Team:MIT/Tooth binding assay protocol

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(Tooth binding assay)
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• Wash 50 mg HA beads 3 times with 1mM phosphate buffer (PB) and equilibrate in PB for 2 hours
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• Wash 50 mg HA beads 3 times with 1mM phosphate buffer (PB) and equilibrate in PB for 2 hours (or overnight)
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• HA beads settle for 30 to 60 s, then remove supernatant
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• HA beads added to 500 microL saliva and stir suspension for 1h at 37 C
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• '''Control'''
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        Aspirate saliva and wash s. mutans with 10x PBS
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        Dilute bacteria with 1x PBS to get the final concentration of 1-2 *10^7 CFU (.075 to .16 OD)
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      o   add 1mM phosphate-phosphate buffered saline (PBS) for 1h
 
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      o   wash with 10mM PBS
 
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      o   add saliva for 1h
 
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      o   wash with 10mM PBS
 
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• '''Variable'''
 
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      o   Add saliva (amount?) for 1h
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Add 1mL S. Mutans suspension to HA beads, incubate at 37 C at 20 rpm in microfuge tubes
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      o   Wash with 10mM PBS
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      o   Add p1025 (amount?) extract
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      o   Wash with 10mM PBS
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• Add 1mL S. Mutans suspension (1-2*10^7 colony-forming units (CFU))
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• Extract 100 μL supernatant after 5 minutes and spot onto plates (10g agar, 15g THB, 500 mL H20)
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• Extract 100 μL supernatant after 5 minutes and plate onto Todd Hewitt Broth (THB), or whatever media the S. Mutans comes in
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• Repeat above after 1h, 2h
• Repeat above after 1h, 2h
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PBS—naCL 8.0 g L-1, KCl 2.0 g L-1, Na2HPO4, 2H20 2.0 g L-1, KH2PO4 2.0 g L-1; pH 7.2
PBS—naCL 8.0 g L-1, KCl 2.0 g L-1, Na2HPO4, 2H20 2.0 g L-1, KH2PO4 2.0 g L-1; pH 7.2
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OD-CFU conversion factor: optical density at 600 nm of 0.75 to 0.8: 1 × 108 CFU/ml)
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Revision as of 15:38, 27 June 2008


Home The Team The Project Parts Submitted to the Registry Modeling Notebook


Tooth binding assay

• Wash 50 mg HA beads 3 times with 1mM phosphate buffer (PB) and equilibrate in PB for 2 hours (or overnight)

• HA beads added to 500 microL saliva and stir suspension for 1h at 37 C 

       Aspirate saliva and wash s. mutans with 10x PBS
       
       Dilute bacteria with 1x PBS to get the final concentration of 1-2 *10^7 CFU (.075 to .16 OD)


• Add 1mL S. Mutans suspension to HA beads, incubate at 37 C at 20 rpm in microfuge tubes

• Extract 100 μL supernatant after 5 minutes and spot onto plates (10g agar, 15g THB, 500 mL H20)

• Repeat above after 1h, 2h

• Count colonies (approximately CFUs) on the three plates and calculate the amount attached to HA beads through the relation “CFU supernatant time 0 – CFU supernatant time 1h, 2h = CFU on HA beads"

PBS—naCL 8.0 g L-1, KCl 2.0 g L-1, Na2HPO4, 2H20 2.0 g L-1, KH2PO4 2.0 g L-1; pH 7.2

OD-CFU conversion factor: optical density at 600 nm of 0.75 to 0.8: 1 × 108 CFU/ml)




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