Difference between revisions of "Team:Aachen/Notebook/Documentation/Glycogen Characterization"
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** series looks good, will be done with glycogen solutions tommorow | ** series looks good, will be done with glycogen solutions tommorow | ||
* cryo cultures of #XULU# in BL21 Gold ΔglgP: #NKKA# #E4QF# #YNAZ# #R8LW# #B8FD# | * cryo cultures of #XULU# in BL21 Gold ΔglgP: #NKKA# #E4QF# #YNAZ# #R8LW# #B8FD# | ||
+ | |||
+ | * Dinitrosalicylic acid staining (OD of WT, ΔglgX and ΔglgP were adjusted) | ||
+ | * 1:100, 1:50, 1:25, 1:12.5, 1:6.25, 1:3.125, and 1:1.5625 dilutions of WT, ΔglgP, and ΔglgX were prepared; 50 µL sample volume. The same volume of Dinitrosalicylic acid was added; total volume was 100 µL. | ||
+ | * blank: 1:1 dilution of dinitrosalicylic acid in water. | ||
+ | * the stained samples were heated for 10 minutes at 90 °C | ||
+ | * the heated samples were cooled down in a 25 °C heater | ||
+ | * samples were analyzed in plate reader at 540 nm | ||
==15-09-09== | ==15-09-09== | ||
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** '''End OD values:''' WT 8.9 CAB 17 C 10.6 A 12,8 deltaX 7.2 deltaP 7.3 | ** '''End OD values:''' WT 8.9 CAB 17 C 10.6 A 12,8 deltaX 7.2 deltaP 7.3 | ||
*10 HPLC samples (of glgB, glgA, WT, ΔglgP, ΔglgX from the 7th September) were given to Philipp: the dried samples were resuspend in 1mL water, centrifuged and filtered. Each in a 1:1 dilution and undiluted. | *10 HPLC samples (of glgB, glgA, WT, ΔglgP, ΔglgX from the 7th September) were given to Philipp: the dried samples were resuspend in 1mL water, centrifuged and filtered. Each in a 1:1 dilution and undiluted. | ||
+ | |||
+ | * Dinitrosalicylic acid staining (OD of WT, ΔglgX and ΔglgP were adjusted) | ||
+ | * 1:100, 1:50, 1:25, 1:12.5, 1:6.25, 1:3.125, and 1:1.5625 dilutions of WT, ΔglgP, and ΔglgX were prepared; 50 µL sample volume. The same volume of Dinitrosalicylic acid was added; total volume was 100 µL. | ||
+ | * blank: 1:1 dilution of dinitrosalicylic acid in water. | ||
+ | * the stained samples were heated for 10 minutes at 90 °C | ||
+ | * the heated samples were cooled down in a 25 °C heater | ||
+ | * samples were analyzed in plate reader at 540 nm | ||
==15-09-11== | ==15-09-11== | ||
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* boiling might not have disrupted the glycogen chains, therefore, cells might not be able to metabolize the feed | * boiling might not have disrupted the glycogen chains, therefore, cells might not be able to metabolize the feed | ||
* experiment should work if the feed is treated with HCl for acid hydrolysis first | * experiment should work if the feed is treated with HCl for acid hydrolysis first | ||
+ | |||
+ | * Dinitrosalicylic acid staining (OD of WT, ΔglgX and ΔglgP were adjusted) | ||
+ | * 1:100, 1:50, 1:25, 1:12.5, 1:6.25, 1:3.125, and 1:1.5625 dilutions of WT, ΔglgP, and ΔglgX were prepared; 50 µL sample volume. The same volume of Dinitrosalicylic acid was added; total volume was 100 µL. | ||
+ | * blank: 1:1 dilution of dinitrosalicylic acid in water. | ||
+ | * the stained samples were heated for 10 minutes at 90 °C | ||
+ | * the heated samples were cooled down in a 25 °C heater | ||
+ | * samples were analyzed in plate reader at 540 nm | ||
==15-09-13== | ==15-09-13== | ||
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* two 10 ml LB overnight cultures of #E4QF# were inoculated | * two 10 ml LB overnight cultures of #E4QF# were inoculated | ||
* no difference in growth or glycogen production could be observed | * no difference in growth or glycogen production could be observed | ||
+ | |||
+ | * Dinitrosalicylic acid staining | ||
+ | ** two replicates of 5 mL LB overnight cultures of WT and ''glgB'' were prepared | ||
==15-09-14== | ==15-09-14== | ||
* End-OD(1)=8,4 End-OD(2)=7,7 End-OD(3)=7,4 (cultures from yesterday) | * End-OD(1)=8,4 End-OD(2)=7,7 End-OD(3)=7,4 (cultures from yesterday) | ||
* main cultures inoculated at 9:25 am to OD 0.3 in M9 (C-limited, 3.3 mM Glucose) + K | * main cultures inoculated at 9:25 am to OD 0.3 in M9 (C-limited, 3.3 mM Glucose) + K | ||
− | + | ** cultures 1-3: POLY in ΔglgP + MeOH | |
+ | ** cultures 4-6: POLY in ΔglgP - MeOH | ||
{| class = "wikitable" | {| class = "wikitable" | ||
! time !! OD culture 1 !! OD 2 !! OD 3 !! OD 4 !! OD 5 !! OD 6 | ! time !! OD culture 1 !! OD 2 !! OD 3 !! OD 4 !! OD 5 !! OD 6 | ||
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**to 22 ml culture volume, 465 µl methanol were added: MeOH concentration of 0.522 M (first thougt the end culture volume would be 23 ml while induction) | **to 22 ml culture volume, 465 µl methanol were added: MeOH concentration of 0.522 M (first thougt the end culture volume would be 23 ml while induction) | ||
**MeOh was added at t: 5 (OD 0.769 - 0.802) at 3:15 p.m. | **MeOh was added at t: 5 (OD 0.769 - 0.802) at 3:15 p.m. | ||
+ | * no influence of MeOH could be observed | ||
+ | * Dinitrosalicylic acid staining | ||
+ | ** 3 biological replicates of ''glg B'' strain and wild type were prepared by transferring 2 mL of LB overnight cultures to M9 Nitrogen limitation media. The calculated starting OD was 0.1. | ||
+ | |||
+ | ==15-09-15== | ||
+ | * Dinitrosalicylic acid staining | ||
+ | ** M9 N-limitation cultures were [[Team:Aachen/Notebook/Protocols#Glycogen_Kit| purified via Glycogen_Kit]] section ''Pre-extraction of glycogen'' | ||
==15-09-16== | ==15-09-16== | ||
*cryos of glgCAB in pSB1A30 in ∆glgP (Bl21 Gold DE3) clones #4 (#LOVE#) and #7 (#TEND#) | *cryos of glgCAB in pSB1A30 in ∆glgP (Bl21 Gold DE3) clones #4 (#LOVE#) and #7 (#TEND#) | ||
− | * | + | * make LB + 20 mM glucose + IPTG overnight cultures of glgCAB in ∆glgP BL21 Gold (DE3) clone #4 and ∆glgP BL21 Gold (DE3) |
==15-09-17== | ==15-09-17== | ||
− | * adjust glgCAB in ∆glgP BL21 Gold (DE3) | + | * adjust glgCAB in ∆glgP BL21 Gold (DE3) clone #4 and ∆glgP BL21 Gold (DE3) to the same OD of 1.97 |
* freeze pellet for iodine staining | * freeze pellet for iodine staining | ||
+ | * *overdays (LB+Antibiotic+IPTG+20 mM glucose) of glgAB in pSB1C30 (#8ZZ4# and #N96D#), glgA in pSB1K30, glgB in pSB1K30 and BL21 WT (incubation since 10 am) | ||
+ | * do iodine staining of all cultures in the evening | ||
+ | ** glgCAB in ∆glgP BL21 Gold (DE3) clone #4 was stained darker than the ∆glgP BL21 Gold (DE3) culture | ||
+ | ** therefore, the combination of the knockoutof glgP and the overexpression of glgCAB leads to higher glycogen production | ||
+ | ** for glgAB, no remarkably darker color was observed | ||
− | = | + | {{Team:Aachen/Figure|Aachen_15-09-17 deltaP +glgCAB vs deltaP.jpg|title=Iodine staining BL21 Gold (DE3) ΔglgP + glgCAB vs. BL21 Gold (DE3) ΔglgP|subtitle=Cultivated in LB+20mM glucose, BL21 Gold (DE3) ΔglgP + glgCAB stained distinctly darker than BL21 Gold (DE3) ΔglgP. It shows that even higher glycogen accumulation can be achieved by combining overexpression of all three synthesis enzymes and the ΔglgP knockout.|size=medium}} |
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+ | * do 10 ml LB + 20 mM glucose + IPTG of BL21 Gold (DE3) glgA, glgB, glgC, glgCAB, ∆glgP, ∆glgX, ∆glgP + glgCAB | ||
+ | * Dinitrosalicylic acid staining | ||
+ | ** dried pellets of the replicates of ''glg B'' and wild type were resuspended in 1 mL water | ||
+ | ** samples were splited into two 500 µL samples | ||
+ | ** [[Team:Aachen/Notebook/Protocols#Dinitrosalicylic_Acid_Staining| staining protocol]] was executed with one 500 µL sample of each replicate | ||
+ | ** the other 500 µL sample was treated with [[Team:Aachen/Notebook/Protocols#Acid_Hydrolysis| the acid hydrolysis protocoll]] | ||
Latest revision as of 03:58, 19 September 2015