Breaking to Reveal: The Peroxisome

Question 1

What does microscopy reveal about organelles? What can’t it reveal?

Answer 1

Reveals location, size, and shape, but can’t reveal function

Question 2

What is cell fractionation?

Answer 2

Process to break apart cells and isolate different organelles; bridges microscopy and biochemistry

Question 3

What is differential centrifugation?

Answer 3

a key technique for separating organelles based on mass, shape, size, and density

Question 4

During differential centrifugation, what is the supernatant?

Answer 4

the part of the test tube where the organelle of interest is after centrifugation; composed of lighter cell materials

Question 5

During differential centrifugation, what is the pellet?

Answer 5

the bottom of the test tube after G-force; composed of denser cell materials

Question 6

What is the cytosol?

Answer 6

the soluble part of the cytoplasm; remains of a cell after very high speeds

Question 7

What is the cytoplasm?

Answer 7

substance between the cell’s plasma membrane and the nucleus

Question 8

What is the process of differential centrifugation?

Answer 8

1. Filter homogenate (disrupted cells without clumps) to remove clumps of unbroken cells, connective tissue, etc.
2. Pour out the supernatant, then spin it at higher speeds.

Question 9

What is centrifugation at low speeds called? What speed? What does it separate out?

Answer 9

Clinical centrifugation spins at 600 g x 10 min and filters the nuclei into the pellet.

Question 10

What is centrifugation at medium speeds called? What speed? What does it separate out?

Answer 10

Super centrifugation occurs at 15,000 g x 5 min and filters out the mitochondria, chloroplasts, lysosomes, and peroxisomes.

Question 11

What is centrifugation at high speeds called? What speed? What does it separate out?

Answer 11

Ultraspeed centrifuges spin at 100,000 g x 60 min and separate the plasma membrane, microsomal fraction (fragments of the ER), and large polyribosomes.

Question 12

What is centrifugation at very high speeds called? What speed? What does it separate out?

Answer 12

Ultraspeed centrifuges spin at 300,000 g x 2 h and separate ribosomal subunits, small polyribosomes, and eventually leave behind the cytosol.

Question 13

DNA and RNA have similar S values. Which is more dense?

Answer 13

RNA is more dense, at about 2.0 g/cm^3 compared to 1.7 g/cm^3.

Question 14

What do the relative sedimentation values communicate about centrifugation?

Answer 14

Very different sedimentation values indicate there’s a good chance of separating organelles via centrifugation. Harder to separate them with similar S values.

Question 15

Peroxisomes and mitochondria have the same S-value. Which is more dense?

Answer 15

Peroxisomes are more dense.

Question 16

What does differential centrifugation separate based on?

Answer 16

mass, shape, size, and density

Question 17

What does rate zonal centrifugation separate based on?

Answer 17

S-value (mass and size)

Question 18

What does equilibrium (buoyant) density gradient centrifugation separate based on?

Answer 18

density

Question 19

What does sucrose do in rate-zonal and equilibrium density gradient centrifugation?

Answer 19

Creates a barrier for molecules separated in the centrifuge’s field based on S-value (for rate zonal) and density (for buoyancy)

Question 20

What happens to molecules closest to the bottom of the test tube in rate zonal centrifugation? Why?

Answer 20

They are slowed down due to sucrose’s resistance. There’s a higher sucrose concentration at the bottom of the tube.

Question 21

Which forms of centrifugation have a solute gradient?

Answer 21

rate zonal and equilibrium density gradient centrifugation

Question 22

What are the 3 names for the form of centrifugation that separates based on density?

Answer 22

Equilibrium Density Gradient Centrifugation
Buoyant Density Centrifugation
Isopycnic Separation

Question 23

Why does isopycnic centrifugation separate based on density?

Answer 23

The range of concentration of the sucrose in the tube allows organelles to migrate to an equivalent point of density.

Question 24

What is the density of the lysosome?

Answer 24

1.12 g/cm^3

Question 25

What is the mitochondria’s density?

Answer 25

1.18 g/cm^3

Question 26

What is the peroxisome’s density?

Answer 26

1.23 g/cm^3

Question 27

What are the three potential methods for determining the contents of a cell fraction?

Answer 27

1. Microscopic observation
2. Enzymatic assays for marker enzymes
3. Probing for marker molecules (usually proteins, but non-enzymes)

Question 28

During an enzymatic assay, which enzyme(s) was associated with the lysosome? Where was the fraction found?

Answer 28

Acid phosphatase, found at the top of the tube

Question 29

During an enzymatic assay, which enzyme(s) was associated with the mitochondria? Where was the fraction found?

Answer 29

Cytochrome oxidase, found near bottom of the tube

Question 30

Researchers believed there may have been some spill over from other organelles into the mitochondria’s fraction after finding the cytochrome oxidase. What did they do to confirm they had found the mitochondria’s fraction? What did they discover?

Answer 30

Labeled mitochondrial DNA with 14C. They discovered they had accurately identified the mitochondria because the peak for the DNA was in the same place as the peak for the marker enzyme.

Question 31

During an enzymatic assay, which enzyme(s) was associated with the peroxisome? Where was the fraction found?

Answer 31

Catalase and ureoxidase

Question 32

How was the peroxisome discovered?

Answer 32

During the enzymatic assays after isopycnic centrifugation, ureoxidase was found in the fraction where the lysosome was. This was confusing because the lysosome’s pH was too low for this enzyme to be active there. This indicated the ureoxidase was operating in another organelle.

Question 33

What does SDS do during SDS-PAGE (SDS-Polyacrylamide Gel Electrophoreses)?

Answer 33

Covers the polypeptides, ensuring
1. a uniform charge to mass ratio (imparts negative charge on all protein samples)
2. uniform shape by denaturing polypeptides
After this, the only physical difference between polypeptides is molecular weight.

Question 34

What does SDS-PAGE do?

Answer 34

Ensures the only difference between polypeptides is molecular weight, so they can be separated based on size

Question 35

Describe the process of SDS-PAGE

Answer 35

1. Denature samples with SDS.
2. Place mix of proteins on gel and apply the electric field, causing proteins to move.
3. Stain the gel to visualize the separated bands.

Question 36

Which side of the gel are the larger proteins are in SDS-PAGE?

Answer 36

They are closer to the negative pole. They didn’t move as quickly as smaller particles through the existing holes.

Question 37

What is immnoblotting (Western blotting)?

Answer 37

method for detecting marker proteins in cell fractions after SDS-PAGE, reveals which fraction target organelles are in

Question 38

Describe the process of immunoblotting.

Answer 38

1. Take the SDS poly gel after SDS-PAGE.
2. Apply electric field from the side, moving the proteins out of the gel.
3. To catch proteins, put membrane behind the gel and allow polypeptide to bind to it.
4. Add an antibody to find the target protein on the membrane.
5. Add a secondary antibody with a detectable (fluorescent) molecule to attach to the first antibody

Question 39

What kind of cells have peroxisomes?

Answer 39

virtually all eukaryotic cells

Question 40

What is the diameter of the peroxisome?

Answer 40

between 0.1 and 1 micrometer

Question 41

What is the diameter of the peroxisome based on?

Answer 41

physiological state and growth conditions of the cell

Question 42

How many peroxisomes are inside a cell?

Answer 42

varies

Question 43

Are peroxisomes membrane-bounded or not?

Answer 43

Membrane-bounded

Question 44

What enzymes are present in peroxisomes?

Answer 44

All peroxisomes have catalases.
Some oxidases are in peroxisomes.

Question 45

Peroxisomes may have a crystalline form? Under what conditions does it form?

Answer 45

Non-primate cells that have a high concentration of ureoxidase crystallize.

Question 46

Describe peroxisome’s relationship to O2 utilization.

Answer 46

The peroxisome is the first organism that utilized atmospheric oxygen when O2 levels rose on earth. The peroxisome reduced O2 to protect cells from oxidative damage.

Question 47

Why do people believe the peroxisome is less important now?

Answer 47

After the evolution of the mitochondria, the mitochondria began reducing O2 and coupled the redox reaction to ATP production, which the peroxisome could not do.

Question 48

What are the five functions of the peroxisome?

Answer 48

1. Hydrogen peroxide metabolism
2. Catabolism of unusual molecules
3. Metabolism of nitrogen-containing compounds
4. Detoxification of organic compounds and reactive oxygen species (radicals)
5. Beta-oxidation of fatty acids

Question 49

Which enzyme forms hydrogen peroxide? When does that occur?

Answer 49

Oxidase forms hydrogen peroxide as a byproduct when utilizing O2.

Question 50

Which enzyme metabolizes hydrogen peroxide?

Answer 50

Catalase in the peroxisome metabolizes hydrogen peroxide into water and O2.

Question 51

Which unusual molecules are catabolized by the peroxisome?

Answer 51

D-amino acids
Xenobiotics

Question 52

If a compound contains nitrogen, what will likely happen to it?

Answer 52

Will be metabolized by the peroxisome

Question 53

Which kinds of molecules are detoxified by the peroxisome?

Answer 53

Organic compounds (ex. aldehydes, ethanol) and reactive oxygen species (hydrogen peroxide, radicals)

Question 54

Why is it necessary for the peroxisome to destroy reactive oxygen species?

Answer 54

to prevent oxidative stress

Question 55

Which enzyme is responsible for detoxifying organic compounds?

Answer 55

catalase

Question 56

What does the beta-oxidation of fatty acids do?

Answer 56

Shortens long fatty acid chains over time and produces acetyl CoA

Question 57

What happens to the acetyl CoA that is produced after the beta-oxidation of fatty acids in the peroxisome?

Answer 57

either anabolism or used in the TCA cycle as energy (building block of lipids)