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Evaluation 3

Chakard Chalayut
Chakard Chalayut

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Cloning, Expression, Purification and Enzymological Characterization of NS2B/NS3 Protease / RNA Helicase protein of Japanese Encephalitis Virus. Chakard Chalayut Advisor: Asst. Prof. Gerd Katzenmeier, Ph.D. Laboratory of Molecular Virology Institute of Molecular Biology & Genetics
Japanese Encephalitis Virus (JEV) -Flaviviridae family -Mosquito-borne neurotropic flavivirus •causes severe central nerve system diseases
Japanese Encephalitis Virus (JEV) Culex tritaeniorhynchus. Source: fehd.gov.hk
Japanese Encephalitis Virus (JEV)
Japanese Encephalitis Virus (JEV) Source : vietnammedicalpractice.com
Japanese Encephalitis Virus (JEV)
Japanese Encephalitis Virus (JEV) JEV causes severe central nerve system diseases such as p o l i o mye l i t i s - l i ke acute flaccid paralysis, aseptic meningitis and encephalitis Source:wonder.cdc.gov
Japanese Encephalitis Virus (JEV)
Japanese Encephalitis Virus (JEV)
Japanese Encephalitis Virus (JEV) 50,000 Cases
Japanese Encephalitis Virus (JEV) 30% fatality rate
Japanese Encephalitis Virus (JEV) 10,000 Cases
Prevention and treatment of JEV disease
Prevention and treatment of JEV disease Drug No drug exist
Prevention and treatment of JEV disease Drug No drug exist Vaccine development Available vaccine
Prevention and treatment of JEV disease Drug No drug exist Vaccine development Available vaccine Elimination of mosquitoes Mosquitoes control breeding places
Molecular biology of Japanese Encephalitis Virus
The NS2B • 130 aa • activating domain central hydrophilic region (Falgout et al, 1993) • 3 membrane spanning parts
The NS2B • 130 aa • activating domain central hydrophilic region (Falgout et al, 1993) • 3 membrane spanning parts hydrophobicity plot
The NS2B • 130 aa • activating domain central hydrophilic region (Falgout et al, 1993) • 3 membrane spanning parts hydrophobicity plot 51 DMWLERAADISWEMDAAITGSSRRLDVKLDDDGDFHLIDDPGVP 95
The NS2B • 130 aa Hypothetical model • activating domain NS2B-NS3 complex central hydrophilic region (Falgout et al, 1993) • 3 membrane spanning parts hydrophobicity plot ฺBrinkworth et al, 1999 51 DMWLERAADISWEMDAAITGSSRRLDVKLDDDGDFHLIDDPGVP 95
The NS3 Theoretical model from PDB 2I84
The NS3 Protease Theoretical model from PDB 2I84
The NS3 Protease NTPase RNA Helicase Theoretical model from PDB 2I84
The NS3 •Chymotrypsin-like fold 2-β barrel domains •Inactive alone Theoretical model from PDB •Enzyme’s pocket is small 2I84
The NS3 protease
The NS3 protease •NS3 serine protease domain 20 kDa •catalytic residues His51, Asp75, Ser135
Background • Lin. C W et al,2007
Background • Ser to Ile60 were essential region required for NS3 46 protease activity. • Ala substition of Trp 50, Glu55, and Arg56 in NS2B shown significantly reduced NS3 protease activity. • Lin. C W et al,2007
Objective
Objective • to perform cloning of the NS2B-NS3 portion of the JEV polyprotein, express in E.coli and biochemically purify to determinants of clevage activity and cofactor requirement will be analyzed and compared to dengue virus. • The second objective is to study differences in substrate specificity and inhibitors by using peptide substrates incorporated with fluorogenic or chromogenic reported groups.
Method & Result pLS with NS2B-NS3 JEV
Method & Result pLS with NS2B-NS3 JEV NS2B(H) NS3p
Method & Result pLS with NS2B-NS3 JEV NS2B(H) NS3p SOE-PCR
Method & Result pLS with NS2B-NS3 JEV NS2B(H) NS3p SOE-PCR NS2B(H)-NS3p
NS2B(H) NS2B(H) Control NS3 protease NS3 protease NS3 protease Control 1500 1500 1000 900 800 1000 700 900 800 600 700 500 600 400 500 400 300 300 200 200 Figure 1 : The PCR product NS2B(H) JEV amplified from NS2B-NS3 Figure 2 : The PCR product NS3protease JEV amplified from NS2B- JEV (Lane 3 and 4). The size of NS2B(H) was 187 bp. NS3 JEV (Lane 3 to 5 ). The size of NS3 protease was 594 bp.
Control NS2B(H)-NS3p NS2B(H)-NS3p Control 1500 1000 900 1500 800 700 600 1000 900 500 800 400 700 600 300 500 400 200 300 100 Figure 4 : The NS2B(H)-NS3protease JEV (Lane 3 ) after digested with BamHI and KpnI. The size of NS2B(H)-NS3 protease was 765 bp. Figure 3 : The SOE-PCR product NS2B(H)-NS3protease JEV (Lane 2 to 5 ). The size of NS2B(H)-NS3 protease was 765 bp.
Method & Result
Method & Result NS2B(H)-NS3p JEV pTrcHis A Ligation & Transformation Site Screening & Digest with Restriction Enzyme
23.13 kb 2.03 kb 2.32 kb 4.56 kb 6.56 kb 9.42 kb pTrc plasmid Control Size Screening Clone 1 Clone 2 Clone 3 Clone 4 Clone 5 Clone 6 Clone 7 Clone 8 Clone 9 Clone 10 Clone 11 Clone 12 Clone 13 Clone 14 Clone 15 Clone 16 Clone 17
Digest with Restriction Enzyme clone 1 undigested clone 1 with BamHI,KpnI clone 1 with BamHI • Lane 1 : λ/BstII marker •Lane 2 : Clone 1 with BamHI and KpnI digerstion 8.454 kb 7.242 kb •Lane 3 : Clone 1 with BamHI digestion 6.369 kb 5.686 kb 4.822 kb 4.324 kb •Lane 4 : Clone 1 without digestion 3.645 kb 2.323 kb 1.929 kb 1.371 kb 1.264 kb 702 bp
Sequencing of candidate clone.
Deduced amino acid sequences of Japanese encephalitis virus NS2B(H) NS2B(H) C-terminal NS3p
Expression of Japanese encephalitis virus NS2B(H)/NS3 protease at different time. 0 Hr 1% 2 Hr 4 Hr 6 Hr incubate overnight O.D.= 0.4-0.6 8 Hr induction by IPTG
SDS-PAGE Analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at different time. marker ptrc 0- 8 Hr. NS2B(H)/NS3p 0- 8 Hr. 210 kD 125 kD 101 kD 56.2 kD 35.8 kD NS2B(H)/NS3 29 kD NS3 21 kD 6.9 kD NS2B(H)
Western blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at different time. marker NS2B(H)/NS3p 0- 8 Hr. 35.8 kD NS2B(H)/NS3 protease 29 kD 21 kD NS3 NS2B(H)
Expression of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different temperatures. 1% 18 ˚C 25 ˚C 37 ˚C incubate overnight O.D.= 0.4-0.6 induction by IPTG Incubate 8 Hrs.
SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different temperatures. pTrc 0 hr 37 ˚C JEV 37 ˚C JEV 18 ˚C JEV 30 ˚C pTrc 18 ˚C pTrc 25 ˚C pTrc 37 ˚C pTrc 30 ˚C JEV 25 ˚C marker 210 kD 125 kD 101 kD 56.2 kD 35.8 kD NS2B(H)/NS3 29 kD 21 kD NS3 protease 6.9 kD NS2B(H)
Western blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different temperatures. NS2B(H)/NS3p 37 ˚C NS2B(H)/NS3p 18 ˚C NS2B(H)/NS3p 30 ˚C NS2B(H)/NS3p 25 ˚C pTrc 0 hr 37 ˚C pTrc 18 ˚C pTrc 25 ˚C pTrc 37 ˚C pTrc 30 ˚C marker 101 kD 35.8 kD NS2B(H)/NS3 NS3 protease 21 kD NS2B(H) 6.9 kD
Expression of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different IPTG concentrations 0.1 mM 0.2 mM 1% 0.3 mM 0.4 mM 0.5 mM incubate overnight 0.6 mM 0.7 mM O.D.= 0.4-0.6 0.8 mM induction by IPTG Incubate 8 Hrs.
SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different IPTG concentrations. 0.1mM 0.8mM marker 210 kD 125 kD 101 kD 56.2 kD 35.8 kD NS2B(H)/NS3 29 kD NS3 protease 21 kD 6.9 kD NS2B(H)
Western blot analysis of Japaneseencephalitis virus NS2B(H)/NS3 protease expressed at different IPTG concentrations 0.1mM 0.8mM marker 35.8 kD NS2B(H)/NS3 protease 29 kD
Expression of Japanese encephalitis virus NS2B(H)/NS3 protease at small scale expression.
Expression of Japanese encephalitis virus NS2B(H)/NS3 protease at small scale expression. 1% Centrifuge, Lysis, Sonication and Collect incubate overnight fraction O.D.= 0.4-0.6 induction by o.1 mM IPTG Incubate 8 Hrs.
SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at small scale expression. marker C T I S 210 kD 125 kD 101 kD Lane 1: maker 56.2 kD NS2B(H)/NS3 protease Lane 2: Control pTrcHis Lane 3: Total fraction (T) 35.8 kD Lane 4: Insoluble fraction (I) Lane 5: Soluble fraction (S) 29 kD NS3 protease 21 kD NS2B(H) 6.9 kD
Western blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at small scale expression. T I S 35.8 kD NS2B(H)/NS3 protease Lane 1: maker Lane 2: Control pTrcHis Lane 3: Total fraction (T) Lane 4: Insoluble fraction (I) Lane 5: Soluble fraction (S)
SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at large scale expression. marker marker T I S TI S 210 kD 101 kD 125 kD 56.2 kD Lane 1: maker Lane 2: Total fraction (T) 35.8 kD NS2B(H)/NS3 protease Lane 3: Insoluble fraction (I) 29 kD Lane 4: Soluble fraction (S) NS3 protease 21 kD 6.9 kD NS2B(H)
Western blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at large scale expression. marker marker TI S T I S Lane 1: maker NS2B(H)/NS3 protease Lane 2: Total fraction (T) Lane 3: Insoluble fraction (I) Lane 4: Soluble fraction (S) NS3 protease NS2B(H)
Purification of the NS2B(H)/NS3p protein harboring the N-terminal polyhistidine tag The NS2B(H)/NS3 protease was purify by HiTrap Chelating column.
Method Soluble fraction in buffer H Wash with Buffer H (30 mM imidazole) Elute with Buffer H (100 mM imidazole)
SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease from Hi-trap purification. Elute and concentrate Washing fraction Soluble fraction fraction Flowtrough unduction induction marker 210 kD 125 kD 101 kD 56.2 kD NS2B(H)/NS3 protease 35.8 kD 29 kD NS3 protease 21 kD 6.9 kD
Western-blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease from Hi-trap column purification Elute and concentrate Washing fraction Soluble fraction fraction unduction Flowtrough induction marker NS2B(H)/NS3 35.8 kD 29 kD NS3 protease 21 kD NS2B(H) 6.9 kD
Characterize the activity of NS2B(H)/ NS3p JEV with Ac-RRRR-pNA The substrate Ac-RRRR-pNA is based on the para- nitroanilide principle the enzyme will cleave between the tetra arginine and release pNA Free pNA will be monitored at A405 by the spectrophotometry method. The change of pNA will change the color of buffer and correlate to the activity of the enzyme
Result Trypsin NS2B(H)/NS3p JEV substrate NS2B(H)/NS3p JEV = 10 μM trypsin = 0.4 μM substrate = 500 μM
Problem • The protein has by products from the purification step. • No activity • The fusion protein was different from the previous work of JEV.
The International Journal of Biochemistry & Cell Biology 39 (2007) 606–614
Method Soluble fraction in buffer A (50mM Hepes pH 7.0, 500mM NaCl) Wash with Buffer A (30 mM imidazole) Elute with Buffer A (100 mM imidazole)
Method The eluted protein (superdex 75 HR 10/300)
peak1 peak2
101 kD 210 kD 125 kD 6.9 kD 29 kD 21 kD 56.2 kD 35.8 kD Soluble Flowthrough wash Elute peak 1 peak2 result Soluble Flowthrough wash Elute peak 1 peak2
29 kD 21 kD 101 kD 210 kD 6.9 kD 125 kD 56.2 kD 35.8 kD uninduction induction Soluble Flowthrough wash Elute Gel filtration
29 kD 21 kD 101 kD 210 kD 6.9 kD 125 kD 56.2 kD 35.8 kD uninduction induction Soluble Flowthrough wash Elute Gel filtration
29 kD 21 kD 101 kD 210 kD 6.9 kD 125 kD 56.2 kD 35.8 kD induction Soluble Flowthrough wash Elute Gel filtration
29 kD 21 kD 101 kD 210 kD 6.9 kD 125 kD 56.2 kD 35.8 kD induction Soluble Flowthrough wash Elute Gel filtration
The substrate
The substrate
Protein assay method 7-Amino-4-Methyl Coumarin (AMC) standard curve • A serial dilution of AMC, from 3 μM - 50 μM, was prepared in 100 μl assay buffer (200 mM Tris-HCl pH. 9.5, 13.5 mM NaCl and 30% Glycerol). • incubated at 37 ํC for 30 minutes • Fluorescence signals were measured at an excitation wavelength 355 nm and emission 460 at 37 ํC nm. Fluorescence signals was plotted against AMC concentration
result Data 1 100000 Fluorescence unit 80000 Fluorecence units 60000 40000 20000 0 0 20 40 60 [AMC] (µM) The correlation between units with AMC concentrations was calculated from 1/ slope of linear regression. 1 fluorescence unit = 6.839 nM [AMC]
Protein assay method Enzyme Activity assay NS2B(H)-NS3p JEV protein 100 μl assay buffer (200 mM Tris-HCl pH. 9.5, 13.5 mM NaCl and 30% Glycerol) • incubated at 37 ํC for 30 minutes adding 200 μM of Pyr-RTKR-AMC substrate • Fluorescence signals were measured at an excitation wavelength 355 nm and emission 460 at 37 ํC nm and monitored every 3 minutes for 2 hr.
result Data 1 30000 Control 200 mM Fluorescence unit 20000 10000 0 0 50 100 150 time Progress curves for enzymes-catalyzed hydrolysis observed at 200 μM of Pyr-RTKR-AMC were plotted between fluorescence signals against time
Protein assay method Determination of kinetic parameters NS2B(H)-NS3p JEV protein 100 μl assay buffer (200 mM Tris-HCl pH. 9.5, 13.5 mM NaCl and 30% Glycerol) • incubated at 37 ํC for 30 minutes Pyr-RTKR-AMC was varied the concentrations from 15 μM to 500 μM • Fluorescence signals were measured at an excitation wavelength 355 nm and emission 460 at 37 ํC nm and monitored for 2 hr.
result Data 1 2000 1500 Velocity (nM/min) 1000 500 0 0 200 400 600 [Pyr-RTKR-AMC] (µM) Vmax (nM/min) Km (µM) Kcat (s-1) Kcat/ Km(M-1s-1) 2672 226.4 3.22 0.014
What’s next? • Try to improve purification and find the amount of active protein • compare to Den NS2B(H)-NS3p

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Evaluation 3

  • 1. Cloning, Expression, Purification and Enzymological Characterization of NS2B/NS3 Protease / RNA Helicase protein of Japanese Encephalitis Virus. Chakard Chalayut Advisor: Asst. Prof. Gerd Katzenmeier, Ph.D. Laboratory of Molecular Virology Institute of Molecular Biology & Genetics
  • 2. Japanese Encephalitis Virus (JEV) -Flaviviridae family -Mosquito-borne neurotropic flavivirus •causes severe central nerve system diseases
  • 3. Japanese Encephalitis Virus (JEV) Culex tritaeniorhynchus. Source: fehd.gov.hk
  • 5. Japanese Encephalitis Virus (JEV) Source : vietnammedicalpractice.com
  • 7. Japanese Encephalitis Virus (JEV) JEV causes severe central nerve system diseases such as p o l i o mye l i t i s - l i ke acute flaccid paralysis, aseptic meningitis and encephalitis Source:wonder.cdc.gov
  • 10. Japanese Encephalitis Virus (JEV) 50,000 Cases
  • 11. Japanese Encephalitis Virus (JEV) 30% fatality rate
  • 12. Japanese Encephalitis Virus (JEV) 10,000 Cases
  • 14. Prevention and treatment of JEV disease Drug No drug exist
  • 15. Prevention and treatment of JEV disease Drug No drug exist Vaccine development Available vaccine
  • 16. Prevention and treatment of JEV disease Drug No drug exist Vaccine development Available vaccine Elimination of mosquitoes Mosquitoes control breeding places
  • 17. Molecular biology of Japanese Encephalitis Virus
  • 18. The NS2B • 130 aa • activating domain central hydrophilic region (Falgout et al, 1993) • 3 membrane spanning parts
  • 19. The NS2B • 130 aa • activating domain central hydrophilic region (Falgout et al, 1993) • 3 membrane spanning parts hydrophobicity plot
  • 20. The NS2B • 130 aa • activating domain central hydrophilic region (Falgout et al, 1993) • 3 membrane spanning parts hydrophobicity plot 51 DMWLERAADISWEMDAAITGSSRRLDVKLDDDGDFHLIDDPGVP 95
  • 21. The NS2B • 130 aa Hypothetical model • activating domain NS2B-NS3 complex central hydrophilic region (Falgout et al, 1993) • 3 membrane spanning parts hydrophobicity plot ฺBrinkworth et al, 1999 51 DMWLERAADISWEMDAAITGSSRRLDVKLDDDGDFHLIDDPGVP 95
  • 22. The NS3 Theoretical model from PDB 2I84
  • 23. The NS3 Protease Theoretical model from PDB 2I84
  • 24. The NS3 Protease NTPase RNA Helicase Theoretical model from PDB 2I84
  • 25. The NS3 •Chymotrypsin-like fold 2-β barrel domains •Inactive alone Theoretical model from PDB •Enzyme’s pocket is small 2I84
  • 27. The NS3 protease •NS3 serine protease domain 20 kDa •catalytic residues His51, Asp75, Ser135
  • 28. Background • Lin. C W et al,2007
  • 29. Background • Ser to Ile60 were essential region required for NS3 46 protease activity. • Ala substition of Trp 50, Glu55, and Arg56 in NS2B shown significantly reduced NS3 protease activity. • Lin. C W et al,2007
  • 31. Objective • to perform cloning of the NS2B-NS3 portion of the JEV polyprotein, express in E.coli and biochemically purify to determinants of clevage activity and cofactor requirement will be analyzed and compared to dengue virus. • The second objective is to study differences in substrate specificity and inhibitors by using peptide substrates incorporated with fluorogenic or chromogenic reported groups.
  • 32. Method & Result pLS with NS2B-NS3 JEV
  • 33. Method & Result pLS with NS2B-NS3 JEV NS2B(H) NS3p
  • 34. Method & Result pLS with NS2B-NS3 JEV NS2B(H) NS3p SOE-PCR
  • 35. Method & Result pLS with NS2B-NS3 JEV NS2B(H) NS3p SOE-PCR NS2B(H)-NS3p
  • 36. NS2B(H) NS2B(H) Control NS3 protease NS3 protease NS3 protease Control 1500 1500 1000 900 800 1000 700 900 800 600 700 500 600 400 500 400 300 300 200 200 Figure 1 : The PCR product NS2B(H) JEV amplified from NS2B-NS3 Figure 2 : The PCR product NS3protease JEV amplified from NS2B- JEV (Lane 3 and 4). The size of NS2B(H) was 187 bp. NS3 JEV (Lane 3 to 5 ). The size of NS3 protease was 594 bp.
  • 37. Control NS2B(H)-NS3p NS2B(H)-NS3p Control 1500 1000 900 1500 800 700 600 1000 900 500 800 400 700 600 300 500 400 200 300 100 Figure 4 : The NS2B(H)-NS3protease JEV (Lane 3 ) after digested with BamHI and KpnI. The size of NS2B(H)-NS3 protease was 765 bp. Figure 3 : The SOE-PCR product NS2B(H)-NS3protease JEV (Lane 2 to 5 ). The size of NS2B(H)-NS3 protease was 765 bp.
  • 39. Method & Result NS2B(H)-NS3p JEV pTrcHis A Ligation & Transformation Site Screening & Digest with Restriction Enzyme
  • 40. 23.13 kb 2.03 kb 2.32 kb 4.56 kb 6.56 kb 9.42 kb pTrc plasmid Control Size Screening Clone 1 Clone 2 Clone 3 Clone 4 Clone 5 Clone 6 Clone 7 Clone 8 Clone 9 Clone 10 Clone 11 Clone 12 Clone 13 Clone 14 Clone 15 Clone 16 Clone 17
  • 41. Digest with Restriction Enzyme clone 1 undigested clone 1 with BamHI,KpnI clone 1 with BamHI • Lane 1 : λ/BstII marker •Lane 2 : Clone 1 with BamHI and KpnI digerstion 8.454 kb 7.242 kb •Lane 3 : Clone 1 with BamHI digestion 6.369 kb 5.686 kb 4.822 kb 4.324 kb •Lane 4 : Clone 1 without digestion 3.645 kb 2.323 kb 1.929 kb 1.371 kb 1.264 kb 702 bp
  • 43. Deduced amino acid sequences of Japanese encephalitis virus NS2B(H) NS2B(H) C-terminal NS3p
  • 44. Expression of Japanese encephalitis virus NS2B(H)/NS3 protease at different time. 0 Hr 1% 2 Hr 4 Hr 6 Hr incubate overnight O.D.= 0.4-0.6 8 Hr induction by IPTG
  • 45. SDS-PAGE Analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at different time. marker ptrc 0- 8 Hr. NS2B(H)/NS3p 0- 8 Hr. 210 kD 125 kD 101 kD 56.2 kD 35.8 kD NS2B(H)/NS3 29 kD NS3 21 kD 6.9 kD NS2B(H)
  • 46. Western blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at different time. marker NS2B(H)/NS3p 0- 8 Hr. 35.8 kD NS2B(H)/NS3 protease 29 kD 21 kD NS3 NS2B(H)
  • 47. Expression of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different temperatures. 1% 18 ˚C 25 ˚C 37 ˚C incubate overnight O.D.= 0.4-0.6 induction by IPTG Incubate 8 Hrs.
  • 48. SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different temperatures. pTrc 0 hr 37 ˚C JEV 37 ˚C JEV 18 ˚C JEV 30 ˚C pTrc 18 ˚C pTrc 25 ˚C pTrc 37 ˚C pTrc 30 ˚C JEV 25 ˚C marker 210 kD 125 kD 101 kD 56.2 kD 35.8 kD NS2B(H)/NS3 29 kD 21 kD NS3 protease 6.9 kD NS2B(H)
  • 49. Western blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different temperatures. NS2B(H)/NS3p 37 ˚C NS2B(H)/NS3p 18 ˚C NS2B(H)/NS3p 30 ˚C NS2B(H)/NS3p 25 ˚C pTrc 0 hr 37 ˚C pTrc 18 ˚C pTrc 25 ˚C pTrc 37 ˚C pTrc 30 ˚C marker 101 kD 35.8 kD NS2B(H)/NS3 NS3 protease 21 kD NS2B(H) 6.9 kD
  • 50. Expression of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different IPTG concentrations 0.1 mM 0.2 mM 1% 0.3 mM 0.4 mM 0.5 mM incubate overnight 0.6 mM 0.7 mM O.D.= 0.4-0.6 0.8 mM induction by IPTG Incubate 8 Hrs.
  • 51. SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease expressed at different IPTG concentrations. 0.1mM 0.8mM marker 210 kD 125 kD 101 kD 56.2 kD 35.8 kD NS2B(H)/NS3 29 kD NS3 protease 21 kD 6.9 kD NS2B(H)
  • 52. Western blot analysis of Japaneseencephalitis virus NS2B(H)/NS3 protease expressed at different IPTG concentrations 0.1mM 0.8mM marker 35.8 kD NS2B(H)/NS3 protease 29 kD
  • 53.
  • 54. Expression of Japanese encephalitis virus NS2B(H)/NS3 protease at small scale expression.
  • 55. Expression of Japanese encephalitis virus NS2B(H)/NS3 protease at small scale expression. 1% Centrifuge, Lysis, Sonication and Collect incubate overnight fraction O.D.= 0.4-0.6 induction by o.1 mM IPTG Incubate 8 Hrs.
  • 56. SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at small scale expression. marker C T I S 210 kD 125 kD 101 kD Lane 1: maker 56.2 kD NS2B(H)/NS3 protease Lane 2: Control pTrcHis Lane 3: Total fraction (T) 35.8 kD Lane 4: Insoluble fraction (I) Lane 5: Soluble fraction (S) 29 kD NS3 protease 21 kD NS2B(H) 6.9 kD
  • 57. Western blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at small scale expression. T I S 35.8 kD NS2B(H)/NS3 protease Lane 1: maker Lane 2: Control pTrcHis Lane 3: Total fraction (T) Lane 4: Insoluble fraction (I) Lane 5: Soluble fraction (S)
  • 58. SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at large scale expression. marker marker T I S TI S 210 kD 101 kD 125 kD 56.2 kD Lane 1: maker Lane 2: Total fraction (T) 35.8 kD NS2B(H)/NS3 protease Lane 3: Insoluble fraction (I) 29 kD Lane 4: Soluble fraction (S) NS3 protease 21 kD 6.9 kD NS2B(H)
  • 59. Western blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease at large scale expression. marker marker TI S T I S Lane 1: maker NS2B(H)/NS3 protease Lane 2: Total fraction (T) Lane 3: Insoluble fraction (I) Lane 4: Soluble fraction (S) NS3 protease NS2B(H)
  • 60. Purification of the NS2B(H)/NS3p protein harboring the N-terminal polyhistidine tag The NS2B(H)/NS3 protease was purify by HiTrap Chelating column.
  • 61. Method Soluble fraction in buffer H Wash with Buffer H (30 mM imidazole) Elute with Buffer H (100 mM imidazole)
  • 62. SDS-PAGE analysis of Japanese encephalitis virus NS2B(H)/NS3 protease from Hi-trap purification. Elute and concentrate Washing fraction Soluble fraction fraction Flowtrough unduction induction marker 210 kD 125 kD 101 kD 56.2 kD NS2B(H)/NS3 protease 35.8 kD 29 kD NS3 protease 21 kD 6.9 kD
  • 63. Western-blot analysis of Japanese encephalitis virus NS2B(H)/NS3 protease from Hi-trap column purification Elute and concentrate Washing fraction Soluble fraction fraction unduction Flowtrough induction marker NS2B(H)/NS3 35.8 kD 29 kD NS3 protease 21 kD NS2B(H) 6.9 kD
  • 64. Characterize the activity of NS2B(H)/ NS3p JEV with Ac-RRRR-pNA The substrate Ac-RRRR-pNA is based on the para- nitroanilide principle the enzyme will cleave between the tetra arginine and release pNA Free pNA will be monitored at A405 by the spectrophotometry method. The change of pNA will change the color of buffer and correlate to the activity of the enzyme
  • 65. Result Trypsin NS2B(H)/NS3p JEV substrate NS2B(H)/NS3p JEV = 10 μM trypsin = 0.4 μM substrate = 500 μM
  • 66. Problem • The protein has by products from the purification step. • No activity • The fusion protein was different from the previous work of JEV.
  • 67. The International Journal of Biochemistry & Cell Biology 39 (2007) 606–614
  • 68. Method Soluble fraction in buffer A (50mM Hepes pH 7.0, 500mM NaCl) Wash with Buffer A (30 mM imidazole) Elute with Buffer A (100 mM imidazole)
  • 69. Method The eluted protein (superdex 75 HR 10/300)
  • 71. 101 kD 210 kD 125 kD 6.9 kD 29 kD 21 kD 56.2 kD 35.8 kD Soluble Flowthrough wash Elute peak 1 peak2 result Soluble Flowthrough wash Elute peak 1 peak2
  • 72.
  • 73. 29 kD 21 kD 101 kD 210 kD 6.9 kD 125 kD 56.2 kD 35.8 kD uninduction induction Soluble Flowthrough wash Elute Gel filtration
  • 74. 29 kD 21 kD 101 kD 210 kD 6.9 kD 125 kD 56.2 kD 35.8 kD uninduction induction Soluble Flowthrough wash Elute Gel filtration
  • 75. 29 kD 21 kD 101 kD 210 kD 6.9 kD 125 kD 56.2 kD 35.8 kD induction Soluble Flowthrough wash Elute Gel filtration
  • 76. 29 kD 21 kD 101 kD 210 kD 6.9 kD 125 kD 56.2 kD 35.8 kD induction Soluble Flowthrough wash Elute Gel filtration
  • 79. Protein assay method 7-Amino-4-Methyl Coumarin (AMC) standard curve • A serial dilution of AMC, from 3 μM - 50 μM, was prepared in 100 μl assay buffer (200 mM Tris-HCl pH. 9.5, 13.5 mM NaCl and 30% Glycerol). • incubated at 37 ํC for 30 minutes • Fluorescence signals were measured at an excitation wavelength 355 nm and emission 460 at 37 ํC nm. Fluorescence signals was plotted against AMC concentration
  • 80. result Data 1 100000 Fluorescence unit 80000 Fluorecence units 60000 40000 20000 0 0 20 40 60 [AMC] (µM) The correlation between units with AMC concentrations was calculated from 1/ slope of linear regression. 1 fluorescence unit = 6.839 nM [AMC]
  • 81. Protein assay method Enzyme Activity assay NS2B(H)-NS3p JEV protein 100 μl assay buffer (200 mM Tris-HCl pH. 9.5, 13.5 mM NaCl and 30% Glycerol) • incubated at 37 ํC for 30 minutes adding 200 μM of Pyr-RTKR-AMC substrate • Fluorescence signals were measured at an excitation wavelength 355 nm and emission 460 at 37 ํC nm and monitored every 3 minutes for 2 hr.
  • 82. result Data 1 30000 Control 200 mM Fluorescence unit 20000 10000 0 0 50 100 150 time Progress curves for enzymes-catalyzed hydrolysis observed at 200 μM of Pyr-RTKR-AMC were plotted between fluorescence signals against time
  • 83. Protein assay method Determination of kinetic parameters NS2B(H)-NS3p JEV protein 100 μl assay buffer (200 mM Tris-HCl pH. 9.5, 13.5 mM NaCl and 30% Glycerol) • incubated at 37 ํC for 30 minutes Pyr-RTKR-AMC was varied the concentrations from 15 μM to 500 μM • Fluorescence signals were measured at an excitation wavelength 355 nm and emission 460 at 37 ํC nm and monitored for 2 hr.
  • 84. result Data 1 2000 1500 Velocity (nM/min) 1000 500 0 0 200 400 600 [Pyr-RTKR-AMC] (µM) Vmax (nM/min) Km (µM) Kcat (s-1) Kcat/ Km(M-1s-1) 2672 226.4 3.22 0.014
  • 85. What’s next? • Try to improve purification and find the amount of active protein • compare to Den NS2B(H)-NS3p