Difference between revisions of "Team:Warwick/Project2"

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<H3>Experiment 1: Establishing Anchor Protein</H3>

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1. ~~Golden gate assembly~~ of plasmid ~~backbones~~ http://synbio.tsl.ac.uk/golden-gate-assembly-protocol/

+

1. Take a briobrick part (JO4450) and transform it into a chemically competent cell (Top 10)

−

and ~~4 G-blocks (one of each candidate anchor protein and Zif268)~~

+

2. Grow cells overnight then miniprep them to extract the transformed plasmid

−

~~Waiting on enzymes (hopefully Friday~~/ ~~Monday)~~

+

3. Double digestion of plasmid to cut out the RFP gene, leaving only the plasmid backbone

−

~~Lpp-OMPa is done~~

+

4. PCR the full construct G-Block (containing Zif268 and Lpp_OmpA) and digest the product with the corresponding enzymes

−

~~BclA, Pgsa,~~ (INP) ~~- waiting on enzymes to cut out~~ anchor proteins

+

5. <a href="http://synbio.tsl.ac.uk/golden-gate-assembly-protocol/">Golden gate assembly</a> of plasmid backbones

−

+

and full construct.

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2. Transform electrocompetent E. ~~Coli cells with plasmid~~

+

6. Transform electrocompetent E. coli cells with full plasmid

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NB - ~~IPTG needs to be added~~

+

7.Grow cells

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~~Grow~~ cells

+

8. Miniprep full construct plasmid from modified cells

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~~ Prepared~~ for microscopy (~~mounting medium)~~

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9. Digest plasmid with enzymes matching the cut sites around the Lpp_OmpA gene

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~~ DNA~~ on glass ~~(waiting epoxy, aminated oligo, fluorescent marker~~) ~~- Friday/Monday~~

+

10. PCR the rest of the anchor proteins from the G-blocks ordered (INP, PGSA, and BCLA)

−

+

11. Ligate the anchor proteins into digested full construct plasmid

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3. Bind antibodies to ~~flag~~ tag - measure ~~using~~ fluorescent ~~detection mechanism~~

+

12. Transform all plasmids into electrocompetent E. coli - End product is 4 different types of cell, each expressing the full construct with slightly different transmembrane domains

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~~Antonia has components~~

+

13. Prepare transformed cells for microscopy (mount cells on glass slides)

−

+

14. Bind antibodies to FLAG tag - measure under fluorescent microscope

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4. Compare intensities - select anchor protein that fluoresces brightest

+

15. Determine whether the gene is being expressed and whether the expressed protein is being transported and is binding to the membrane of the E. coli

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+

16. Compare intensities - select anchor protein that fluoresces brightest, this anchor protein with be used for all subsequent experiments.

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~~ Back-up:~~

+

−

~~ Lyse cells to see if expression is taking place~~

+

@@ Line 36: / Line 36: @@
 <H3>Experiment 1: Establishing Anchor Protein</H3>
-<br>1. Golden gate assembly of plasmid backbones http://synbio.tsl.ac.uk/golden-gate-assembly-protocol/
+<br>1. Take a briobrick part (JO4450) and transform it into a chemically competent cell (Top 10)
-and 4 G-blocks (one of each candidate anchor protein and Zif268)
+<br>2. Grow cells overnight then miniprep them to extract the transformed plasmid
-<br>Waiting on enzymes (hopefully Friday/ Monday)
+<br>3. Double digestion of plasmid to cut out the RFP gene, leaving only the plasmid backbone
-<br>Lpp-OMPa is done
+<br>4. PCR the full construct G-Block (containing Zif268 and Lpp_OmpA) and digest the product with the corresponding enzymes
-<br>BclA, Pgsa, (INP) - waiting on enzymes to cut out anchor proteins
+<br>5. <a href="http://synbio.tsl.ac.uk/golden-gate-assembly-protocol/">Golden gate assembly</a> of plasmid backbones
+and full construct.
-<br>2. Transform electrocompetent E. Coli cells with plasmid
+<br>6. Transform electrocompetent E. <i>coli</i> cells with full plasmid
-<br>NB - IPTG needs to be added
+<br>7.Grow cells
-<br>Grow cells
+<br>8. Miniprep full construct plasmid from modified cells
-<br>Prepared for microscopy (mounting medium)
+<br>9. Digest plasmid with enzymes matching the cut sites around the Lpp_OmpA gene
-<br>DNA on glass (waiting epoxy, aminated oligo, fluorescent marker) - Friday/Monday
+<br>10. PCR the rest of the anchor proteins from the G-blocks ordered (INP, PGSA, and BCLA)
+<br>11. Ligate the anchor proteins into digested full construct plasmid
-<br>3. Bind antibodies to flag tag - measure using fluorescent detection mechanism
+<br>12. Transform all plasmids into electrocompetent E. <i>coli</i> - End product is 4 different types of cell, each expressing the full construct with slightly different transmembrane domains
-<br>Antonia has components
+<br>13. Prepare transformed cells for microscopy (mount cells on glass slides)
+<br>14. Bind antibodies to FLAG tag - measure under fluorescent microscope
-<br>4. Compare intensities - select anchor protein that fluoresces brightest
+<br>15. Determine whether the gene is being expressed and whether the expressed protein is being transported and is binding to the membrane of the E. <i>coli</i>
+<br>16. Compare intensities - select anchor protein that fluoresces brightest, this anchor protein with be used for all subsequent experiments.
-<br>Back-up:
-<br>Lyse cells to see if expression is taking place
 </p>
 <p>

Difference between revisions of "Team:Warwick/Project2"

Revision as of 13:34, 9 September 2015

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Experiment 1: Establishing Anchor Protein

Experiment 2: Establishing Zinc Finger DNA Binding Proteins

Experiment 3: Checking Colour

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