 15 16 B 1718 -B-B- ++ + + ++++ + ++ + ------ 14 10 25 14 10 2514 10 25 1 nt 5 nt15 nt Lane Time (min) 5’ flap length.

Mph1 (60 fmol) B B-B nt 5 nt15 nt Lane Time (min) 5’ flap length.
Novel Drug Design Modified Megestrol by Group II.

Novel Drug Design Modified Megestrol by Group II.
Measurement in Science Bioassays and Immunoassays Karim Meeran 23 October 2009.

Measurement in Science Bioassays and Immunoassays Karim Meeran 23 October 2009.
SOUTHERN BLOTTING Presented by: Imran Fakhroni Nurkholis Nugroho Nino Radiansyah Indra Ardi Fauzi Arfita Sari.

SOUTHERN BLOTTING Presented by: Imran Fakhroni Nurkholis Nugroho Nino Radiansyah Indra Ardi Fauzi Arfita Sari.
Introduction to Immunoassays

Introduction to Immunoassays
MAP Kinase family regulates the nuclear localization of Nrf2 By: Ngan Nguyen Tory Hagen Linus Pauling Institute.

MAP Kinase family regulates the nuclear localization of Nrf2 By: Ngan Nguyen Tory Hagen Linus Pauling Institute.
Altogen Labs, 4020 S Industrial Dr, Suite 130, Austin TX 78744, USA  512-433-6177 ELIS A Enzyme-Linked Immunosorbent Assay ELISA.

Altogen Labs, 4020 S Industrial Dr, Suite 130, Austin TX 78744, USA  ELIS A Enzyme-Linked Immunosorbent Assay ELISA.
Production of Modified Megestrol by Jittima Khorungkul.

Production of Modified Megestrol by Jittima Khorungkul.
Inhibited Enzyme Kinetics Inhibitors may bind to enzyme and reduce their activity. Enzyme inhibition may be reversible or irreversible. For reversible.

Inhibited Enzyme Kinetics Inhibitors may bind to enzyme and reduce their activity. Enzyme inhibition may be reversible or irreversible. For reversible.
1 CLINICAL CHEMISTRY CHAPTER 6 IMMUNOASSAYS. 2 Introduction –In the last chapter, we discussed a variety of analytical techniques –In this chapter we’ll.

1 CLINICAL CHEMISTRY CHAPTER 6 IMMUNOASSAYS. 2 Introduction –In the last chapter, we discussed a variety of analytical techniques –In this chapter we’ll.
Quantifying the drug-target binding affinity. Receptors as targets (Receptors are 45% of current drug targets) Receptors are areas of proteins found in.

Quantifying the drug-target binding affinity. Receptors as targets (Receptors are 45% of current drug targets) Receptors are areas of proteins found in.
PHC 222 Part(I) Dr. Huda Al Salem Lecture (7). Factors that affect the efficacy 2- Concentration-Response Curves: Agonist Antagonist Partial agonist Desensetization.

PHC 222 Part(I) Dr. Huda Al Salem Lecture (7). Factors that affect the efficacy 2- Concentration-Response Curves: Agonist Antagonist Partial agonist Desensetization.
PROTEIN PURIFICATION AND ANALYSIS. Assays Need measures for the object (enzyme activity, chromophore, etc.) and for total protein concentration:

PROTEIN PURIFICATION AND ANALYSIS. Assays Need measures for the object (enzyme activity, chromophore, etc.) and for total protein concentration:
Electro Mobility Shift Assay EMSA Band Shift Assay Gel Shift Assay

Electro Mobility Shift Assay EMSA Band Shift Assay Gel Shift Assay
CENTER FOR BIOLOGICAL SEQUENCE ANALYSIS BiC BioCentrum-DTU Technical University of Denmark Cleavage sites and binding affinities.

CENTER FOR BIOLOGICAL SEQUENCE ANALYSIS BiC BioCentrum-DTU Technical University of Denmark Cleavage sites and binding affinities.
BioIntelligence Lab Reaction discovery enabled by DNA-templated synthesis and in vitro selection Matthew W. Kanan, Mary M. Rozenman, Kaori Sakurai, Thomas.

BioIntelligence Lab Reaction discovery enabled by DNA-templated synthesis and in vitro selection Matthew W. Kanan, Mary M. Rozenman, Kaori Sakurai, Thomas.

Similar presentations

Ads by Google