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Experiment 12 Large-Scale Purification Of Plasmids pRIT4501 and pRIT4502 by Cesium Chloride Density Gradient Centrifugation Now that you have identified your two recombinant plasmids, you need to produce large-scale preparations of each so that you can study them further. To do this, you will prepare lysates of 500 ml cultures and purify the DNA by density gradient centrifugation. Although you could have used the alkaline lysis procedure from Experiment 11, you will use a different method here. In the current procedure, 500 ml of cells are concentrated and spheroplasted. They are then treated with Triton X-100, a very mild detergent, which produces holes in the cell wall without actually destroying it. The bulk of the plasmid will leak out of the cell wall but the chromosome remains trapped within and is removed when the cells are pelleted. The resulting plasmid solution is purified further by density gradient centrifugation. CsCl is added and the lysate is transferred to ultracentrifuge tubes. The tubes are spun at 40,000 rpm for two days. During this time, the CsCl forms a gradient and the molecules migrate according to their density until they float at their individual isopycnic points (the point in the gradient that equals the buoyant density of the molecule). Density is a function of AT/GC ratios. Each of the four bases has its unique density, and the final density of any DNA is the collective sum of the densities of the individual bases. Since the DNA’s of different species have different AT/GC ratios, it stands to reason that they also have different densities and, therefore, different isopycnic points. The relationship between AT/GC content and density is: ρ = 1.660 + 0.00098 x (%GC) %GC = ρ -1.660 0.00098 where ρ = density in g/ml and 1.660 is the density of DNA containing 100% AT. 89 Experiment 12 Relationship between AT/GC ratio and isopycnic point Percentage of Each Base Species A G C T A+T G+C E. coli 24.6 25.5 26.6 24.3 48.9 52.1 S. typhimurium 22.9 27.1 27.0 23.0 45.9 54.1 B. subtilis 28.4 21.0 21.6 29.0 57.4 42.6 bacteiophage λ 26.0 23.8 24.3 25.8 51.8 48.1 AT/GC 0.94 0.85 1.35 1.08 %GC 51.58 54.10 42.60 48.15 Buoyant Density (g/ml) 1.7106 1.7130 1.7017 1.7072 The two species that we are working with this semester, E. coli and B. subtilis have different AT/GC ratios, the later being somewhat poorer in GC. According to the table above, B. subtilis DNA has a lower density and, accordingly a lower isopycnic point. The difference in density between the two is significant; the two DNA’s would have different peaks in the gradient, and could easily be separated. Salmonella typhimurium is very closely related to E. coli and their DNA’s accordingly have very similar isopycnic points. The table also shows the density of phage λ DNA. After transferring the lysate to the ultracentrifuge tube, ethidium bromide is added. While ethidium bromide certainly facilitates collection of the DNA at the end of the centrifuge run by virtue of its fluorescence, it is actually an integral part of the separation process. Plasmid DNA and contaminating chromosome have about the same AT/GC ratio and thus cannot be separated easily. The addition of ethidium bromide rectifies this problem. Density is a function of AT/GC ratio, but it is also a function of conformation. For supercoiled DNA, there is more DNA per unit volume than for relaxed DNA. Intercalation of ethidium bromide into DNA causes the helix to unwind (negative supercoiling) and become more relaxed. As the DNA relaxes, mass is spread over a larger volume and the density decreases. When DNA is linear, its free ends can compensate for the supercoiling, and its isopycnic point is lowered. However, when the DNA is circular the ends are connected and cannot compensate for the supercoiling. In order to do so, the plasmid “kinks up” into a very tight knot, forcing more mass into a smaller volume. Thus, ethidium bromide causes the plasmid density to be increased. This principle can be demonstrated by the famous “rubber band experiment.” Find out more about density gradient ultracentrifugation in Appendix VIII 90 Large-Scale Plasmid Purification The Famous Rubber Band Experiment The Day Before Cell Lysis First Day 1. Obtain two identical rubber bands. Cut one and leave the other intact. 2. Holding one end of the cut rubber band, twist the other end 20 times. Hold on to both ends but let the rubber band relax and note the extent of collapse. 3. Holding the uncut rubber band in the middle, twist it 20 times at a point on the opposite side of the circle. Hold on to both points but let the rubber band relax and compare the extent of collapse in cut and uncut rubber bands. 4. Tape both twisted rubber bands into your lab notebook or include a cell phone photograph. 1. Prepare two 500 ml flasks of LB broth in liter flasks and autoclave. When cool, add enough ampicillin to give a final concentration of 50 µg/ml. 2. Inoculate each flask with one of your transformants and incubate over night shaking at 37o. 1. Harvest your cultures as follows: Transfer half of each culture to a 250 ml polypropylene bottle, balance, and centrifuge at 7,000 rpm for 10 minutes in the large floor-model centrifuge. Decant the supernatant. Pour the remaining half of the culture into the bottle now containing only the pellet. Centrifuge again and decant. Be very careful not to mix your cultures!! 2. In a normal lab situation you would continue through to the end of the protocol. However, due to the time constraints of our class schedule, we will stop here and continue next period. Some lysis protocols include a freeze/thaw step to break down the cell walls. Although this protocol does not, a freeze/thaw cycle can only help. 91 Experiment 12 Materials for Second Day Cell Lysis Second Day 25% sucrose lysozyme solution (5 mg/ml) 0.25 M EDTA, pH 8 Triton X-100 lytic mix 1. Prepare an ice bath and chill all of the materials. 2. Thaw the cell pellets and resuspend each in 1 ml ice-cold 25% sucrose. Place the tubes on ice for 30 minutes. Add 0.2 ml lysozyme solution, mix, and place on ice for 10 minute. Lysozyme breaks down the glycosydic bonds in the polysaccharide backbone of peptidoglycan. The isotonic environment created by the sucrose prevents the spheroplasts from lysing. 3. 4. Add 0.4 ml EDTA, mix, and place on ice for 10 minutes. EDTA is a chelating agent that absorbs divalent cations (Ca++ and Mg++), which are required by most bacterial nucleases. When the cells lyse, these nucleases will no longer be regulated and will begin degrading plasmid DNA. The addition of EDTA therefore inactivates these nasty enzymes. 5. Add 1.6 ml Triton X-100 lytic mix. Mix by rocking the tubes very gently and place on ice for 20 minutes. Triton X-100, which is a detergent, gently lyses the cells by dissolving the lipids in the cell membrane. Because of the gentle lysis, most of the chromosomal DNA remains unfragmented and becomes entangled in the cellular debris. Plasmids, being considerably smaller, diffuse out into the surrounding solution. Your samples should become very viscous and “snotty.” 6. Centrifuge the lysate at 17,000 rpm for 30 minutes. The resulting supernatant contains approximately 95% of the plasmid in about 3.2 ml. This may be purified further by CsCl density gradient centrifugation. 92 Large-Scale Plasmid Purification Preparing the Gradient 1. Transfer your lysate to a plastic disposable centrifuge tube. Add 2 ml TES and 4.9 g CsCl. Shake gently to dissolve. CsCl becomes very cold as it dissolves. 2. Obtain a Beckman “Quick-Seal” tube and a long-tip Pasteur pipet. Carefully transfer your DNA to the “Quick-Seal” tube by inserting the tip of the pipet into the tube’s neck. 3. Using a 1 ml syringe with a 16 g needle, carefully add 200 µl of ethidium bromide (10 mg/ml) to the sample so that the ethidium bromide floats on top. Visible light will cause nicks in DNA when ethidium bromide is present. It is not necessary to work in the dark, but on the other hand, you shouldn’t go out of your way to expose the DNA to bright light. Fill the remaining space in the “Quick-Seal” tube up to, but not into, the neck with mineral oil. If you do not fill up the unused space, the tube will collapse during the centrifugation. 4. 5. Balance the tubes. The class will gather together and balance all of the tubes at once. You may remove liquid by wrapping a kimwipe around the mouth of the tube and squeezing. If extra weight is needed, add additional mineral oil. Each pair of tubes must weigh within 0.02 g of each other. 6. Seal the tubes according to the diagrams below. 93 Experiment 12 Collecting the Gradient 7. Rock the tubes to mix the ethidium bromide and place them in a Beckman Ti50 ultracentrifuge rotor and spin at 40,000 rpm for 44 hours at 20o. During most of the spin, the CsCl will sort itself out into a density gradient -dilute at the top and concentrated at the bottom. Towards the end of the spin the samples will begin to sort themselves out according to their buoyant densities. 1. At the end of the run, carefully remove your samples and look at them under blacklight. You should see two bands. The upper, narrower band is residual chromosome that was not removed during lysis. The lower, heavy band is plasmid. You should also see a pellet of RNA on the bottom and a cap of residual protein floating on top. 2. Carefully clamp the tube to a ring stand. Puncture the top of the tube with a wide-bore hypodermic needle (16 g x 1 1/2”). 3. Puncture the gradient just below the plasmid band with a narrowbore needle (21 g x 1 1/2”) attached to a 10 ml syringe. Never use a wide-bore needle to collect a gradient. It will create currents in the tube that will mix up the gradient. The needle should be pointed down so as to not disturb the plasmid, and away from the pellet so as not to become contaminated with RNA. This can be a very stressful operation the first time you try it. The most common error is to jerk your hand back when the needle suddenly goes through the wall of the tube. This results in pulling the needle out, and the plasmid running out through the hole. It is a rare person who can stick the needle back in the hole in time to save the DNA. The second most common error is to push so hard that the needle penetrates the wall, goes through the gradient, and comes out the other side. Your other hand will be holding the tube to steady it, so you must be mindful of where you put your fingers. 94 Large-Scale Plasmid Purification 4. When the needle is in the gradient, turn it so that the beveled side is up and tip it so that it touches the underside of the band. Carefully draw off the plasmid. As you draw off the plasmid, you are introducing a discontinuity into an originally continuous gradient. There is a great enough difference in refractive index on either side of the discontinuity to see an interface. This interface is in the same position as the plasmid band and it could fool you into thinking that there is still plasmid there. It is good to get all of the plasmid, but if you get too greedy, you will end up collecting chromosome DNA that is following just behind the plasmid band. 5. When you have recovered the plasmid band, withdraw the needle and allow the gradient to dribble into a beaker. Cut the tube in half so that the remaining ethidium bromide and mineral oil can drain into the beaker for disposal by the instructor. 6. Extract the ethidium bromide with isopropanol saturated with cesium chloride. Remove the 21 g needle you used to collect the plasmid and replace it with a wider 16 g needle. Draw up a large volume of isopropanol into the syringe, rock it a few times, and hold the syringe needle-up for a moment to let the phases separate. The DNA will be on the bottom. Near the collection setup there will be a flask containing a 25 ml pipet with a rubber bulb. Holding the syringe needle-up, insert the needle into the bulb and eject the isopropanol into the bulb, where it will run down the pipet and collect in the flask. Repeat as many times as necessary to remove all of the ethidium bromide, but do at least two extractions. 95 Experiment 12 7. Obtain a dialysis bag and two dialysis clips. Drain as much liquid out of the bag as possible and then clip one end. Carefully transfer the DNA into the bag. Half close the clip on the top of the bag and pull the neck of the bag through the clip until all of the liquid is forced into the bottom. Snap the clip shut. The bag should be taut. Dialyze the DNA over night in 4 liters of TE buffer. 8. On the following day, carefully remove the DNA with a pasteur pipet and store it in a microfuge tube for use in Experiment 7. TES Buffer 1 M Tris, pH 8................................................................... 2.5 ml 0.25 M EDTA, pH 8........................................................ 1.0 ml 5 M NaCl.......................................................................... 0.5 ml water................................................................................. 46.0 ml 96 Large-Scale Plasmid Purification 25% Sucrose 1 M Tris, pH 8 ................................................................. 2.5 ml 0.25 M EDTA, pH 8....................................................... 0.2 ml sucrose.............................................................................. 12.5 g water................................................................................. 47.3 ml Triton X-100 Lytic Mix 10% Triton X-100............................................................ 1 ml 1 M Tris, pH 8.................................................................. 5 ml 0.25 M EDTA, pH 8........................................................ 25 ml water................................................................................. 69 ml Isopropanol Saturated with Cesium Chloride Prepare a solution of CsCl (1 g/ml) in water. Add enough to saturate 250 ml of isopropanol. Once isopropanol is saturated, it becomes immiscible with water. You will know when the isopropanol is saturated because the excess CsCl will form a clearly visible layer at the bottom of the bottle. If you use unsaturated isopropanol to extract ethidium bromide from your plasmid prep, the isopropanol will draw water from your sample and the CsCl will precipitate. Preparation of Dialysis Tubing 1. Cut the tubing into lengths of 15 - 20 cm. 2. Boil for 10 minutes in a large volume of 1 mM EDTA, pH 8, and 2% sodium bicarbonate. 3. Rinse well in distilled water. 4. Boil for 10 minutes in distilled water. 5. Allow to cool and store in water in refrigerator. Make sure that tubing is always wet. 6. Always handle tubing with gloves!! 97