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Experimental Design
Hello everybody this is Doctor Vishal Trivedi from department of biosciences andbioengineering, IIT Guwahati. And in what we were discussing? We were discussing about theelectrophoresis and in this particular module we have discussed about the basics ofelectrophoresis followed by the vertical gel electrophoresis, horizontal gel electrophoresis. Andthen in the previous lectures, we have also discussed about the different variants of the gelelectrophoresis.And then ultimately we have also discussed about the some of the research problems where youcan be able to utilize the electrophoresis as a tool to answer those questions. And in thisparticular series now today we are also going to discuss few more experiments and few moreresearch problems and while discussing these research problems, you will be able to understandmore and more potential of the electrophoresis to solve the research problems related to yourwork.(Refer Slide Time: 02:04)
So the first problem today what we are going to see is, and this is a old problem what we havediscussed before also that the scientists have discovered a transcription factor, and in skin cellsbinds to the set of gene X which is responsible for changing its color due to the exposure to thesunlight. Now, they would like to identify the transcription factor from the skin cells. What theywant to do is if you remember in the previous lecture what we have discussed that they wereinterested to identify the transcription factor.And then on the top they are also interested how the DNA as well as this transcription factor isinteracting with each other So as we I think discussed that the gene structure is made up ofpromoter and then you have the coding region. So this coding region is not responsible forbinding of the transcription factor. Only the promoter region is responsible for binding of thetranscription factor and in this event, what will happen is that the DNA is making a complex withthe protein.And as the result it is forming a DNA protein complex. Now if you see how it is can be it howthis interaction can be mapped with the help of the electrophoresis?(Refer Slide Time: 03:34)
So in the experimental design what we have, we have the 2 molecules. One is DNA the other oneis the protein and what they are doing is there interacting with each other to form the DNAprotein Complex. Now let us assume that the DNA is of the molecular weight of 1 unit and the
protein is also of a molecular weight of the 1 unit which means the DNA protein complex isgoing to have the molecular weight of 2 units.Now, let us assume that the DNA if you do the electrophoresis of these 3 molecules then theelectrophoretic mobility of DNA is X. The electrophoretic mobility of Y is the protein is Y thenand the DNA protein complex is Z, then the question comes whether the X is going to be biggerto the Z or X is going to be the smaller to the Z which means whether the DNA is going to be runfastest than the DNA what is present in the complex or whether the DNA what is present is goingto be run slower that the DNA what is present in the complex.As obvious that the molecular weight of the DNA protein complex is bigger. So it is actuallygoing to run on a slower size, which means the DNA is going to have the higher electrophoreticmobility compared to the DNA what is present in the protein. Because as you remember; that theelectrophoretic mobility in the gel electrophoresis is directly proportional to the chart andinversely proportional to the molecular weight.This means you have a smaller molecular weight, you are going to run faster and you are goingto have a larger distance, you will cover the larger distance where as if you have a biggermolecular weight then you are going to run the smaller distances.(Refer Slide Time: 05:43)
So this interaction of the protein and DNA is been mapped with the technique or with the assaywhich is called as the gel mobility shift assay. In this technique is relies on the fact that a small
DNA has a much higher mobility in gel electrophoresis then what is bound to the protein. Sowhat you can see is if I am running the electrophoresis or if I am doing the electrophoresis of theDNA alone the DNA will run up to this point. But if I keep adding the protein molecules, theprotein molecules are actually binding to the protein to the DNA and as a result it is actuallyreducing its electrophoretic mobility.Now Imagine that the DNA what you are putting it for the electrophoresis is 100 kilo Dalton, okand the protein what we are putting is a 25 kilo Dalton. Now see when you are running the DNAalone, it is actually having a molecular weight of 100 kilo Dalton. But when you are adding thesmall amount of protein it is actually the 1 molecule of the protein if the 1 molecule of protein isinteracting with the DNA, the resultant molecular weight is going to be 125 kilo Dalton.Similarly if the 2 molecules of the protein will interact then it is going to have the molecularweight of 150 kilo Dalton and if the 3 molecules of the protein are going to interact, it is actuallygoing to have the 170 kilo Dalton as a molecular weight. This means as the more and moreprotein molecules will bind to this DNA molecule the resultant molecular weight of the complexis going to be keep increasing which means you can be able to map the interaction between the 2molecules simply by looking at the molecular mass.(Refer Slide Time: 07:38)
So for performing this experiment what you are supposed to do? You have to first prepare thecell lysate you have to do the incubation reactions where you are actually going to incubate the
DNA plus the protein, ok and then you are going to done the polyacrylamide gel electrophoresis,and that actually is going to give you the resultant that addition of the DNA bands.(Refer Slide Time: 08:08)
The material reagents the material and equipment what your required. So the first reagent whatyou required is the labeling reaction mixtures so that you will be able to label the DNA. Because,how are you going to monitor the migration of retardation of the DNA molecule is that youactually going to label the DNA with a radioactive material. So in this case we are using the P32labeled oligonucleotides.So what you going to do is you are going to take the oligonucleotides you are going to run the10X PNK reaction buffers and then you are going to add the enzyme that T4 polynucleotidekinase and then you are going to add the alpha 32 labels ATP and the double distilled water. Andthis labeling reactions is going to be catalyzed and then it is actually going to label the DNAmolecule which is the oligonucleotide which you are going to use in the gel shift assays.You also need the binding assay buffer. So the composition of the binding assay buffer is givenhere which actually mostly contains the buffers, then you have the reducing agents and then youhave the EDTA so that you should take care of the contaminating metals and all that and thenyou need to resolving the buffer which you are going to use for running the page. So 5X TBEbuffer where you are going to have Tris, boric acid and EDTA and then the final volume whatyou are going to make up to the 1 liter.
And then you need to prepare the recipe for the non-denaturing page gel, so where you going totake the acrylamide, water, TBE then APS and TEMED are going to be added as thepolymerization agents. And then you would require the sense as well as the antisenseoligonucleotides. So that you can be able to design the oligonucleotides and then in theinstrument what you required you need gel electrophoresis system and as well as the microfuge.Microfuge means you required a small centrifuge so that you will be able to pallet down thereaction mixture. This can be done in a multistep.(Refer Slide Time: 10:33)
So in the step 1 you are going to prepare the labeled probe. So the labeled probe can be preparedby multiple ways and that all we are going to discuss in detail when we are going to discuss thesouthern blotting. So for the time being you can just simply understand that you are going to addyou are going to take the oligonucleotide you are going to add the radioactivity or radio labeledATP.And then you are just simply going to add the PNK and that actually is going to catalyze thereactions to add the ATP to the oligonucleotides. So here you are going to take the 2oligonucleotide, one is sense oligonucleotide the other one is the antisense onigonucleotide sothat you can be able to design a double stranded DNA. So for example, they have given you asequence of the sense and antisense oligonucleotide.
So this is the sense strand this is the antisense strand which you can use and this is the sequencewhich is actually going to bind or which is going to facilitate the binding of the protein. So that isthe region which you have to keep in the centre of this particular sequence. So that they will beadequate amount of nucleotides will be available on both the sides. So that the protein could beable to fit on top of this particular sequence and will be able to bind very nicely.Then you have to do the, you know several steps of doing the labeling reactions and thenultimately you have to purify the labeled nucleotide by the gel filtration column using the G50columns. And this column is pre-equilibrated with the buffers so that you will be able to removethe excess radio activity from the radio labeled nucleotide. So once your labeled probe is ready,then you have to go to the step 2.(Refer Slide Time: 12:39)
So in the step 2 you have to set up the reactions, so for the setting of the binding reactions whatyou have do is you have to take up the nuclear protein extracts are incubated with the labeledprobe. While setting of the binding reactions the following components are added in the givenorder under the ice cold condition. So this is very important that you do all these experimentsunder the low temperature conditions.So that there will be no degradation of the DNA or there will be no decoration of protein as well.Because either of these degradations; are going to compromise the overall effects. So what youneed is you need the Salmon sperm DNA which you are going to prepare in DEPC treated water.
So DEPC treated water is a water which is free of the RNA so that there will be no degradationof the RNA.If at all the RNA is present because that actually is going to mask the signal what you are goingto get from the DNA. Then you also need the binding buffers so the composition of the bindingbuffers is already been given the previous slide. Then you have to prepare the nuclear extracts.So you have to add the X microliter of nuclear extract. So that depends what kind of activity ispresent in your sample and all that.Then you require the labeled probe. So this nuclear extract is actually going to be the source ofthe protein because the nuclear extract is going to have the transcription factor. So that you areinterested to test and then you have to make up the volume with the double distilled water. Soafter the addition of the all the components over the eyes the tubes are spinned briefly inmicrofuge so that you can be able to collect all the reaction mixtures.And then they are incubated for 45 minutes at 25 degree Celsius so that there will be interactionof the transcription factors, what is present in the nuclear extract with the oligonucleotide whichis you are adding and then is it is actually going to form the complex. In this there will be avariation that for the super shift experiment. So super shift experiments are the experimentswhere are you are also been interested that which protein in actually binding.So in those cases what you can do is, you can simply add the antibodies directed against aparticular transcription factor so that you will be able to not know only that the proteins arebinding but also which protein is binding. So those kinds of experiments are called super shiftexperiments. Because in a normal shift, normal gel shift assay what you are going to do is, youare going to see a gradual retardation of the DNA or gradual moving of the DNA on the upwardside.But in the super shift experiment as soon as you add the antibodies, the antibodies are going toincrease the molecular weight of the complex very high. So because of that it is actually going togive you at additional shift into the retardation. So the 2 microgram of the respective antibody isadded to the binding reaction before prior to the addition of the labeled probe. Because of that itactually going to label or it is going to bind the protein or the transcription factor of your interest.
So because of that it is actually going to show you the super shift which means in a normal thingwhat you have is, you have a DNA here and then it will gradually grow actually. Whereas in thesuper shift what will happen is you have a DNA here and then it will show a very large jump interms of shift. Because here; you have only the protein whereas here you have the protein as wellas the antibody.So that actually is going to increase the molecular weight in very large quantities. So it will beactually going to add up a lot in terms of the final protein DNA complex what is going to beformed. So this mixture was incubated for 20 minutes and then the labeled probe is added andincubation are carrying out for another 45 minutes. So the only difference between a normal gelshift assay as well as the super shift assay is that you have to add antibodies prior to adding theoligonucleotide.So that the antibodies will go and bind to their respective target protein and then if those proteinsare go and bind into your DNA they are actually going to show you the super shift.(Refer Slide Time: 17:20)
Then the step 3 you have to do the analysis of the reaction. So once the analysis incubationperiods are over then what you have to do is you have to take these samples and then you have toanalyze them onto the 5% non-denaturing polyacrylamide gels. In each well, you can you canresolve the 20 microliter of the reaction mixture and to monitor the progress of the gel a tube
containing the labeled probe alone together with the dye bromophenol blue is added in one of thelanes.So that you will be able to do you will be able to see how long the DNA will migrate if theprotein component is not available. Because that will be your reference point how much shift ofthe DNA band you are getting when you are adding the nuclear extracts. Then the 5X TBE isused as a running buffer. The gel is run at the 50 volts constant and it has to be done in a coldcondition so that there will be no degradation of the DNA.Because if there will be any degradation of the DNA that also is going to give you a gradualdecrease in molecular evidence so that also is going to give you a mere lie condition. So if therewill be a DNA degradation what will happen is the DNA will be here and then you are going tosee a lot of bands at that actually is going to mask the actual DNA samples. Even if you have asample of DNA here, it is actually going to be masked by that degradation of the DNA probewhat you have added in this reaction mixture.So because of that, it is important that you should keep the DNA in a very stable condition. Andyou should when even when you are resolving the samples and also should resolve it in a coldcondition so that there will be no degradation. After completion of the electrophoresis the gel isdried up by wrapping it in the gel wrap and it is exposed to a sensitive x-ray film for 1 to 3 days.Band can be seen after developing the film and densitometrically analyzed using image Jsoftware.So the image analysis anyway we have discussed in a detail. So that you can be able to have thedigital image you can be able to utilize many software’s what we have discussed before also.That you know either you can use image J or any other commercial software what are availablefrom the different companies.(Refer Slide Time: 20:04)
Let us see what results you are going to see so the in the results section the positive autoradiographs shows that the positive binding experiments which means what you can see in atypical experiment that when you are running the probe alone, it is actually going to run in a veryfar away from your lane. But as you increase or as you put the nuclear extract what will happenis that band is going to be keep moving towards the upper side.Which; means the proteins are now binding in a very low quantity and then ultimately the wholeprotein is bound. And what you see is actually there will be a separation which means what yousee is the kind of the curve which means at this stage the whole DNA, what you have added inbeen saturated by the proteins which are present in the nuclear extract. Now how you can be ableto verify this? You can be able to verify this by adding the cold oligonucleotides.So what will happen if you add the cold nucleotides? The cold nucleotide is going to compatitewith the protein what is bound here. And because of that it is actually going to release the boundoligonucleotide which is the labeled oligonucleotide. So what will happen is that you will bekeep observing the band at the bottom. So if you are going to form the protein complexes andthen if you add the cold oligonucleotide.What is mean by the cold oligonucleotide is the unlabeled oligonucleotide. So that unlabeledoligonucleotide is going to compatite with the complex and it is going to release the radio labeledoligonucleotide. And in that process, you are going to again going to see the re-appearance of the
radio labeled oligonucleotide. Because that the protein is making a complex with DNA is givingyou the protein DNA complex.But if you add the probe which is not radio labeled so this probe is actually radio labeled, that iswhy you have a radio labeled complex. So if you add the probe or the DNA which is not radiolabeled so what will happen is in that this protein is going to be fractionate between the labeledprobe versus the unlabeled probe. So ultimately what will happen is it is going to start formingthe complex with the unlabeled probe and the labeled probe is now going to be released from thereactions.And this labeled probe is again going to be electrophorate or it is going to have the similar kindof electrophoretic mobility what a free probe is having. So that is why you are actually going tosee the reappearance of the labeled probe. So that is a kind of a verification that this is a specificinteractions on the top if you are more interested. What you can do also is you can simply blockthe sides; what is present on to the DNA as well with the help of different types of antibodies andin those cases the protein what you are going to add will not be able to interact.So these are the different ways in which you are going to get the result and in which you can beable to verify the results. So with this I would like to conclude our lecture here in our subsequentlecture we are going to discuss some more problems related to electrophoresis.
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