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Line 448: |
Line 448: |
| * adjust glgCAB in ∆glgP BL21 Gold (DE3) clones #4+7 and ∆glgP BL21 Gold (DE3) to the same OD of 1.97 | | * adjust glgCAB in ∆glgP BL21 Gold (DE3) clones #4+7 and ∆glgP BL21 Gold (DE3) to the same OD of 1.97 |
| * freeze pellet for iodine staining | | * freeze pellet for iodine staining |
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− | ==NEXT==
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− | * for iodine staining:
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− | ** overnights of BL21 glgAB in C30 (sequencing confirmed clones), BL21 glgA, BL21 glgB and BL21 WT
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− | ** 5 ml LB medium and 5 ml LB + 20 mM Glucose
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− | * '''growth experiment with XULU in ΔglgP BL21'''
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− | ** inoculate precultures of BL21 XULU in ΔglgP and ΔglgP
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− | ** inoculate three 25 ml LB main cultures
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− | *** LB + MeOH BL21 XULU in ΔglgP
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− | *** LB - MeOH BL21 XULU in ΔglgP
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− | *** LB + MeOH BL21 ΔglgP
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− | * '''feed glycogen-producing cells to WT'''
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− | ** inoculated 2 BL21 wild type LB precultures (5 ml LB) at 1:20 pm
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− | **inoculate two 10 ml M9 cultures of WT over night
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− | **inoculate one 10 ml LB + 20mM glucose overnight culture of WT and one of glgCAB
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− | ** adjust LB WT and the CAB cultures to same OD
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− | ** centrifuge, resolve in water and boil for 10 minutes at 95 °C
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− | ** inoculate three 25 ml M9 C-limited cultures of WT
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− | ***3.3 mM glucose, 18.7 mM NH4Cl
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− | ** feed the boiled WT to one culture and the CAB mixture to the other
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− | ** measure growth in Aquila System
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