1. Chapter 16 The Molecular Basis of Inheritance

2. Determining the Chemical Composition of DNA After Morgan determined that genes were on chromosomes, scientists began wondering what they were made of. Early on, scientists thought they were made of proteins because they were large and structurally sound. Nucleic acids were deemed too simple to carry out the complex tasks chromosomes required. After Morgan determined that genes were on chromosomes, scientists began wondering what they were made of. Early on, scientists thought they were made of proteins because they were large and structurally sound. Nucleic acids were deemed too simple to carry out the complex tasks chromosomes required.

3. Determining the Chemical Composition of DNA As scientists continued their experiments with viruses and bacteria, many results were observed that gave support to the notion that DNA was the hereditary material. A classic experiment demonstrated the genetic role of DNA. As scientists continued their experiments with viruses and bacteria, many results were observed that gave support to the notion that DNA was the hereditary material. A classic experiment demonstrated the genetic role of DNA.

4. Frederick Griffith Studied the bacterium that caused pneumonia--S. pneumonia. Worked with two strains: pathogenic and non-pathogenic. Studied the bacterium that caused pneumonia--S. pneumonia. Worked with two strains: pathogenic and non-pathogenic.

5. Frederick Griffith An experimental overview: (S) smooth cells produce mucous capsules that protect the bacteria from an organism’s immune system--pathogenic. (R) rough cells have no mucous capsule and are attacked by an organism’s immune system--non pathogenic. An experimental overview: (S) smooth cells produce mucous capsules that protect the bacteria from an organism’s immune system--pathogenic. (R) rough cells have no mucous capsule and are attacked by an organism’s immune system--non pathogenic.

6. Frederick Griffith, His Experiment Mixed heat-killed pathogenic (S) bacteria with living non-pathogenic (R) bacteria, the non-pathogenic (R) bacteria began producing the mucous capsule and became pathogenic (S). The new bacteria that arose from the bacteria were somehow transformed into pathogenic S. pneumonia. Griffith called this process transformation. Mixed heat-killed pathogenic (S) bacteria with living non-pathogenic (R) bacteria, the non-pathogenic (R) bacteria began producing the mucous capsule and became pathogenic (S). The new bacteria that arose from the bacteria were somehow transformed into pathogenic S. pneumonia. Griffith called this process transformation.

7. Frederick Griffith, His Experiment

8. Griffith’s Transformation Experiment Did not identify DNA as the transforming factor, but it set the stage for other experiments.

9. Oswaldt Avery Avery worked for a long time trying to identify the transforming factor. After isolating and purifying numerous macromolecules from the heat killed pathogenic bacteria he and his colleagues could only get DNA to work. The prevailing beliefs about proteins vs. DNA continued to generate skepticism. Avery worked for a long time trying to identify the transforming factor. After isolating and purifying numerous macromolecules from the heat killed pathogenic bacteria he and his colleagues could only get DNA to work. The prevailing beliefs about proteins vs. DNA continued to generate skepticism.

10. T2 Phage Reproduction Movie

11. The Hershey-Chase Experiment In 1952, Alfred Hershey and Martha Chase performed experiments with viruses showing that DNA is genetic material. Viruses (aka phages) are DNA or RNA wrapped in a protein. E. coli is a bacteria that is often used in experiments. In 1952, Alfred Hershey and Martha Chase performed experiments with viruses showing that DNA is genetic material. Viruses (aka phages) are DNA or RNA wrapped in a protein. E. coli is a bacteria that is often used in experiments.

12. The Hershey-Chase Experiment Used the T2 phage because it was generally accepted to be DNA wrapped in protein. Used E. coli because it was easily obtainable and was readily attacked by T2. Had to demonstrate whether or it was DNA or protein that was the hereditary factor. Used the T2 phage because it was generally accepted to be DNA wrapped in protein. Used E. coli because it was easily obtainable and was readily attacked by T2. Had to demonstrate whether or it was DNA or protein that was the hereditary factor.

13. The Hershey-Chase Experiment Their experiment demonstrated which part of the T2 entered the E. coli. They grew T2 in the presence of radioactive sulfur--proteins contain sulfur, DNA does not. Next, they grew the T2 in a separate batch of radioactive phosphorous. The DNA of T2 contains phosphorous--the proteins do not. Their experiment demonstrated which part of the T2 entered the E. coli. They grew T2 in the presence of radioactive sulfur--proteins contain sulfur, DNA does not. Next, they grew the T2 in a separate batch of radioactive phosphorous. The DNA of T2 contains phosphorous--the proteins do not.

14. The Hershey-Chase Experiment The scientists now had 2 batches of T2, one labeled with radioactive sulfur and one labeled with radioactive phosphorous. These 2 batches were separately incubated with non-radioactive samples of E. coli and analyzed shortly after infection. The scientists now had 2 batches of T2, one labeled with radioactive sulfur and one labeled with radioactive phosphorous. These 2 batches were separately incubated with non-radioactive samples of E. coli and analyzed shortly after infection.

15. The Hershey-Chase Experiment Shortly after infection, the E. coli samples were spun in a blender to knock off loose parts of T2. The mixtures were then spun in high speed centrifuges for a long time to separate out various parts of the mixture. At the bottom of the tube was a pellet of E. coli. Shortly after infection, the E. coli samples were spun in a blender to knock off loose parts of T2. The mixtures were then spun in high speed centrifuges for a long time to separate out various parts of the mixture. At the bottom of the tube was a pellet of E. coli.

16. The Hershey-Chase Experiment The pellet was examined for radioactivity and radioactive phosphorous was found. The supernatant was analyzed and a lot of radioactive sulfur was found, but no radioactive phosphorous. This indicates that the DNA got into the E. coli and was in the pellet The protein did not get into the bacteria and was left in the supernatant. The pellet was examined for radioactivity and radioactive phosphorous was found. The supernatant was analyzed and a lot of radioactive sulfur was found, but no radioactive phosphorous. This indicates that the DNA got into the E. coli and was in the pellet The protein did not get into the bacteria and was left in the supernatant.

17. The Hershey-Chase Experiment Furthermore, when the bacteria in the pellet were plated on culture medium, they produced more T2 containing radioactive phosphorous.

21. The Hershey-Chase Experiment They concluded: That the virus injects DNA into the E. coli and it is the genetic material that programs the cells to produce new T2 phages. The protein stays outside. This experiment provided firm evidence that DNA was the hereditary material and not protein. They concluded: That the virus injects DNA into the E. coli and it is the genetic material that programs the cells to produce new T2 phages. The protein stays outside. This experiment provided firm evidence that DNA was the hereditary material and not protein.

22. The Hershey-Chase Experiment Movie

23. Erwin Chargaff’s Experiment It provided more evidence that DNA was the genetic material. He abolished the notion that DNA was not complex enough to comprise hereditary material. Chargaff showed the diversity of the DNA molecule and that its composition varied from organism to organism. It provided more evidence that DNA was the genetic material. He abolished the notion that DNA was not complex enough to comprise hereditary material. Chargaff showed the diversity of the DNA molecule and that its composition varied from organism to organism.

24. Erwin Chargaff’s Experiment He discovered that the amount of adenine is equal to the amount of thymine and cytosine equaled the amount of guanine. Chargaff did not know what all of this meant, but after the elucidation of the shape of the DNA molecule, these became known as Chargaff’s Rules. He discovered that the amount of adenine is equal to the amount of thymine and cytosine equaled the amount of guanine. Chargaff did not know what all of this meant, but after the elucidation of the shape of the DNA molecule, these became known as Chargaff’s Rules.

25. Watson and Crick In 1953, James Watson and Francis Crick visited a lab of Maurice Wilkins. Examined an X-ray diffraction image of DNA produced by Rosalind Franklin. Their familiarity with such diffraction patterns allowed them to quickly deduce that DNA consisted of 2 strands and was helical in shape. In 1953, James Watson and Francis Crick visited a lab of Maurice Wilkins. Examined an X-ray diffraction image of DNA produced by Rosalind Franklin. Their familiarity with such diffraction patterns allowed them to quickly deduce that DNA consisted of 2 strands and was helical in shape.

26. Watson and Crick Through trial and error they concluded A paired with T and C with G. This gave the uniform width they determined from the work of Franklin and explained Chargaff’s findings. They explained the base paring rules, the shape and the width of the DNA and showed that none of this was dependent on the sequence of the nucleotides. Thus, the DNA could be put together an infinite number of ways. Through trial and error they concluded A paired with T and C with G. This gave the uniform width they determined from the work of Franklin and explained Chargaff’s findings. They explained the base paring rules, the shape and the width of the DNA and showed that none of this was dependent on the sequence of the nucleotides. Thus, the DNA could be put together an infinite number of ways.

27. Watson and Crick The question now arose for how DNA was replicated. The strands are said to be complimentary to each other. That is, they contain the information necessary to reconstruct each other. But how? The question now arose for how DNA was replicated. The strands are said to be complimentary to each other. That is, they contain the information necessary to reconstruct each other. But how?

28. Watson and Crick These men proposed a semiconservative model in which the new DNA strand formed contained 1/2 of the original DNA and 1/2 newly synthesized DNA--one strand was original and one strand was new. They couldn’t rule out a model where somehow the old DNA stayed together and the newly synthesized DNA strand was completely new. These men proposed a semiconservative model in which the new DNA strand formed contained 1/2 of the original DNA and 1/2 newly synthesized DNA--one strand was original and one strand was new. They couldn’t rule out a model where somehow the old DNA stayed together and the newly synthesized DNA strand was completely new.

29. Watson and Crick Additionally, they could not rule out a dispersive model where both strands of DNA consisted of old and new DNA. The mechanisms for these three models were difficult to elucidate but Matthew Meselson and Franklin Stahl developed experiments to test them. Additionally, they could not rule out a dispersive model where both strands of DNA consisted of old and new DNA. The mechanisms for these three models were difficult to elucidate but Matthew Meselson and Franklin Stahl developed experiments to test them.

30. The Meselson-Stahl Experiment E. coli cells were cultured in a medium containing heavy nitrogen, 15 N. After several generations the bacteria were transferred into a medium containing normal nitrogen, 14 N. Ideally, all DNA synthesized the first time through contained heavy nitrogen. All DNA synthesized in the normal nitrogen tube (after the transfer) would be lighter than the DNA from the original culture. E. coli cells were cultured in a medium containing heavy nitrogen, 15 N. After several generations the bacteria were transferred into a medium containing normal nitrogen, 14 N. Ideally, all DNA synthesized the first time through contained heavy nitrogen. All DNA synthesized in the normal nitrogen tube (after the transfer) would be lighter than the DNA from the original culture.

31. The Meselson-Stahl Experiment Their hypotheses: (what would be seen after centrifuging the tubes containing DNA) If replication followed the conservative model, the first replication would contain 2 bands of DNA, one light and one heavy; and the 2nd replication would show the same thing (2 bands). Their hypotheses: (what would be seen after centrifuging the tubes containing DNA) If replication followed the conservative model, the first replication would contain 2 bands of DNA, one light and one heavy; and the 2nd replication would show the same thing (2 bands).

32. The Meselson-Stahl Experiment Their hypotheses: (what would be seen after centrifuging the tubes containing DNA) If it followed the dispersive model, one band would be seen containing hybrid DNA. This was seen after the first replication, but not the second*. Their hypotheses: (what would be seen after centrifuging the tubes containing DNA) If it followed the dispersive model, one band would be seen containing hybrid DNA. This was seen after the first replication, but not the second*.

33. The Meselson-Stahl Experiment Their hypotheses: (what would be seen after centrifuging the tubes containing DNA) If it followed the semiconservative model one band would be seen after the first replication and 2 would be seen after the 2nd replication. Their hypotheses: (what would be seen after centrifuging the tubes containing DNA) If it followed the semiconservative model one band would be seen after the first replication and 2 would be seen after the 2nd replication.

35. The Meselson-Stahl Experiment After they transferred the DNA from the 15 N tube to the 14 N tube, they waited 20 minutes (1 replication) and then centrifuged the tube. They were able to detect one band in the centrifuge tube. In a separate tube, they waited for 2 rounds of replication (40 min.) and were able to detect 2 bands in the centrifuge tube. After they transferred the DNA from the 15 N tube to the 14 N tube, they waited 20 minutes (1 replication) and then centrifuged the tube. They were able to detect one band in the centrifuge tube. In a separate tube, they waited for 2 rounds of replication (40 min.) and were able to detect 2 bands in the centrifuge tube.

37. The Meselson-Stahl Experiment Conclusion: The semiconservative model was followed. A light band was detected following the 1st replication and 2 bands, (one light and one heavy) were detected following the 2nd replication. Conclusion: The semiconservative model was followed. A light band was detected following the 1st replication and 2 bands, (one light and one heavy) were detected following the 2nd replication.

38. DNA Replication Movie

39. DNA Replication Begins at a site called the origin of replication. Prokaryotes have one origin of replication. Eukaryotes have hundreds of thousands of origins of replication. Begins at a site called the origin of replication. Prokaryotes have one origin of replication. Eukaryotes have hundreds of thousands of origins of replication.

40. DNA Replication Here is an electron micrograph and a schematic representation of bacterial DNA replication.

41. DNA Replication Primers are the short nucleotide fragments (DNA or RNA) with an available free 3’ end to which DNA polymerase III (DNA pol III) will add nucleotides according to the base paring rules. Primase is the enzyme that starts an RNA chain from scratch creating a primer that can initiate the synthesis of a new DNA strand. Primers are the short nucleotide fragments (DNA or RNA) with an available free 3’ end to which DNA polymerase III (DNA pol III) will add nucleotides according to the base paring rules. Primase is the enzyme that starts an RNA chain from scratch creating a primer that can initiate the synthesis of a new DNA strand.

43. DNA Replication The leading strand of DNA synthesis only needs one primer. The lagging strand needs a new primer for each Okazaki fragment added to the growing strand. The leading strand of DNA synthesis only needs one primer. The lagging strand needs a new primer for each Okazaki fragment added to the growing strand.

44. DNA Replication DNA polymerases are enzymes that catalyze the elongation of DNA at the replication fork. One by one, nucleotides are added by DNA polymerase to the growing end of the DNA strand--the free 3’ end. DNA always grows 5’- ->3’ adding to the free 3’ end. DNA polymerases are enzymes that catalyze the elongation of DNA at the replication fork. One by one, nucleotides are added by DNA polymerase to the growing end of the DNA strand--the free 3’ end. DNA always grows 5’- ->3’ adding to the free 3’ end.

46. DNA Replication The 2 strands of the DNA are antiparallel, they are oriented in opposite directions. This poses replication problems. DNA polymerase only adds nucleotides to the free 3’ end. Thus, it can only elongate in the 5’-->3’ direction. You get what is known as a leading strand and a lagging strand. The 2 strands of the DNA are antiparallel, they are oriented in opposite directions. This poses replication problems. DNA polymerase only adds nucleotides to the free 3’ end. Thus, it can only elongate in the 5’-->3’ direction. You get what is known as a leading strand and a lagging strand.

47. DNA Replication Along the leading strand, DNA pol III synthesizes a complementary strand continuously in the 5’-->3’ direction.

48. Leading Strand Movie

49. DNA Replication Along what is known as the lagging strand, DNA pol III synthesizes the new DNA strand in the 5’-->3’ direction in a series of segments known as Okazaki fragments which form as the replication fork opens up.

50. DNA Replication The opening of the fork allows the DNA pol III to hop from one fragment to the next on the lagging strand template and synthesize more DNA. These fragments are spliced together by DNA ligase forming a single strand. The opening of the fork allows the DNA pol III to hop from one fragment to the next on the lagging strand template and synthesize more DNA. These fragments are spliced together by DNA ligase forming a single strand.

51. Lagging Strand Movie

53. DNA Replication As we said earlier, primase works to join RNA nucleotides together creating primers complementary to the DNA template strand. This is the site of initiation, and new DNA strands will be synthesized here. When cellular DNA is replicated, the primer is a short stretch of RNA with a free 3’ end. As we said earlier, primase works to join RNA nucleotides together creating primers complementary to the DNA template strand. This is the site of initiation, and new DNA strands will be synthesized here. When cellular DNA is replicated, the primer is a short stretch of RNA with a free 3’ end.

54. DNA Replication DNA pol I functions to replace the RNA nucleotide primers with DNA. All of the nucleotides of the RNA primer are replaced by DNA pol I. DNA ligase joins the gap left between the last two nucleotides joining all of the Okazaki fragments into one continuous strand. DNA pol I functions to replace the RNA nucleotide primers with DNA. All of the nucleotides of the RNA primer are replaced by DNA pol I. DNA ligase joins the gap left between the last two nucleotides joining all of the Okazaki fragments into one continuous strand.

55. DNA Replication Helicase is the enzyme responsible for untwisting the double helix at the replication fork. This separates the parental strands of DNA making them available for use as template strands. Helicase is the enzyme responsible for untwisting the double helix at the replication fork. This separates the parental strands of DNA making them available for use as template strands.

56. DNA Replication This untwisting actually causes a greater amount of twisting ahead of the replication fork, and an enzyme called topoisomerase helps to reduce this twisting.

57. DNA Replication After helicase separates the two parental strands, single strand binding protein binds to the DNA strands stabilizing them until new DNA synthesis occurs.

58. DNA Replication Keep in mind that all of the molecules described in the replication process actually work together to maximize DNA production. Think of them as the individual parts of a “DNA synthesis machine.” Keep in mind that all of the molecules described in the replication process actually work together to maximize DNA production. Think of them as the individual parts of a “DNA synthesis machine.”

59. DNA Replication The main importance of replicating the DNA is the ability to do it without error. Errors in completed eukaryotic DNA occur in approximately 1 in 10 billion nucleotides. Initial errors occur at a rate of about 1 in 100,000. Proofreading mechanisms by DNA polymerase fix many of the problems. The main importance of replicating the DNA is the ability to do it without error. Errors in completed eukaryotic DNA occur in approximately 1 in 10 billion nucleotides. Initial errors occur at a rate of about 1 in 100,000. Proofreading mechanisms by DNA polymerase fix many of the problems.

60. DNA Replication If an error escapes proofreading, they are often fixed by special enzymes within the cell-- but even these are not 100% effective at removing all errors. Additionally, some errors occur after DNA synthesis has been completed. If an error escapes proofreading, they are often fixed by special enzymes within the cell-- but even these are not 100% effective at removing all errors. Additionally, some errors occur after DNA synthesis has been completed.

61. DNA Replication Overview Movie

62. Excision Repair Errors that occur as a result of the environment (radiation, chemicals, X-rays, etc.) can often be fixed by DNA polymerase and ligase. This is a way the cell tries (usually effectively) to fix problems before they get perpetuated (cancer). Errors that occur as a result of the environment (radiation, chemicals, X-rays, etc.) can often be fixed by DNA polymerase and ligase. This is a way the cell tries (usually effectively) to fix problems before they get perpetuated (cancer).

63. Telomeres When we get to the end of the chromosome, we encounter what are known as telomeres, and they create a problem for linear DNA. At the end of the lagging strand, when the RNA primer is removed, there is no free 3’ end to which nucleotides can be added. Telomeres consist of multiple repetitions of one short nucleotide sequence. When we get to the end of the chromosome, we encounter what are known as telomeres, and they create a problem for linear DNA. At the end of the lagging strand, when the RNA primer is removed, there is no free 3’ end to which nucleotides can be added. Telomeres consist of multiple repetitions of one short nucleotide sequence.

65. Telomeres This helps protect the DNA from multiple rounds of DNA synthesis and postpone the erosion of genes near the end of the DNA molecule. Thus, successive rounds of DNA synthesis would result in shorter and shorter DNA molecules. This helps protect the DNA from multiple rounds of DNA synthesis and postpone the erosion of genes near the end of the DNA molecule. Thus, successive rounds of DNA synthesis would result in shorter and shorter DNA molecules.

67. Telomeres This is okay in somatic cells where cell division is somewhat limited. In gametes, however, it is necessary to preserve the genetic complement. This is okay in somatic cells where cell division is somewhat limited. In gametes, however, it is necessary to preserve the genetic complement.

68. Telomeres Cells do this using an enzyme called telomerase. This enzyme catalyzes the length of the germ cell telomeres thus preserving the amount of DNA. Cells do this using an enzyme called telomerase. This enzyme catalyzes the length of the germ cell telomeres thus preserving the amount of DNA.

70. Telomerases Telomerases act to elongate the DNA of human gametes which would become progressively shorter during successive rounds of DNA synthesis. Eventually, the germ cells’ telomeres would become so short that the genes would become eroded and the cell would begin to lose genes. Telomerases act to elongate the DNA of human gametes which would become progressively shorter during successive rounds of DNA synthesis. Eventually, the germ cells’ telomeres would become so short that the genes would become eroded and the cell would begin to lose genes.