Team:Bilkent UNAM Turkey/Protocols

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<h1> Growth Conditions </h1>
<h1> Growth Conditions </h1>
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'''Tris Acetate Phosphate (TAP) medium
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<b>Tris Acetate Phosphate (TAP) medium</b>
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'''
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from Gorman, D.S., and R.P. Levine (1965) Proc. Natl. Acad. Sci. USA 54, 1665-1669.<br>
from Gorman, D.S., and R.P. Levine (1965) Proc. Natl. Acad. Sci. USA 54, 1665-1669.<br>

Revision as of 01:42, 22 September 2011

Growth Conditions

Tris Acetate Phosphate (TAP) medium from Gorman, D.S., and R.P. Levine (1965) Proc. Natl. Acad. Sci. USA 54, 1665-1669.
This is probably the most widely-used medium at present for experimental work.
Following solutions are prepared.

1. TAP salts
NH4Cl 15.0 g
MgSO4 . 7H2O 4.0 g CaCl2 . 2H2O 2.0 g
water to 1 liter

2. phosphate solution

K2HPO4 28.8 g
KH2PO4 14.4 g
water to 100 ml

3. Hutner's trace elements


To make the final medium, mix the following:
2.42 g Tris
25 ml solution #1 (salts)
0.375 ml solution #2 (phosphate)
1.0 ml solution #3 (trace elements)
1.0 ml glacial acetic acid
water to 1 liter

For solid medium, add 15 g agar per liter

Autoclave.
For Tris-minimal medium omit the acetic acid and titrate the final solution to pH 7.0 with HCl

Reference: [[http://www.chlamy.org/TAP.html]]

'''Hutner's trace elements'''


Hutner et al. (1950) Proc. Am. Philos. Soc. 94, 152-170

This mixture is used both in TAP and in the Sueoka high salt medium.

For a detailed analysis of how well this trace elements solution meets the nutritional requirements of C. reinhardtii,
see Merchant et al. (2006) Biochim. Biophys. Acta 1763, 578-594.
For 1 liter final mix, dissolve each compound in the volume of water indicated.

The EDTA should be dissolved in boiling water, and the FeSO4 should be prepared last to avoid oxidation.
compound amount water
EDTA disodium salt 50 g 250 ml
ZnSO4 . 7 H2O 22 g 100 ml
H3BO3 11.4 g 200 ml
MnCl2 . 4 H2O 5.06 g 50 ml
CoCl2. 6 H2O 1.61 g 50 ml
CuSO4 . 5 H2O 1.57 g 50 ml
(NH4)6Mo7O24. 4 H2O 1.10 g 50 ml
FeSO4. 7 H2O 4.99 g 50 ml

Mix all solutions except EDTA. Bring to boil, then add EDTA solution. The mixture should turn green. When
everything is dissolved, cool to 70 degrees C. Keeping temperature at 70, add 85 ml hot 20% KOH solution (20 grams / 100 ml final volume).
Do NOT use NaOH to adjust the pH.

Bring the final solution to 1 liter total volume. It should be clear green initially. Stopper the flask with a
cotton plug and let it stand for 1-2 weeks, shaking it once a day. The solution should eventually turn purple and
leave a rust-brown precipitate, which can be removed by filtering through two layers of Whatman#1 filter paper,
repeating the filtration if necessary until the solution is clear. Store refrigerated or frozen convenient
aliquots. Some people shorten the time for formation of the precipiate by bubbling the solution with filtered air.

If no precipitate forms, the solution is still usable. However, you might want to check the pH in this case and
adjust it to around 7.0 using either KOH or HCl as needed.

To prepare sulfur-free trace elements for hydrogen generation, the sulfate salts can be replaced with equimolar
chloride salts (ZnCl2 10.0 g; CuCl2 . 2 H2O 1.00 g; FeCl2 . 4 H2O, 3.60 g). .
Reference: [[http://www.chlamy.org/trace.html]]

A. Glass bead method for nuclear transformation of Chlamydomonas reinhardtii
Materials.
- Cell-wall deficient (e.g. cw15) host cell strain. (If you need to use a strain with a wild-type cell-wall, the
cells must be treated with autolysin prior to vortexing with glass beads (step 7).)
- Sterile liquid growth medium (permissive for the host cell line). (Approximately 35mL of culture / transformation
plate.)
- Sterile liquid growth medium (corresponding to selective conditions). (This will be used to wash the cells by
centrifugation before transformation. Use appropriate medium( minimal, arginine free, etc) depending on the
selection for transformants that will be applied.)
- Prepare glass tubes (3 mL) with 0.3g glass beads (Thomas Scientific), sterilize by baking in oven. (A convenient
scoop can be made from the bottom of an Eppendorf tube and a blue pipetman tip, glued by gently melting the tip).
- Sterile centrifugation bottles and tubes.
- Sterile, cotton-plugged 5 mL pipets.
- Plates with appropriate solid medium for selection of the transformants.
- DNA with selection marker. (Circular, supercoiled DNA can be used, but in cases where single insertions are
desirable (e.g. insertional mutagenesis), a linear DNA fragment is preferable. The amount of DNA used will also
influence the number of insertions (approx. range: 0.2 – 1.0 ug / transformation).

Protocol.
1. Grow cells in appropriate medium (permissive) to a density of ~2 x 106/ mL.
2. Collect cells by centrifugation in sterile centrifugation bottles at room temperature (3500 g x 10 min). Discard
supernatant.
3. Resuspend cells in 1/25 – 1/50 initial volume in selective medium with a cotton-plugged pipet. Transfer to a
sterile centrifugation tube.
4. Collect cells by centrifugation at room temperature (3500 g x 10 min). Discard supernatant
5. Resuspend cells at approximately in 1/70 initial volume in selective medium (approximately 3.0 x 108 cells / mL.
Count a 1/100 dilution with the hemacytometer under the microscope. Adjust the volume to obtain a concentration of
2. x 108 cells / mL.
6. To a tube containing 0.3g glass beads (sterilized by baking) add:
- 0.3 mL cell suspension.
- ~ 0.5 – 1.0 ug DNA.
7. Vortex at full speed for 15 seconds.

8. Pour the contents of the tube on a selective plate, gently tilt and rotate the plate to spread the medium
evenly.
9. Allow the liquid to dry (protect from light to avoid phototactic movements of the cells). Seal the plates with
Parafilm (Micropore tape for minimal medium), and incubate under appropriate conditions for selection. (If cells
were grown under auxotrophic conditions (acetate, dark) and will be selected for photoautotrophic growth (minimal,
light), put the plates in dim light for 16 – 24 hours before transferring to light. Colonies will appear within 1-3
weeks depending on the selection applied.)
References:
Kindle, K. (1990) High-frequency nuclear transformation of Chlamydomonas reinhardtii. Proc. Natl. Acad. USA 87:
1228-1232.
B. Electroporation method for nuclear transformation of Chlamydomonas reinhardtii
Materials
- Cell-wall deficient host cell strain
- Sterile centrifugation bottles and tubes
- Electroporation cuvettes
- Plates with appropriate solid medium for selection of the transformants
- DNA with selection marker
- TAP, 40mM sucrose
- TAP, 40mM sucrose, 0.4% PEG 8 000 - Starch 20%
Starch 20% preparation
20 g starch in a centrifuge tube
Wash with ethanol 100%
Wash with water
Repeat 2 times
Resuspend in 100 ml Ethanol 70%
Aliquots of 20 ml and keep at room temperature
The day of transformation, centrifuge an aliquot 1 minute at 1 000 rpm
Wash 4 times with TAP + sucrose 40 mM
Resuspend in 20 ml of TAP + sucrose 40 mM + PEG 8 000 0.4%
Protocol
1. Grow 250 ml of cells to a density of 2 x 106 cells/ml
2. Collect cells by centrifugation at room temperature at 3 500 rpm for 5 minutes in sterile centrifugation
bottles. Discard supernatant

3. Resuspend in 1.25 ml of TAP, 40mM sucrose
4. Incubate on ice 10 minutes
5. Transfer 250 μl of cells in a cuvette containing 1 μg of DNA
6. Incubate at room temperature 5 minutes
7. Electroporate 0.75 kV, 25 μF, no R, 6 msec
8. Incubate at room temperature 10 minutes
9. Add 1 ml of starch 20% and pour the contents of the cuvette on a selective plate, gently tilt and rotate the
plate to spread the medium
10. Allow the liquid to dry (protect from light), seal the plates with parafilm and incubate under appropriate
conditions for selection of transformants.

References.
Boynton et al (1988) Chloroplast transformation in Chlamydomonas with high velocity microprojectiles. Science 240:
1534-1538.
Finer et al. (1992) Development of the particle inflow gun for DNA delivery to plant cells. Plant Cell Reports 11:
323-328.
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