Team:SUSTC-Shenzhen/Notebook/Preparation work

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Team SUSTC-Shenzhen

Notebook

Element of an endeavor

experiment training& plasmid building

To build the plasmid

2014.6.12, 10:00

bacteria transformation

‘’protocol’’

  1. add 2ul plasmid into the active bacteria(100 ul)
  2. incubate on ice for 20min
  3. 42°C water bath for 20 min
  4. ice, 2 min
  5. add 500ul LB
  6. 37°C shake, 14 min , 100 rpm
  7. 3000 rpm, 2 min
  8. incubate
    • plate streaking
    • plate pouring(100ul)
    • liquid incubate(10ul)
  9. incubate in 37°C incubator overnight
  10. liquid medium in shaker 36.4°C, 200rpm

2014.6.13

LB media composition

‘’protocol’’

  • 1L LB medium
    • 950ml ddH2O
    • 10g tryptone
    • 5g yeast extract
    • 10g sodium chloride
    • 15g agar
    • PH 7.0

2014.6.18

Sterilization 121°C 20min

2014.6.19

results

result recoveryplasmidbacteria volume
PSBIC3-BBa-I13521C+-20 min5ul100ul
PSBIC3-BBa-I13521A+-20 min5ul100ul
PSBIC3-BBa-I13521K++20 min5ul100ul
PET28a-SUMOK++15 min1ul50ul
mLDHA-PGEM-TA++15 min5ul50ul
PET-M3CA++15 min5ul50ul
PSBIC3-BBa-I13522C+-20 min5ul100ul
PSBIC3-BBa-I13522A+-20 min5ul100ul
PSBIC3-BBa-I13522K++20 min5ul100ul


2014.6.21

select the success of transformed plasmid

plasmid

plasmidrestrictionddH2Osample
PSBIC3-BBa-I13521C+A+K+20ul5G,P3
PSBIC3-BBa-K608008C+A+K+20ul5I,P1

protocol

  1. take out the competent cell from -80.2°C, and put with plamid in ice until they melt.(about 5min)
  2. put the plasmid into the cell, and put it on the ice for about 30min
  3. 42°C water bath for 90sec
  4. ice deal for 2min
  5. add LB in the this system(500ul)
  6. shake in the shaker for 30min
  7. spread plate

2014.6.21

Select the colony of mLDHA-PGEM7 and PEFM3C into the liquid medium
shake for 16hrs

2014.6.22

pladmid extract

Use the tiangen mini extract plasmid kit to extract plasmids, and got 16704ng/ul

Electrophoresis &extract plasmid

protocol

  1. component of gel
    1. 1% agarose(0.41g)
    2. TAB 41ml
    3. golden gel 0.5ul
    4. add on the ice for 30min(without any bubble)
  2. use kit(Tiangen) to make buffer
    • 5XM3C+5XmcDHA, add bacteria into the tube, then add P2 to mix up
  3. centrifuge 2minX2
  4. P1(150ul), P2(150ul), P3(150ul), store at 4°C, centrifuge 5min
  5. silica gel column, 600ul supernatant, centrifuge 30sec
  6. pour the percolate, add PWT 300ul, centrifuge for 1min, pour out percolate, add nothing but centrifuge for 2min to remove the alcohol.
  7. add 50ul TB buffer, centrifuge for 1min, keep the percolate, put on the ice.
  8. make the 50X TAE buffer, and add TAE, drown the gel.
  9. add marker 3ul,
  10. DNA loading buffer(1 drop)+plasmid extract(20ul)
  11. test the concentration by the nanodrop

2014.7.16, 4:00

group

Bacteria 50ul per group, and plasmid:bacteria is 3%

I13521(C+)K+C+A+0
K571005(C+)K+C+A+0
K608008(C+)K+C+A+0
K608008 plasmid:bacteria(C+)1:11:101:1001:1000

results

Only the antibiotics-free(0) group grow up bacteria

repeat experiment

Shake bacteria about 20hrs
incubate in incubator about 16hrs

C+K608008C+K571005K+I13521
fewfewdense but concentrate

All of above do not have fluorescence

2014.7.18

gradient antibiotics&single colonies Make 100ml liquid LB medium

2014.7.19

Extract the plasmid of K608008 and do the restriction by restriction enzyme

2014.7.20

  1. make 0 and A+ LB liquid medium
  2. plasmid data(following table)
  3. transformation of biobricks
    1. add 20ul ddH2O into the hole in the plate
    2. get 5ul plasmid
    3. use the transformation protocol
    4. spread plate 50ul

BBa_J2310120Kplate126056bpC+
BBa_I2026018aplate42989bpC+
BBa_J2311522Iplate121056bp C+
BBa_E024024Bplate22946bp C+

2014.7.21

2:45pm

C+ J23115 +(only one grew up)

4:00pm

biobrick colony number
BBa_J23101+1
BBa_I20260 in C+-0
BBa_I20260 in K++2
BBa_J23115++2
BBa_E0240+2

2014.7.22,8:24

biobrick colony number
BBa_J23101+++10
BBa_I20260 in C+-0
BBa_I20260 in K++1
BBa_J23115+2
BBa_E0240+2

Note: the concentration of I20260 is less than 5ul.

2014.7.24,11:00am

‘’explore the situation suitable for transformation of biobricks’’ K608008, C+
The heat-streak time

45s60s75s90s105s120s

2014.7.25

8:00am

Blank

15:30pm

All have the single colony but the same

2014.7.27

The plasmid building

plasmidrestriction enzymeposition
pX330XBaI NotI5100 3400
pBx084, Mcherry AflIII1300 5500
pBx093AflIII1300 8000
pBx090PstI500 1400 4000
pBx083AflIII1300 2400 4100
J23101PstI2100
J23115PstI2100

Maintained by the iGEM team SUSTC-Shenzhen.

Licensed under CC BY 4.0.