Team:Cambridge/Lab book/Week 7

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This is a detailed record of our work during the Summer...Read More

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Week:	3	4	5	6	7	8	9

Contents

1 Monday (06/08/12)
2 Tuesday (07/08/12)
3 Wednesday (08/08/12)
4 Thursday (09/08/12)
5 Friday (10/08/12)
6 Saturday (11/08/12)
7 Sunday (12/08/12)

Monday (06/08/12)

PCR of Magnesium riboswitch vector fragment B and Magnesium promoter

Riboswitch and promoter gel. Lanes 2+3: Fragment B without 8 codon substitution, lanes 4+5: Fragment B with 8 codon substitution, lanes 6+7: magnesium sensitive promoter, lane 8: +ve control

Normal PCR settings used, annealing temperature 57 °C, elongation step 90s long.

Lane 5 accidentally loaded with a DNA ladder instead of loading dye.

Expected fragment sizes:

Lane 2-5: 3kbp

Lane 6-7: 300bp

After electrophoresis, found vector products had, for the most part, worked. Promoter elements were not amplified - no band of the expected size was observed.

Positive control also failed, although this has ceased to work for several days, potentially due to DNA degradation.

Tuesday (07/08/12)

Production of electrocompetent e.coli

Gibson assembly of magnesium riboswitch and fluorescent construct

NAD+ added to isothermal buffer*5 mix

Gel slices from yesterday (of vector fragment B) purified.

DNA added as follows:

Without 8 codon substitution:

Reaction 1: Tube 2 (07/08/12) (fragment B), Tube 1 (05/08/12) (fragment A), Tube 28 (29/08/12) (riboswitch DNA).

Reaction 2: Tube 3 (07/08/12) (fragment B), Tube 2 (05/08/12) (fragment A), Tube 29 (29/08/12) (riboswitch DNA).

With 8 codon substitution:

Reaction 3: Tube 4 (07/08/12) (fragment B), Tube 1 (05/08/12) (fragment A), Tube 2 (18/07/12) (riboswitch DNA).

Wednesday (08/08/12)

Electrical transformation of competent e.coli with Gibson products

Gibson constructs from yesterday (fluorescent and magnesium riboswitch) transformed into e.coli produced yesterday.

Cells plated out onto 50 μg/ml ampicillin plates. Put in incubator overnight.

Thursday (09/08/12)

Making chemically competent e.coli

1l SOB made up.

PCR of mOrange vector

Split mOrange vector amplification attempted again.

Friday (10/08/12)

Saturday (11/08/12)

Transformation of e.coli with Magnesium riboswitch construct

Gibson products from 07/08/12 transformed into chemically competent cells.

Transformants plated out on 100 μg/ml ampicillin plates

Sunday (12/08/12)

Assembly of sfGFP construct from known functional DNA fragments

Fragments provided by who? assembled with Gibson.

Transformation of e.coli with fluorescent construct and sfGFP positive control

Chemically competent e.coli cells transformed with fluorescent construct Gibson product from 07/08/12.

E.coli cells also transformed with sfGFP Gibson product made earlier today in triplicate.

All transformants plated out on 100 μg/ml ampicillin.

sfGFP fragments have produced successful Gibson products in the past, so this will act as our positive control. If cells grow with the plasmid and fluoresce properly, we will know the master mix works. Otherwise, we will remake the master mix.

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