Team:USTC CHINA/Notebook/Protocols/Expression of proteins in Escherichia coli

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<h1>Expression of proteins in Escherichia coli</h1>
<h1>Expression of proteins in Escherichia coli</h1>
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<p>Protocol:The induction expression isolation and purification of protein in E.coli-BL21
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LB medium (1L)                            Binding buffer(1L)                    Elution Buffer(1L)
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Tryptone            10g                  Tris              20mM            Add 500mM iminazole to binding
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Yeast extract          5g Sodium chloride    500mM            buffer
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Sodium chloride        5g                  Add HCl or NaOH until the pH is 8.0
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experimental procedure:
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1.Add 100~200 uL E.coli Bl21 storing in -40℃ 50mL LB medium which has been added 5mg ampicillin and culture the bacterial 12hours in a 37℃ Incubator shaker.
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2.Add all the 50ml LB medium to an 1L LB medium which has been added 100mg ampicillin and culture the bacterial in a 16℃ incubator shaker until the OD is between 1.0 and 1.2..
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3.Add 3300mM IPTG into the medium and culture the bacterial for 20 to 24 hours.
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4.Bacteria Collection:Dispense all the bacterial suspension into several 500mL centrifuge bottles and ensure that the error does not exceed 0.1g.Centrifuge under these conditions:The speed is 6000rpm/min,the time is 10 minutes and the temperature is 4℃ and discard the supernatant.
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5.Resuspend The bacteria in the centrifuge bottles with 40mL binding buffer and transfer the bacterial suspension to an 80ml beaker for ultrasonic disruption under these conditions:The power is 40%,the total working time is 20min and the on time is 2s while the off time is 4s.
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6.Dispense the bacterial suspension into two 500mL centrifuge bottles and ensure that the error does not exceed 0.1g.Centrifuge under these conditions:The speed is 13000rpm/min,the time is 30 minutes and the temperature is 4℃.
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7.Purify the protein through nickel-affinity chromatography column.
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Revision as of 14:13, 25 September 2013

Expression of proteins in Escherichia coli

Protocol:The induction expression isolation and purification of protein in E.coli-BL21 LB medium (1L) Binding buffer(1L) Elution Buffer(1L) Tryptone 10g Tris 20mM Add 500mM iminazole to binding Yeast extract 5g Sodium chloride 500mM buffer Sodium chloride 5g Add HCl or NaOH until the pH is 8.0 experimental procedure: 1.Add 100~200 uL E.coli Bl21 storing in -40℃ 50mL LB medium which has been added 5mg ampicillin and culture the bacterial 12hours in a 37℃ Incubator shaker. 2.Add all the 50ml LB medium to an 1L LB medium which has been added 100mg ampicillin and culture the bacterial in a 16℃ incubator shaker until the OD is between 1.0 and 1.2.. 3.Add 3300mM IPTG into the medium and culture the bacterial for 20 to 24 hours. 4.Bacteria Collection:Dispense all the bacterial suspension into several 500mL centrifuge bottles and ensure that the error does not exceed 0.1g.Centrifuge under these conditions:The speed is 6000rpm/min,the time is 10 minutes and the temperature is 4℃ and discard the supernatant. 5.Resuspend The bacteria in the centrifuge bottles with 40mL binding buffer and transfer the bacterial suspension to an 80ml beaker for ultrasonic disruption under these conditions:The power is 40%,the total working time is 20min and the on time is 2s while the off time is 4s. 6.Dispense the bacterial suspension into two 500mL centrifuge bottles and ensure that the error does not exceed 0.1g.Centrifuge under these conditions:The speed is 13000rpm/min,the time is 30 minutes and the temperature is 4℃. 7.Purify the protein through nickel-affinity chromatography column.