Difference between revisions of "Team:Uppsala/Phage Display"

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Phage titering is done after every affinity screening to assess the amount of phages that bind to the target. By following the titering protocol consisting of plating phages together with mid-log phase bacteria visible blue plaques are formed on Xgal/IPTG plates. Xgal is a substrate for the enzyme β-galactosidase, which hydrolyzes the compound into a form that spontaneously dimerizes into an insoluble blue pigment. Our cell strain can only express the enzyme after phage infection and induction by IPTG. This makes it simple to distinguish infected from non infected colonies since only the infected ones will appear blue.  
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Phage titering is done after every affinity screening to assess the amount of phages that bind to the target. By following the titering protocol consisting of plating phages together with mid-log phase bacteria visible blue plaques are formed on Xgal/IPTG plates.
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Xgal is a substrate for the enzyme β-galactosidase, which hydrolyzes the compound into a form that spontaneously dimerizes into an insoluble blue pigment. Our cell strain can only express the enzyme after phage infection and induction by IPTG. This makes it simple to distinguish infected from non infected colonies since only the infected ones will appear blue.  
 
The goal with plating is to achieve plates with around 100 plaques, which is fulfilled by doing several dilution series of the infected bacteria. The reason for this is that plaques will only increase linearly with added phages when the multiplicity of infection (MOI) is much less than 1. Also low MOI result in one DNA sequence per plaque. To asses the titre, plaque forming unit (pfu) can be calculated by multiple numbers of plaques with the bacteria dilution.  
 
The goal with plating is to achieve plates with around 100 plaques, which is fulfilled by doing several dilution series of the infected bacteria. The reason for this is that plaques will only increase linearly with added phages when the multiplicity of infection (MOI) is much less than 1. Also low MOI result in one DNA sequence per plaque. To asses the titre, plaque forming unit (pfu) can be calculated by multiple numbers of plaques with the bacteria dilution.  
 
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Revision as of 20:42, 17 October 2018