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  • Hi. It's Mr. Andersen and welcome to biology essentials video number 27. This

  • is on DNA and RNA. I want to start with a picture of a peanut plant. Right here we have

  • the same peanut plant in both of these. On the left side it's being decimated by the

  • larvae from a corn stalk bore. The one on the right however you can see the bore sitting

  • right here but it's not eating the peanut. And the reason why is this one over here has

  • been engineered. They've actually added a gene from a bacteria called bacillus thuringiensis.

  • And it produces a toxin that the larvae doesn't like. So it takes a couple of bites. Quits

  • eating it. So there are two things that I wanted to show you with this picture. Number

  • one is this idea that no matter what you are, a virus, a bacteria, eukaryote, like a plant

  • or an animal, you have the same genetic material. And that's called DNA. The other thing that's

  • interesting is that humans can tamper with this. We can actually transfer DNA from one

  • organism to another. We can transform that organism. And that whole field is called genetic

  • engineering and it's exploding right now. So in this podcast I'm going to try to accomplish

  • five things. First of all we're going to talk about the history of DNA. How these three

  • experiments, the Avery-MacLeod-McCarty, the Hershey-Chase and finally the Watson-Crick-Wilkins

  • and Franklin experiments showed us what DNA looks like. Where it is and how it works.

  • Next I'll talk about how DNA is organized in chromosomes. Both prokaryotic and eukaryotic.

  • We'll talk about the structure of DNA and RNA. Mostly how they're different. And then

  • how DNA makes copies of itself. We'll then discuss the Central Dogma. How DNA is transferred

  • through transcription into RNA. Which is then translated into proteins which then makes

  • you. And then finally we're going to talk about this brave frontier of genetic engineering.

  • And how we can do things like transform bacteria to make important things. Especially for diabetics,

  • like human insulin. And so that's a lot to do. So we better get started. Let's start

  • way back in history with the Frederick Griffith experiment. This was in 1928. He was a medical

  • doctor. And so what he was looking at was bacteria. And they would do serological testing.

  • So they're trying to figure out what bacteria causes disease and they were using a mouse

  • as a lab experiment. So right here they're using streptococcus pneumoniae, they're taking

  • one type of that. It's called rough, because when you grow it in plates it has a rough

  • appearance. They would inject that into the mouse and the mouse would be happy. They'd

  • then inject a different type of that streptococcus, a virulent type. This one is smooth. They'd

  • inject it into the mouse and then it would die. And so he hasn't learned anything at

  • this point. He then took this evil smooth strain of streptococcus. He heat killed it.

  • So he heated it up. And he found when he injected that heated into the mouse, the mouse was

  • good to go. So we haven't learned anything yet. What he then found, and this would be

  • that discrepant event, is that when he took the rough strain, which normally doesn't hurt

  • the mouse at all, he then mixed it with the heat killed smooth strain which normally doesn't

  • hurt the mouse at all. The mouse died. And so what did he learn from that? Well he learned

  • a lot. And the big thing he learned is that there was a transforming factor. Something

  • was being transferred from these dead smooth strain to these live rough strain. It was

  • transforming them into a virulent type of a bacteria. He didn't know what it was, but

  • we took the next 30 years to figure out that is was DNA. And we figured out the structure

  • of that. So the first step came through the Avery-McCarty-MacLeod experiments. And this

  • is in the 30s and 40s. And what they did is looked at Fredrick Griffith's experiment and

  • they tried to figure out what was this transforming factor? What was being transferred from these

  • heat killed smooth strain over to these rough strain? And so they broke down the bacteria.

  • They then isolated the major molecules inside that. And so what they had was RNA. They also

  • had proteins. And then the last thing that they found was DNA. And we knew what DNA was.

  • We'd known it for you know 50 years before then. And so what they then used was enzymes

  • that broke down each of these. And then they'd see if you could transform the bacteria again.

  • So they add a ribonuclease and broke down the RNA and it still was able to transform.

  • They added a couple enzymes, trypsin and chimotrypsin that break down proteins. It was still able

  • to transform. And then they added a deoxyribonuclease which breaks down DNA and then they couldn't

  • transform. And so what did Avery-McCarty-MacLeod figure out? DNA was this transforming factor.

  • Now most of their work was largely ignored and the reason why is most scientists thought

  • DNA was not complex enough to be the stuff of life. It only has four different letters

  • and we'll talk about that in just a second. And so that couldn't be the stuff of life.

  • And so a lot of their work was actually ignored. But in retrospect we look back and they show

  • that they were the ones who figured out it was DNA. Where was the definitive answer?

  • Well most of the argument came form is it DNA? Or is it proteins that are actually being

  • transferred? And proteins are very complex. And so most of the people were thinking that

  • it's proteins that was the genetic material. Not DNA. And so the Hershey-Chase experiment,

  • sometimes called the blender experiment, used bacteriophages. And a bacteriophage is simply

  • a virus that infects a bacteria. It looks kind of like lunar lander. It lands on the

  • bacteria. It injects its hereditary material in. And then it hijacks that bacteria to make

  • more of the bacteriophage. And so what Hershey and Chase did, it's a really elegant experiment,

  • is they used two different atoms. They used in one experiment sulfur. And in this case

  • the sulfur is labelled red. They used a red dye to dye the bacteriophages in this experiment.

  • They then infect the bacteria, blend it all up. They precipitate it out and see what color

  • came out. Now why was it important they use sulfur? It's because sulfur is found in proteins

  • but it's not found in DNA. They then used a different dye to dye phosphorus. Phosphorus

  • is found in DNA but it's not found in proteins. And so what they were able to show is that

  • the only one that was doing the transforming was this green dye. That means that it was

  • the phosphorus. And that means that it wasn't proteins that were transferring the information.

  • That it was DNA. And so the Hershey-Chase experiment was definitive proof that DNA was

  • the hereditary material. And so this is in the 50s. And now the race is on to figure

  • out, not only, mostly to figure out what's the structure of DNA. How's it all work. These

  • are interesting people. Apparently Hershey and Chase, they worked together. Their lab

  • was totally silent and they just worked very effectively together. Sadly Martha Chase goes

  • crazy later in life. But a really cool experiment. Now we go to the ones that you're probably

  • familiar with. The names that you're familiar with. And that's probably Watson and Crick.

  • James Watson and Francis Crick are mostly given credit for discovering the structure

  • of DNA. But there were three other, probably even more people that played in this discovery

  • of this structure of DNA. One of those is Maurice Wilkins. Maurice Wilkins was really

  • good at x-ray crystallography. So that is taking pictures of crystalized material. It's

  • kind of like shining light through a chandelier and then figuring out what the structure of

  • the chandelier is. He was working with Rosalind Franklin. They didn't get along that well.

  • And Maurice Wilkins is an interesting guy. Died just a few years ago. They didn't work

  • well together but they had the best data out there. This is a picture of some of the, this

  • would be the x-ray crystallography of DNA. So they were looking at DNA and trying to

  • figure out its structure. If you know anything about crystallography you'd know that this

  • is a helix. Or it suggests the structure of a helix. Actually James Watson sat in on one

  • of Rosalind Franklin's secret meetings and took notes on it. And it actually helped them

  • to figure the structure a lot. Next we've got Erwin Chargaff. Erwin Chargaff was looking

  • at different organisms and studying the amount of As, Ts, Cs and Gs. And so A, G, C and T

  • are the four different bases that are found in DNA. And he found something unique. If

  • you look at for example an octopus, the amount of A, 33.2 and the amount of T is exactly

  • the same, about the same. And if you look at the amount of G, 17.6 and 17.1, that's about the

  • same as well. In other words the amount of A and the amount of T is always the same.

  • And the amount of G and the amount of C is always the same. We sometimes call this Chargaff's

  • Rule. So as you look all the way down here, like in humans, we have 29.3% A and 30% T.

  • Likewise we have 20% G and C. And so he didn't know what that meant, but Crick and Watson

  • knew that. They knew the structure of a helix coming from the work the Franklin and Wilkins.

  • And so they used models to figure out the structure of DNA. Why do we always have the

  • A and the T equal? And the G and C equal? Well if you look at the structure of DNA,

  • you have a backbone. This is actually a model of, this is the model that Watson and Crick

  • were working on. So you've got a backbone that looks like this. But then on the inside

  • you have your bases. And if you have an A on this side, a T will be on the other side.

  • And if you have a C on this side a G will be on the other side. And so the amount of

  • As and the amount of Ts are always equal because they bond to each other. And so this that

  • double helix. So Watson and Crick are given the credit for that. They actually share the

  • Noble prize with Maurice Wilkins. Rosalind Franklin doesn't get the Nobel Prize because

  • sadly she had died before then of cancer. And it was probably as a result of the x-rays

  • that she was using in her lab. And you can't get a Nobel prize if you die. Okay. So let's

  • now go to the structure. Structure of DNA. DNA doesn't just sit loose inside the nucleus.

  • It's organized into something called a chromosome. And so in us, in eukaryotic cells, we have

  • this characteristic shape of a chromosome. If you actually look at how the DNA is organized,

  • the DNA is wrapped around these proteins called histone proteins. And those are swirled around

  • other proteins and other proteins and eventually you get to the structure of the chromosome

  • that looks like this. Now the reason it characteristically looks like an X is that when we take a picture

  • of our chromosomes, this would be a picture of our chromosomes, they're usually in metaphase.

  • And so they usually have this characteristic X structure. What does that mean? That means

  • that the left side is a mirror copy of the right side. And so in a lot of my diagrams,

  • you'll see me drawing it, a chromosome just looking like this. With a centromere in the

  • middle. And that's because that's what a chromes usually looks like. It's a linear stretch.

  • And so in eukaryotic cells we have this long stretch of DNA wrapped around proteins and

  • that's where the genetic material is found. And it's really really really long compared

  • to the size of the actual cell itself. If we look at prokaryotic chromosomes it's different.

  • In a prokaryotic chromosome, the chromosome is simply loose here. It's not in a nucleus

  • at all. And it's also a loop. And so in us, we have a linear chromosome. In other words

  • it's a length with a definite end of either side. But in prokaryotics they've got just

  • a loop. Now the loop is wrapped around itself so it can fit in what's called the nucleoid

  • region of the bacteria. But it's a loop none the less. They also have extra little tiny

  • loops called plasmids. And those have DNA in them as well. And they carry genetic information.

  • And these can actually be swapped between bacteria. So it's like an extra set of genes.

  • Another important difference between us and bacteria is that a lot of our chromosomes

  • is what's called junk DNA. In other words it's DNA that's not actual genes. It's between

  • genes. And if you look at the DNA of a prokaryotic cell, each of those little stretches is going

  • to be one gene after gene after gene after gene. Now we're starting to figure out that

  • it's not really junk DNA. That it actually has an important function. We'll talk about

  • that in a different podcast.

Hi. It's Mr. Andersen and welcome to biology essentials video number 27. This

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DNAとRNA - パート1 (DNA and RNA - Part 1)

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    Cheng-Hong Liu に公開 2021 年 01 月 14 日
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